US20150240261A1 - RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX - Google Patents
RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX Download PDFInfo
- Publication number
- US20150240261A1 US20150240261A1 US14/683,443 US201514683443A US2015240261A1 US 20150240261 A1 US20150240261 A1 US 20150240261A1 US 201514683443 A US201514683443 A US 201514683443A US 2015240261 A1 US2015240261 A1 US 2015240261A1
- Authority
- US
- United States
- Prior art keywords
- cas9
- crrna
- dna
- complex
- cleavage
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Abandoned
Links
Images
Classifications
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N15/00—Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
- C12N15/09—Recombinant DNA-technology
- C12N15/11—DNA or RNA fragments; Modified forms thereof; Non-coding nucleic acids having a biological activity
- C12N15/113—Non-coding nucleic acids modulating the expression of genes, e.g. antisense oligonucleotides; Antisense DNA or RNA; Triplex- forming oligonucleotides; Catalytic nucleic acids, e.g. ribozymes; Nucleic acids used in co-suppression or gene silencing
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N15/00—Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
- C12N15/09—Recombinant DNA-technology
- C12N15/10—Processes for the isolation, preparation or purification of DNA or RNA
- C12N15/102—Mutagenizing nucleic acids
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N15/00—Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
- C12N15/09—Recombinant DNA-technology
- C12N15/87—Introduction of foreign genetic material using processes not otherwise provided for, e.g. co-transformation
- C12N15/90—Stable introduction of foreign DNA into chromosome
- C12N15/902—Stable introduction of foreign DNA into chromosome using homologous recombination
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N15/00—Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
- C12N15/09—Recombinant DNA-technology
- C12N15/87—Introduction of foreign genetic material using processes not otherwise provided for, e.g. co-transformation
- C12N15/90—Stable introduction of foreign DNA into chromosome
- C12N15/902—Stable introduction of foreign DNA into chromosome using homologous recombination
- C12N15/907—Stable introduction of foreign DNA into chromosome using homologous recombination in mammalian cells
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N9/00—Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
- C12N9/14—Hydrolases (3)
- C12N9/16—Hydrolases (3) acting on ester bonds (3.1)
- C12N9/22—Ribonucleases RNAses, DNAses
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12P—FERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIRED CHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERS FROM A RACEMIC MIXTURE
- C12P19/00—Preparation of compounds containing saccharide radicals
- C12P19/26—Preparation of nitrogen-containing carbohydrates
- C12P19/28—N-glycosides
- C12P19/30—Nucleotides
- C12P19/34—Polynucleotides, e.g. nucleic acids, oligoribonucleotides
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12Q—MEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
- C12Q1/00—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
- C12Q1/68—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
- C12Q1/6811—Selection methods for production or design of target specific oligonucleotides or binding molecules
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N2310/00—Structure or type of the nucleic acid
- C12N2310/10—Type of nucleic acid
- C12N2310/12—Type of nucleic acid catalytic nucleic acids, e.g. ribozymes
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N2310/00—Structure or type of the nucleic acid
- C12N2310/10—Type of nucleic acid
- C12N2310/14—Type of nucleic acid interfering N.A.
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N2310/00—Structure or type of the nucleic acid
- C12N2310/10—Type of nucleic acid
- C12N2310/20—Type of nucleic acid involving clustered regularly interspaced short palindromic repeats [CRISPRs]
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N2310/00—Structure or type of the nucleic acid
- C12N2310/30—Chemical structure
- C12N2310/35—Nature of the modification
- C12N2310/351—Conjugate
- C12N2310/3513—Protein; Peptide
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N2310/00—Structure or type of the nucleic acid
- C12N2310/50—Physical structure
- C12N2310/53—Physical structure partially self-complementary or closed
- C12N2310/531—Stem-loop; Hairpin
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N2320/00—Applications; Uses
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N2800/00—Nucleic acids vectors
- C12N2800/80—Vectors containing sites for inducing double-stranded breaks, e.g. meganuclease restriction sites
Definitions
- CRISPR Clustered Regularly Interspaced Short Palindromic Repeats
- cas CRISPR-associated genes comprise an adaptive immune system that provides acquired resistance against invading foreign nucleic acids in bacteria and archaea (Barrangou et al., 2007. Science 315:1709-12).
- CRISPR consists of arrays of short conserved repeat sequences interspaced by unique variable DNA sequences of similar size called spacers, which often originate from phage or plasmid DNA (Barrangou et al., 2007. Science 315:1709-12; Bolotin et al., 2005. Microbiology 151:2551-61; Mojica et al., 2005. J Mol Evol 60:174-82).
- the CRISPR-Cas system functions by acquiring short pieces of foreign DNA (spacers) which are inserted into the CRISPR region and provide immunity against subsequent exposures to phages and plasmids that carry matching sequences (Barrangou et al., 2007. Science 315:1709-12; Brouns et al., 2008. Science 321: 960-4)
- the CRISPR-Cas immunity is generally carried out through three stages, referred to as i) adaptation/immunization/spacer acquisition, ii) CRISPR expression/crRNA biogenesis, iii) interference/immunity. (Horvath & Barrangou, 2010. Science 327:167-70; Deveau et al., 2010. Annu Rev Microbiol.
- CRISPR-Cas systems are categorized into three major types, which are further subdivided into ten subtypes, based on core element content and sequences (Makarova et al., 2011. Nat Rev Microbiol 9:467-77).
- the structural organization and function of nucleoprotein complexes involved in crRNA-mediated silencing of foreign nucleic acids differ between distinct CRISPR/Cas types (Wiedenheft et al., 2012. Nature 482:331-338).
- Cascade CRISPR-associated complex for antiviral defence
- RNP complexes involved in DNA silencing by Type II CRISPR/Cas systems more specifically in the CRISPR3/Cas system of Streptococcus thermophilus DGCC7710 (Horvath & Barrangou, 2010. Science 327:167-70), consists of four cas genes cas9, cas1, cas2, and csn2, that are located upstream of 12 repeat-spacer units ( FIG. 1A ).
- Cas9 (formerly named cas5 or csn1) is the signature gene for Type II systems (Makarova et al., 2011. Nat Rev Microbiol 9:467-77). In the closely related S.
- thermophilus CRISPR1/Cas system disruption of cas9 abolishes crRNA-mediated DNA interference (Barrangou et al., 2007. Science 315:1709-12).
- S. thermophilus CRISPR3/Cas system can be transferred into Escherichia coli, and that this heterologous system provides protection against plasmid transformation and phage infection, de novo (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82).
- the interference against phage and plasmid DNA provided by S.
- thermophilus CRISPR3 requires the presence, within the target DNA, of a proto-spacer sequence complementary to the spacer-derived crRNA, and a conserved PAM (Proto-spacer Adjacent Motif) sequence, NGGNG, located immediately downstream the proto-spacer (Deveau et al., 2008. J Bacteriol 190:1390-400; Horvath et al., 2008. J Bacteriol 190:1401-12; Mojica et al., 2009. Microbiology 155:733-40). Single point mutations in the PAM or defined proto-spacer positions allow the phages or plasmids to circumvent CRISPR-mediated immunity (Deveau et al., 2008.
- cas9 is the sole cas gene necessary for CRISPR-encoded interference (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82), suggesting that this protein is involved in crRNA processing and/or crRNA-mediated silencing of invasive DNA.
- Cas9 of S. thermophilus CRISPR3/Cas system is a large multi-domain protein comprised of 1,409 aa residues (Sapranauskas et al., 2011.
- Nucleic Acids Res 39:9275-82 It contains two nuclease domains, a RuvC-like nuclease domain near the amino terminus, and a HNH-like nuclease domain in the middle of the protein. Mutational analysis has established that interference provided in vivo by Cas9 requires both the RuvC- and HNH-motifs (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82).
- the method includes incubating under suitable conditions a composition that includes a target double stranded polydeoxynucleotide or single stranded polydeoxynucleotide; wherein a double stranded polydeoxynucleotide contains a short proto-spacer adjacent motif (PAM), which is non-obligatory for a single stranded polydeoxynucleotide; and where PAM comprises a 5′-NGGNG-3′ sequence; a polyribonucleotide (crRNA) comprising a 3′ and 5′ regions wherein the 3′ region comprises at least 22 nt of the repeat present in a microbe containing CRISPR locus and 5′-region comprises of at least 20 nt of the spacer sequence immediately downstream of the repeat in the CRISPR locus, which is substantially complementary, optionally complementary, to a portion of the target polynucleotide, a polypeptide wherein the amino acid sequence of polypeptide and amino acid sequence of SEQ ID
- thermophilus or genetically modified microorganism, including a genetically modified E. coli, or wherein the polypeptide is produced by a method selected from recombinant DNA technology or chemical synthesis; a polyribonucleotide tracrRNA of nucleotide sequence SEQ ID NO: 5 (or have at least 80% identity) comprising a 5′ and 3′ regions wherein the 5′ region is comprised of at least 22 nucleotides is complementary to the 22 nucleotides 3′ region of crRNA, and 3′ region.
- polyribonucleotides are produced by in vitro transcription or chemical synthesis.
- suitable conditions means conditions in vitro or in vivo where reaction might occur.
- a method for the conversion of Cas9 polypeptide into a nickase, cleaving only one strand of double-stranded DNA, by inactivating one of the active sites (RuvC or HNH) in the polypeptide by at least on point mutation, exemplified by D31A (SEQ ID NO: 2), N891A (SEQ ID NO: 3) and H868A (SEQ ID NO: 4) point mutations, is provided.
- RuvC motif mutant cleaves only bottom DNA strand in respect to 5′NGGNG-3′ motif, while HNH motif mutant cleaves top strand.
- Polypeptide-polyribonucleotides complex might be isolated from a genetically modified microbe (for example Escherichia coli or Streptoccocus thermophilus ), or assembled in vitro from separate components.
- a genetically modified microbe for example Escherichia coli or Streptoccocus thermophilus
- components of the complex might be encoded on the one, two or three separate plasmids containing host promoters of the genetically modified microbe or promoters from a native host genome.
- a method for assembly of active polypeptide-polyribonucleotides complex in vitro comprising incubating the components of the complex under conditions suitable for complex assembly is provided.
- the complex might be assembled using three or four components.
- Method for three components assembly comprises incubating the Cas9 polypeptide, 78 nt tracrRNA polyribonucleotide (SEQ ID NO: 5), and 42 nt crRNA polyribonucleotide (5′-NNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNGUUUUAGAGCUGUGUUGUUUCG-3′) (SEQ ID NO: 15) under conditions suitable for complex assembly.
- Method for four components assembly comprises incubating the Cas9 polypeptide; 102 nt tracrRNA polyribonucleotide (SEQ ID NO: 6); polyribonucleotide containing sequence 5′-NNNNNNNNNNNNNNNNNNNNNNGUUUUAGAGCUGUGUUGUUUCG-3′ (SEQ ID NO: 15) and flanking regions and RNase III polypeptide, cleaving double stranded RNA polynucleotide.
- polyribonucleotide containing sequence 5′-NNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNGUUUUAGAGCUGUGUUGUUUCG-3′ are SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11 and SEQ ID NO: 12).
- source for suitable RNaseIII include Escherichia coli or Streptococcus thermophilus.
- a method for re-programming of a Cas9-crRNA complex specificity by mixing separate components or using a cassette containing a single repeat-spacer-repeat unit is provided. Any sequence might be inserted between two repeats in the cassette using suitable restriction endonucleases.
- Cassette might be used to target sequences in vivo, or to produce RNA ribonucleotide suitable for complex assembly in vitro.
- FIG. 1 shows Cas9 protein co-purifies with crRNA.
- A Schematic representation of CRISPR3/Cas system of S. thermophilus.
- cas genes cas9, cas1, cas2, csn2
- cas1, cas2, csn2 cas1, cas2, csn2
- R repeat
- S1-S12 unique spacers
- the tracrRNA required for crRNA maturation in Type II CRISPR systems (Deltcheva et al., 2011. Nature 471:602-7), is located upstream the cas9 gene and encoded on the opposite DNA strand (showed by an arrow) in respect to the other elements of CRISPR3/Cas system.
- FIG. 1 Schematic representation of heterologous loci in two plasmids used for the co-expression of the Cas9-crRNA complex.
- E. coli RR1 strain contained pCas9( ⁇ )1SP (encoding Cas1, Cas2, Csn2, SP1 and tracrRNA) and pASKIBA-Cas9 (encoding Strep-tagged version of Cas9) plasmids.
- C Northern analysis of Cas9-crRNA complexes using anti-crDNA oligonucleotide as a probe.
- FIG. 2 shows DNA cleavage by Cas9-crRNA complexes obtained by Cas9 co-expression with full length CRISPR locus.
- A Schematic representation of CRISPR/Cas locus of recombinant pCas9( ⁇ ) plasmid carrying indigenous 12 spacer-repeat array of SthCRISPR3/Cas system and pASKIBA-Cas9 plasmid carrying cas9 gene with a Strep-tag at the C-terminus.
- B Oligoduplex cleavage assay. Both pCas9( ⁇ ) and pASKIBA-Cas9 plasmids were co-expressed in E.
- FIG. 3 shows immunity against plasmid transformation in E. coli cells provided by the SthCRISPR3/Cas system.
- A Schematic representation of CRISPR/Cas locus of recombinant plasmid pCRISPR3 carrying indigenous 12 spacer-repeat array of SthCRISPR3/Cas system and engineered pCRISPR3-SP1 plasmid carrying 1 spacer-repeat unit.
- B Interference of plasmid transformation by SthCRISPR3/Cas system in E. coli cells.
- FIG. 4 shows comparison of Type IIA CRISPR/Cas systems from S. thermophilus DGCC7710, LMD-9 and S. pyogenes SF370 strains.
- A Schematic organization of the CRISPR/Cas systems. Nucleotide sequences corresponding to the tracrRNA required for the crRNA maturation in of S. pyogenes (2) are present in LMD-9 and DGCC7710. Percentage of identical and similar (in parenthesis) residues between corresponding protein sequences that are connected by dashed lines.
- B Alignment of the conserved repeat sequences and tracrRNA. Corresponding sequences from DGCC7710 and LMD-9 are identical.
- Nucleotide positions which are identical in all three strains are labeled with an asterisk below aligned sequences.
- B discloses SEQ ID NOS 50, 50-52, and 52-53, respectively, in order of appearance.
- C Comparison of crRNA sequences. The sequence and length of S. pyogenes crRNA was determined by deep sequencing analysis (2). The approximate length of crRNA from S. thermophilus LMD-9 (2) and DGCC7710 (this work) strains were determined by the northern blot analysis.
- C discloses SEQ ID NOS 54-56, respectively, in order of appearance.
- FIG. 5 shows Cas9-crRNA complex cleaves in vitro double-stranded DNA within a proto-spacer.
- A Oligoduplex substrate used in the cleavage assay. 55 nt oligoduplex SP1 contains the proto-spacer1(red letters), PAM (blue letters) and 10 nt flanking sequences on both sides identical to those in pSP1 plasmid. In the SP1 oligoduplex DNA strand complimentary to the 5′-terminal fragment of crRNA (red letters) is named (+)strand, an opposite DNA strand is named ( ⁇ )strand.
- A discloses SEQ ID NOS 31, 7, and 34, respectively, in order of appearance.
- B Oligoduplex SP1 cleavage.
- Cleavage positions are designated by arrows.
- B discloses SEQ ID NO: 31.
- C Schematic representation of pSP1 plasmid (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) used in the plasmid cleavage assay.
- C discloses SEQ ID NO: 57.
- D pSP1 plasmid cleavage. Agarose gel analysis of pSP1 cleavage products (left panel). SC—super-coiled plasmid DNA, OC—open circular DNA nicked at one of the strands, FLL—full length linear DNA cut at both strands. Final reaction mixtures at 37° C.
- FIG. 6 shows DNA binding and cleavage analysis of Cas9-Chis protein lacking crRNA.
- Electrophoretic mobility shift analysis (EMSA) of Cas9-Chis protein binding to (A) the double stranded SP1 oligoduplex and (B) the single stranded s(+)SP1 oligonucleotide. Electrophoretic mobility shift experiments were performed in the binding buffer (40 mM Tris-acetate, pH 8.3 at 25 C, 0.1 EDTA, 0.1 mg/ml BSA, 10% v/v glycerol). The reactions contained 0.5 nM of the 33P-labelled oligoduplex, and the protein at concentrations as indicated above each lane. (C). Oligonucleotide cleavage assay.
- FIG. 7 shows reprograming of Cas9-crRNA complex.
- A Schematic representation of heterologous loci in two plasmids used for reprogramming of Cas9-crRNA complex.
- pCas( ⁇ )SPN were constructed from pCas9( ⁇ ) plasmid (See FIG. 2 ), by inserting new spacer sequence (SN) (5′-CC ACC CAG CAA AAT TCG GTT TTC TGG CTG-3′ (SEQ ID NO: 16)) and inactivating Cas9 gene as described in (1).
- SN new spacer sequence
- B Agarose gel analysis of plasmid DNA cleavage products.
- SPN oligoduplex contains the new proto-spacer (red letters), PAM (blue letters). Cleavage positions are designated by arrows.
- D discloses SEQ ID NO: 39.
- FIG. 8 shows impact of spacer length on CRISPR-encoded immunity.
- A Schematic representation of shortened versions of proto-spacers inserted in the transformed plasmids.
- A discloses SEQ ID NOS 7 and 61-66, respectively, in order of appearance.
- B Effect of proto-spacer length on the plasmid transformation efficiency. Transformation efficiency is expressed as cfu per nanogram of plasmid DNA (mean ⁇ SD).
- C Schematic representation of oligoduplexes used in the in vitro cleavage and binding experiments.
- C discloses SEQ ID NOS 31 and 38, respectively, in order of appearance.
- FIG. 9 shows PAM is required for in vitro DNA binding and cleavage by the Cas9-crRNA complex.
- A Agarose gel analysis of plasmid DNA cleavage products.
- Three different plasmids PAM+Proto-spacer+ (pSP1 plasmid containing both the proto-spacer and PAM), PAM-Protospacer-(pUC18 plasmid containing multiple PAMs but no protospacer) and PAM-Protospacer+ (pSP1-p ⁇ (Sapranauskas et al., 2011.
- SC super-coiled plasmid DNA
- OC open circular DNA nicked at one of DNA strands
- FLL full length linear DNA cut at both strands.
- the reactions contained 0.5 nM of the 33P-labelled ssDNA or dsDNA oligonucleotide, and the protein at concentrations as indicated above each lane. After 15 min at room temperature, the samples were subjected to PAGE for 2 h and analysed as described in ‘Materials and Methods’
- FIG. 10 shows RNA binding and cleavage analysis of Cas9-crRNA complex.
- Electrophoretic mobility shift analysis of Cas9-crRNA complex binding to 84 nt RNA fragment containing proto-spacer-1, PAM and 24 nt flanking sequences on both sides.
- Left panel RNA ( ⁇ ) strand; center panel: RNA (+) strand; right panel: double stranded RNA.
- RNA fragments used for analysis were generated by in vitro transcription (TranscriptAidTM T7 High Yield Transcription Kit, Fermentas) from PCR fragments with inserted T7 promoter at the front end of RNA coding sequence.
- RNA polymerase promoter underlined, transcription start on bold.
- FIG. 11 shows RuvC and HNH active site motifs of Cas9 contribute to the cleavage of opposite DNA strands.
- A Localization of the conserved active site motifs within Cas9 protein. Amino acid residues identified as crucial for Cas9 in vivo activity (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) are indicated.
- B Agarose gel analysis of pSP1 plasmid cleavage by Cas9 and mutant proteins. Reactions were performed as described in and ‘Materials and Methods’
- C Strand preference of D31A mutant. Reactions were performed as described in FIG. 2 and ‘Materials and Methods’.
- D31 mutant cleaves only (+)strand of SP1 oligoduplex.
- C discloses SEQ ID NOS 31.
- D Strand preference of N891A mutant. N891 mutant cleaves only ( ⁇ )strand of SP1 oligoduplex. Cleavage positions are designated by arrows.
- D discloses SEQ ID NOS 31.
- FIG. 12 shows properties of Cas9 active site mutant-crRNA complexes.
- A Direct sequencing of reaction products obtained with Cas9 mutant D31A (RuvC-like active site motif).
- A discloses SEQ ID NOS 58, 59, 58, and 58, respectively, in order of appearance.
- B Direct sequencing of reaction products obtained with Cas9 N891A mutant (HNH-like active site motif).
- B discloses SEQ ID NOS 58, 58, 58, and 60, respectively, in order of appearance.
- C SP1 oligoduplex binding by the wt Cas9-crRNA and active site mutant complexes.
- D Cleavage of (+)SP1 strand by Cas9-crRNA mutant complexes.
- FIG. 13 shows molecular mass of the wt Cas9-Chis protein.
- FIG. 14 shows schematic arrangement and mechanism of crRNA-directed DNA cleavage by the Cas9-crRNA complex. Domain architecture of Cas9 is shown schematically on the top. Cas9-crRNA complex binds to the dsDNA containing PAM. crRNA binds to the complementary (+)strand resulting in DNA strand separation and the R-loop formation.
- RuvC active site of Cas9 is positioned at the scissile phosphate on the unpaired ( ⁇ )strand, while HNH active site is located at the scissile phosphate on the DNA (+)strand bound to crRNA. Coordinated action of both active sites results in the double strand break 3 nt away from the 5′-NGGNG-5′ PAM generating blunt end DNA.
- FIG. 14 discloses SEQ ID NOS. 31 and 7, respectively, in order of appearance.
- FIG. 15 shows native electrophoresis of Cas9-crRNA and cleavage products.
- Samples was mixed with loading dye solution (0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol) and analysed by non-denaturing PAGE.
- the cartoons in each side of the gel illustrate protein-DNA complexes and DNA that correspond to each band, while cartoons below the gel illustrate major substrate form after reaction.
- FIG. 16 shows plasmid DNA cleavage by Cas9-crRNA complex.
- A pSP1 and pUC18 plasmid DNA cleavage. Cas9-crRNA complex was incubated with pSP1 and pUC18 plasmids in a reaction buffer provided in the Example 1.
- pSP1 plasmid contained a proto-spacer1 sequence flanked by the the 5′-NGGNG-3′ PAM sequence. Proto-spacer1 sequence was not present in pUC18. Reaction products were analysed in the agarose gel. Under these conditions pSP1 plasmid is converted into a linear form while pUC18 plasmid lacking proto-spacer1 sequence is resistant to cleavage.
- FIG. 17 shows DNA oligoduplex cleavage by Cas9-crRNA complex.
- the strand of oligoduplex which is complementary to crRNA is marked as (+) strand, while the other strand—( ⁇ ) strand.
- (+) or ( ⁇ ) strand of the oligoduplex was P33-labeled at the 5′-terminus.
- M1 and M2 are synthetic oligonucleotide markers corresponding to the 37 nt of ( ⁇ ) strand and 18 nt of (+) strand which were used to determine the size of the cleavage products and map the cleavage position.
- Cas9 protein cleaves both strands of oligoduplex inside the proto-spacer, after the 37th nucleotide, 3 nt upstream of the PAM (5′-NGGNG-3′) leaving blunt ends. Both strands of non-specific substrate (K1 and K2) are not cleaved when incubated with Cas9-crRNA complex for 30 min.
- FIG. 17 discloses SEQ ID NO: 31.
- FIG. 18 shows plasmid DNA cleavage by Cas9-crRNA complex assembled in the absence of RNaseIII.
- Cas9-crRNA complex was incubated with pSP1 plasmid and reaction products analysed in the agarose gels.
- the pSP1 plasmid is resistant for cleavage in the presence of complex assembled without crRNA (left panel).
- the pSP1 plasmid is converted into linear form in the presence of complex assembled using synthetic 42 nt crRNA (no RNAseIII) (middle panel).
- the pSP1 plasmid is converted into a mixture of linear and circular DNA forms in the presence of complex assembled using CRISPR RNA transcript (no RNAseIII) (right panel).
- FIG. 19 shows DNA oligoduplex cleavage by Cas9-crRNA complex.
- the strand of oligoduplex which is complementary to crRNA is marked as (+) strand, while the other strand—( ⁇ ) strand.
- (+) or ( ⁇ ) strand of the oligoduplex was P33-labeled at the 5′-terminus.
- M1 and M2 are synthetic oligonucleotide markers corresponding to the 37 nt of ( ⁇ ) strand and 18 nt of (+) strand which were used to determine the size of the cleavage products and map the cleavage position.
- Cas9 protein cleaves both strands of oligoduplex inside the proto-spacer, after the 37th nucleotide form the 5′-end, 3 nt upstream of the PAM (5′-NGGNG-3′) leaving blunt ends. Both strands of non-specific substrate (K1 and K2) are not cleaved when incubated with Cas9-crRNA complex for 30 min.
- FIG. 19 discloses SEQ ID NO: 31.
- FIG. 20 shows (A) Schematic representation of the CRISPR3/Cas system of S. thermophilus DGCC7710.
- cas genes cas9, cas1, cas2, csn2
- cas9, cas1, cas2, csn2 are located upstream of the CRISPR repeat-spacer array, consisting of 13 repeat (R) sequences and 12 unique spacers (S1-S12).
- the tracrRNA required for crRNA maturation in Type II CRISPR/Cas systems (Deltcheva et al.,2011. Nature 471, 602-7), is located upstream the cas9 gene and encoded on the opposite DNA strand (shown by an arrow) with respect to the other elements of this system.
- B The pathways for a new spacer insertion in to CRISPR region and CRISPR RNA synthesis.
- Synthetic oligoduplex encoding desired spacer sequence and containing Sapl and Eco31I restriction compatible ends was inserted between two repeats.
- the CRISPR region was amplified using PCR.
- the new spacer encoding CRISPR RNA was obtained by In vitro transcription.
- C In vitro assembly of Cas9-RNA complex.
- the CRISPR RNA and tracrRNA transcripts were assembled in to duplex.
- the Cas9 protein was first pre-incubated with RNA duplex, followed by the subsequent incubation with RNAseIII to generate a catalytically competent Cas9-RNA complex.
- FIG. 21 shows A. Schematic representation of pUC18 plasmid. The distance between Sapl and AatII restriction sites is 775 bp, while the distance between two spacers is 612 bp. B. pUC18 plasmid cleavage by re-programed Cas9-crRNA complexes.
- FIG. 22 shows genomic DNA cleavage with in vitro assembled Cas9-RNA complex.
- A Agarose gel analysis of linear A DNA cleavage products. Phage A DNA was incubated with Cas9-RNA complex in the reaction buffer for various time intervals. The target site for Cas9-RNA complex is located 8 kb away from the cos site.
- B Probe selection for Southern blot experiments. Genomic DNA was fragmented by treating with Pstl enzyme. The proto-spacer is located between two Pstl sites. If genomic DNA is cleaved with Cas9-RNA complex, 466 by fragment should be detected. Otherwise the probe will hybridize with 1499 by length fragment.
- C Southern blot analysis of genomic DNA fragments. C line— E.
- Cas9-RNA genomic DNA was incubated with Cas9-RNA complex before fragmentation.
- D Human genomic DNA cleavage by Cas9-crRNA complex. Relative amount of intact DNA DNA fragments were estimated by qPCR.
- Genomic DNA of Streptococcus thermophilus DGCC7710 strain was used as a template in PCR reactions to clone cas9.
- PCR fragment amplified with following primers: 5′-ACGTCTCAAATGTTGTTTAATAAGTGTATAATAATTTC-3′ (SEQ ID NO: 21) and 5′-ACGTCTCCGCGCTACCCTCTCCTAGTTTG-3′ (SEQ ID NO: 22) was cloned into the pASK-IBA3 expression vector via Esp3l sites.
- Cas9 protein and Cas9-crRNA complex 6xHis-tagged (“6 ⁇ His” disclosed as SEQ ID NO: 23) version of Cas9 protein was expressed and purified using a scheme described for the Cas3 protein from S. thermophilus CRISPR4/Cas system (Sinkunas et al.,2011. EMBO J 30:1335-42).
- Strep-tagged version of the Cas9 protein was expressed in E. coli RR1 strain, bearing pCas9( ⁇ )SP1 plasmid ( FIG. 1B ).
- LB broth was supplemented with Ap (100 ⁇ g/ml) and Cm (10 ⁇ /ml.
- coli cells for the Cas9-crRNA complex isolation were grown in two steps. First, 4 ml of cells culture were grown at 37° C. to OD600 of ⁇ 0.5, and expression induced by adding 0.2 ⁇ g/ml of anhydrotetracycline (AHT) (Sigma). After for 4 h, 1/400 of the pre-induced culture was inoculated into fresh LB medium supplemented with Ap (100 ⁇ g/ml), Cm (12 ⁇ g/ml) and AHT (0.2 ⁇ g/ml) and was grown at 37° C. overnight. Harvested cells were disrupted by sonication and cell debris removed by centrifugation.
- AHT anhydrotetracycline
- the supernatant was loaded onto the 1 ml StrepTrap HP column (GE Healthcare) and eluted with 2.5 mM of desthiobiotin. Approximately 1.5 ⁇ g of the Cas9 protein was obtained in a single run from 1 L of E. coli culture. The fractions containing Cas9 were stored at +4° C. for several days. The homogeneity of protein preparations was estimated by SDS-PAGE. Protein concentrations in the Cas9-crRNA complexes were determined by densitometric analysis of SDS-PAGE gels containing samples of Strep-Tactin purified Cas9 proteins along with known amounts of His-tagged Cas9 protein. The concentration of the Cas9-crRNA complexes is expressed as Cas9 protein concentration assuming that Cas9 is a monomer and binds crRNA in a complex with 1:1 stoichiometry.
- RNA was cross-linked to the membrane with 0.16 M l-ethyl-3-(3-dimethylaminopropyl) carbodiimide (EDC) (Pierce)/0.13 M 1-methylimidazole (Sigma) pH 8 at 60° C. for 1 h.
- EDC carbodiimide
- the membrane was pre-hybridized with 2 ⁇ SSC buffer containing 1% SDS and 0.1 mg/ml denatured DNA from fish testes (Ambion) for 1 h at 40° C.
- Blots were probed for 12 h with a 32 P-5′-labelled 42 nt anti-crRNA DNA oligonucleotide containing 20 nt of spacer1 and 22 nt of the repeat sequence (5′-TCGAAACAACACAGCTCTAAAACTGTCCTCTTCCTCTTTAGC-3′ (SEQ ID NO: 28)). The blots were washed 3 ⁇ for 15 min with 0.2 ⁇ SSC buffer containing 0.2% SDS, and were visualized using phosphorimaging.
- a 42 nt synthetic oligoribonucleotide (5′-CGCUAAAGAGGAAGAGGACAGUUUUAGAGCUGUGUUGUUUCG-3′ (SEQ ID NO: 7)) and 84 nt DNA oligonucleotide.
- Oligonucleotide substrates All oligonucleotide substrates used in this study are given in Table 1. Oligodeoxyribonucleotides were purchased from Metabion (Martinsried, Germany). The 5′-ends of oligonucleotides were radiolabelled using PNK (Fermentas) and [y-33P]ATP (Hartmann Analytic). Duplexes were made by annealing two oligonucleotides with complementary sequences (SP1, SP1- ⁇ p, SP2). Radioactive label was introduced at the 5′ end of individual DNA strand prior to the annealing with unlabelled strand.
- PNK Fermentas
- [y-33P]ATP Hard Analytic
- Reactions with oligonucleotide substrates were typically carried out by adding 2 nM of Cas9-crRNA complex to 1 nM labeled oligonucleotide in 10 mM Tris-HCl (pH 7.5 at 37° C.), 10 mM NaCl, 0.1 mg/ml BSA and 10 mM MgCl2 at 37° C. Aliquots were removed at timed intervals and quenched with loading dye (95% v/v formamide, 0.01% bromphenol blue, 25 mM EDTA, pH 9.0) and subjected to denaturing gel electrophoresis through 20% polyacrylamide followed by a FLA-5100 phosphorimager (Fujilm) detection.
- loading dye 95% v/v formamide, 0.01% bromphenol blue, 25 mM EDTA, pH 9.0
- Reactions with plasmid substrates Reactions on pUC18 plasmid and its derivatives (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) were conducted at 37° C. in the buffer used for reactions on oligonucleotide substrates. Reaction mixtures typically contained 2.5 nM supercoiled plasmid and 2 nM of Cas9-crRNA complex. The reactions were initiated by adding protein to the mixture of the other components. Aliquots were removed at timed intervals and quenched with phenol/chloroform. The aqueous phase was mixed with loading dye solution (0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol) and analyzed by electrophoresis through agarose.
- loading dye solution 0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol
- Plasmid cleavage position determination To achieve complete cleavage of plasmid substrate, 8 nM of Cas9-crRNA complex was incubated with 2.5 nM of supercoiled plasmid in the reaction buffer at 37° C. for 10 min. Reaction products were purified and concentrated using GeneJET PCR Purification Kit (Fermentas).
- Spacer1 surrounding region of Cas9 linearized and nicked plasmids were directly sequenced with the following primers: 5′-ccgcatcaggcgccattcgcc-3′ (SEQ ID NO: 29) (sequencing of (+)strand) and 5′-gcgaggaagcggaagagcgccc-3′ (SEQ ID NO: 30) (sequencing of ( ⁇ )strand).
- Binding assay Increasing amounts of protein-crRNA complex were mixed with 0.5 nM of 33P-labeled double-stranded and single-stranded DNA substrates (Table 1) in the binding buffer (40 mM Tris-acetate, pH 8.3 at 25 C, 0.1 EDTA, 0.1 mg/ml BSA, 10% v/v glycerol) and incubated for 15 min at room temperature. Free DNA and protein-DNA complexes were separated on the non-denaturing 8% polyacrylamide gel (ratio of acrylamide/N,N′-methylenebisacrylamide 29:1) using 40 mM Tris-acetate (pH 8.3) supplemented with 0.1 mM EDTA as the running buffer. Electrophoresis was run at room temperature for 3 h at 6 V/cm.
- mutants D31A and N891A were obtained by the site-directed mutagenesis as previously described (Tamulaitis et al., 2007. Nucleic Acids Res 35:4792-9). Sequencing of the entire gene for each mutant confirmed that only the designed mutation had been introduced.
- Oligonucleotide substrates Proto-spacer sequence is underlined, PAM is on bold.
- Oligonucleotide Sequence Specification SP1 5′-GCTCGAATTG AAATTCTAAACGCTAAAGAGGAAGAGGACA T GG T G AATTCGTAAT-3 55 bp oligoduplex (SEQ ID NO: 31) 3′-CGAGCTTAAC TTTAAGATTTGCGATTTCTCCTTCTCCTGT A CC A C TTAAGCATTA-5′ substrate containing proto-spacer1 and PAM SP1-p ⁇ 5′-GCTCGAATTG AAATTCTAAACGCTAAAGAGGAAGAGGACA AATTCGTAAT-3′ 50 bp oligoduplex (SEQ ID NO: 32) 3′-CGAGCTTAAC TTTAAGATTTGCGATTTCTCCTTCCTGT TTAAGCATTA-5′ substrate containing proto-spacer2 SP2 5′-GCTCGAATTG TACTGCTGTATTAGCTTGGTTGTTGGTTTG T
- oligonucleotide substrate (+) strand of SP1- ⁇ oligoduplex s(+) SP2 5′-ATTACGAATTCACCA CAAACCAACAACCAAGCTAATACAGCAGTA CAATTCGAGC-3′ 55 nt ssDNA
- oligonucleotide substrate (+) strand of SP2 oligoduplex s( ⁇ ) SP1 5′-GCTCGAATTG AAATTCTAAACGCTAAAGAGGAAGAGGACA T GG T G AATTCGTAAT-3′ 55 nt ssDNA
- SEQ ID NO: 37 oligonucleotide substrate, ) strand of SP1 oligoduplx SP1-20 5′-GCTCGAATTG CGCTAAAGAGGAAGAGGACA T GG T G AATTCGTAAT-3 45 nt oligoduplex (SEQ ID NO: 38) 3′-CGAGCTTAAC GCGATTTCCTTCTCCTGT A CC A C TTA
- the cas9 gene from the CRISR3 system of S. thermophilus DGCC7710 strain was cloned into the pASK-IBA3 vector to produce a construct encoding a Cas9 protein fusion containing a C-terminal Strep(II)-tag ( FIG. 1B ).
- a construct encoding a Cas9 protein fusion containing a C-terminal Strep(II)-tag FIG. 1B .
- we have tried to purify Cas9-crRNA complex from E. coli strain RR1 expressing Cas9 protein on the pASK-IBA3 vector and other Cas proteins (except Cas9) on pCas9( ⁇ ) plasmid (Sapranauskas et al, 2011).
- pCas9( ⁇ ) also contained a complete CRISPR3 array comprised of 12 spacer-repeat units ( FIG. 2A ).
- cas9 gene expression was performed in two steps. First, we induced Cas9 expression in a small volume of E. coli culture and after 4 h transferred an aliquot of pre-induced culture into a larger volume of fresh LB media already containing inductor and incubated overnight. Cas9 protein complex was purified from the crude cell extract using Strep-Tactin Sepharose. We managed to isolate a small amount of the Cas9-crRNA complex which showed only traces of nucleolytic activity on the oligoduplex SP1 containing a proto-spacer1 and PAM.
- CRISPR3/Cas system of S. thermophilus belongs to the Type IIA subtype (former Nmeni or CASS4) of CRISPR/Cas systems (Makarova et al., 2011. Nat Rev Microbiol 9:467-77). It has been shown that in the Type IIA CRISPR/Cas system of Streptococcus pyogenes trans-encoded small RNA (tracrRNA) and bacterial RNaseIII are involved in the generation of crRNA (Deltcheva et al., 2011. Nature 471:602-7).
- Streptococcus pyogenes crRNA is only 42 nt in length and has no “5′-handle” which is conserved in crRNA's from Type I and III CRISPR systems (Hale et al., 2009. Cell 139:945-56; Jore et al., 2011. Nat Struct Mol Biol 18:529-36). According to the northern blot analysis crRNA of similar length is generated in the S. thermophilus LMD-9 CRISPR3/Cas system (Makarova et al., 2011. Nat Rev Microbiol 9:467-77), which is almost identical to the CRISPR3/Cas system of DGCC7710 strain ( FIGS. 4A and B).
- crRNA isolated from the Cas9-crRNA complex expressed in the heterologous E. coli strain may have the same length ( FIG. 4 ). Therefore, to probe nucleic acids extracted from the Strep-Tactin purified Cas9 complex we used 42 nt anti-crRNA DNA oligonucleotide comprised of 22 nt region corresponding to the 3′-end of the repeat sequence and 20 nt at the 5′-end of SP1 fragment. Nucleic acid present in the Cas9 complex hybridized with anti-crRNA oligonucleotide, and was sensitive to RNAse but not DNAse treatment ( FIG. 1C ).
- the size of extracted crRNA was identical to the 42 nt synthetic oligoribonucleotide corresponding to the putative crRNA of the CRISPR3 system of S. thermophilus DGCC7710 strain ( FIG. 3A , FIG. 4C ). Taken together, these data confirm that Cas9 Strep-tag protein co-purifies with 42 nt crRNA, which is derived from CRISPR3 region.
- Cas9 protein cleaves double-stranded DNA within a proto-spacer.
- SP1 oligoduplex Table 1 containing the proto-spacer sequence identical to spacer SP1 in the CRISPR3 array, the PAM sequence 5′-TGGTG-3′ downstream of the proto-spacer, and 10 nt flanking sequences from pSP1 plasmid (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) ( FIG. 5A ).
- the oligoduplex strand complementary to crRNA is named (+)strand, while the opposite duplex strand is called the ( )strand.
- Cas9-crRNA cleavage specificity is directed by the crRNA sequence.
- the cleavage specificity of Cas9-crRNA complex was analysed using plasmids pSP1+SPN and pSP1.
- the length of the spacer in the CRISPR3 region of S. thermophilus is 30 nt.
- the mature crRNA copurified with the Cas9 protein is comprised of 42 nt. It means that only 20 nt of crRNA is complementary to the (+)strand of proto-spacer. To assess whether 5′-end of proto-spacer is important for the plasmid interference by the CRISPR3 system of S.
- thermophilus we engineered plasmids pSP1-27, pSP1-23, pSP1-19, pSP1-15, pSP1-11 with the 5′-truncated proto-spacer1 (the length of proto-spacer 27 bp, 23 bp, 19 bp, 15 bp, 11 bp, respectively), and analyzed transformation efficiency of the recipient strain containing pCRISPR3 ( FIG. 8B ). Plasmids containing 4 or 7 by truncations at the 5′ end of proto-spacer1, had no effect on the recipient strain ability to interfere with plasmid transformation. Shorter versions of proto-spacer (11, 15, 19 bp) abolished recipient strain ability to prevent plasmid transformation.
- PAM is required for DNA binding and cleavage by Cas9-crRNA. Plasmids carrying a proto-spacer but not PAM (pSP1-p ⁇ ) or multiple PAM's but no proto-spacer (pUC18) are resistant for Cas9-crRNA cleavage ( FIG. 8A ). Hence, in accordance with in vivo data both PAM and proto-spacer are required for double-stranded DNA cleavage by Cas9-crRNA complex (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82).
- single-stranded oligonucleotides ((+)strand) are bound by Cas9-crRNA with the same affinity independently of the PAM presence ( FIG. 9D ). Again, no binding was observed for single-stranded DNA oligonucleotide without proto-spacer ( FIG. 9D ), or for Cas9 protein lacking crRNA ( FIG. 6C ). Taken together these data indicate that Cas9-crRNA complex discriminates PAM only in the double-stranded but not a single-stranded DNA.
- both mutants produced nicked DNA form ( FIG. 11B ) indicating that both active sites mutants cleave only one DNA strand of plasmid substrate within a proto-spacer.
- Cas9 protein is functional as a monomer and uses two active sites for the cleavage of opposite DNA strands. Similar strategy is exploited by some restriction endonucleases (Armalyte et al., 2005. J Biol Chem 280: 41584-94).
- Cas9-crRNA complex of CRISPR3/Cas system of S. thermophilus is crRNA-guided endonuclease. This work demonstrates that Cas9-crRNA complex of CRISPR3/Cas system of S. thermophilus is crRNA-directed endonuclease which cuts both DNA strands in the presence of Mg2+-ions within a protospacer 3 nt downstream of the PAM sequence to produce blunt end cleavage products. Sequence specificity of the Cas9-crRNA complex is dictated by the 42 nt crRNA which include ⁇ 20 nt fragment complementary to the proto-spacer sequence in the target DNA. In this respect the mature crRNA in the Cas9 complex of CRISPR3/Cas system of S.
- thermophilus is similar to crRNA of Streptoccocus pyogenes which has a 3′-handle of repeat sequence but lacks part of the spacer sequence and 5′-handle corresponding to the repeat fragment (Deltcheva et al, 2011). Therefore, crRNA present in the Cas9-crRNA complex of CRISPR3/Cas system of S. thermophilus is complementary only to the part of the proto-spacer sequence distal to PAM. Not surprisingly, truncation of the 3′-end of the proto-spacer sequence by 10 nucleotides has no effect on Cas9-crRNA cleavage of synthetic oligoduplexes or plasmid DNA ( FIG. 8 ).
- the cleavage machinery of Cas9-crRNA complex resides in the Cas9 protein which provides two active sites for the phosphodiester bond cleavage.
- the RuvC- and HNH-like active sites of Cas9 protein are located on different domains and act independently on individual DNA strands. Alanine replacement of the active site residues in the RuvC- and HNH-motifs transforms Cas9-crRNA complex into a strand-specific nicking endonucleases similar to the nicking enzymes (Chan et al., 2011. Nucleic Acids Res 39:1-18).
- both PAM and proto-spacer sequences are necessary prerequisite for double-stranded DNA binding and subsequent cleavage.
- PAM sequence motif has no effect on the single-stranded DNA binding by: a single-stranded oligodeoxynucleotide containing proto-spacer with or without PAM sequence is bound equally well but with lower affinity than double-stranded DNA.
- Cas9 cuts single-stranded DNA bound to the crRNA using its HNH-active site.
- the N-terminal domain containing the catalytic D31A residue of the RuvC motif is positioned at the displaced ( ⁇ ) DNA strand, while the central part of Cas9 containing the HNH motif is located in the vicinity of the scissile phosphodiester bond of (+) DNA strand paired to crRNA.
- Cas9-crRNA remains bound to the reaction products ( FIG. 15 ).
- RNA interference complexes Comparison to other RNA interference complexes.
- the mechanism proposed here for the double-stranded DNA cleavage by the Cas9-crRNA complex differs significantly from that for the Type I-E (former Ecoli or CASS2) system (Jore et al., 2011. Nat Struct Mol Biol 18:529-36).
- CRISPR RNA and complementary target sequences Jore et al., 2011. Nat Struct Mol Biol 18:529-36.
- Target recognition is dependent on PAM and governed by the “seed” crRNA sequence located at the 5′-end of the spacer region (Semenova et al., 2011. Proc Natl Acad Sci USA 108:10098-103).
- Cascade-crRNA complex alone is able to bind double-stranded DNA containing PAM and proto-spacer, it requires an accessory Cas3 protein for DNA cleavage.
- Cas3 is a single-stranded DNA nuclease and helicase which is able to cleave single-stranded DNA producing multiple cuts (Sinkunas et al.,2011. EMBO J 30:1335-42).
- Cas module RAMP (Cmr) proteins and cRNA assemble into the effector complex that targets invading RNA (Hale et al., 2009. Cell 139:945-56; Hale et al., 2012. Mol Cell 45:292-302).
- Pyroccus furiosus RNA silencing complex comprised of six Cmr1-6 proteins and crRNA binds to the target RNA and cuts it at fixed distance in respect to 3′-end the psiRNA. The cleavage activity depends on Mg2+-ions however individual Cmr protein(-s) responsible for target RNA cleavage has yet to be identified.
- the effector complex of Sulfolobus solfataricus comprised of seven Cmr1-7 proteins and crRNA cuts invading RNA in an endonucleolytic reaction at UA dinucleotides (Zhang et al., 2012. Mol Cell 45: 303-13).
- both Cmr-crRNA complexes perform RNA cleavage in a PAM independent manner.
- Cas9-crRNA complex of CRISPR3 system is so far the most simple DNA interference system comprised of a single Cas9 protein bound to the crRNA molecule.
- the simple modular organization of the Cas9-crRNA complex where specificity for DNA target is encoded by the crRNA and cleavage machinery is brought by the Cas protein provides a versatile platform for engineering of universal RNA-guided DNA endonucleases.
- Cas9-crRNA complex can be assembled in vitro by mixing 4 individual components: the C-terminal 6 ⁇ His-tagged variant of Cas9 protein (“6 ⁇ His” disclosed as SEQ ID NO: 23), tracrRNA transcript (SEQ ID NO: 5), CRISPR RNA transcript (SEQ ID NO: 8) and E. coli RNAseIII (Abgene).
- Cas9 protein is first pre-incubated with tracrRNA and CRISPR RNA transcripts, followed by the subsequent incubation with RNAseIII to generate a catalytically competent Cas9-crRNA complex which is used for the site-specific DNA cleavage.
- RNA fragments required for complex assembly were produced by in vitro transcription (TranscriptAidTM T7 High Yield Transcription Kit, Fermentas) of PCR-generated fragment containing a T7 promoter at the proximal end of RNA coding sequence.
- PCR-generated DNA fragments encoding CRISPR RNA and tracrRNA were produced using pCas9( ⁇ )SP1 plasmid as a template with a following primer pair: 5′-taatacgactcactataGggtagaaagatatcctacgagg-3′ (SEQ ID NO: 40)/5′-CAACAACCAAGCTAATACAGCAG-3′ (SEQ ID NO: 41) and 5′-aaaaacaccgaatcggtgccac-3′ (SEQ ID NO: 42)/5′-taatacgactcactataGggTAATAATAATTGTGGTTTGAAACCATTC-3′ (SEQ ID NO: 43) (T7 RNA polymerase promoter underlined, transcription start shown in bold).
- the 150 nt CRISPR RNA transcript is comprised of 102 nt Repeat-Spacerl-Repeat sequences flanked by the 23 nt upstream and 25 nt downstream regions required for primer annealing.
- the 105 nt transcript of tracrRNA is comprised of a 38 nt stretch partially complimentary to the S. thermophilus DCGG7710 CRISPR3 repeat sequence fragment (anti-repeat sequence), flanked by the 16 nt upstream and 51 nt downstream region.
- RNA fragments produced by in vitro transcription were purified using RNeasy MinElute Cleanup Kit (Qiagen).
- 6 ⁇ His-tagged Cas9 protein (“6 ⁇ His” disclosed as SEQ ID NO: 23) was mixed with CRISPR RNA and tracrRNA transcripts at 1:0.5:1 molar ratio and pre-incubated in a buffer containing 10 mM Tris-HCl (pH 7.5 at 37° C.), 100 mM NaCl at 37° C. for 30 min followed by addition of RNAseIII (Ambion), MgCl2 and DTT and subsequent incubation for additional 30 min.
- the final concentrations of the components in the assembly mix were the following: 100 nM of 6 ⁇ His-tagged Cas9 protein (“6 ⁇ His” disclosed as SEQ ID NO: 23), 50 nM of CRISPR RNA, 100 nM of tracrRNA, 50 nM RNAseIII, 10 mM MgCl 2 and 1 mM DTT.
- Cas9-crRNA complex guided by the crRNA sequence cleaves DNA at the specific site to generate blunt ends.
- Cas9-crRNA complex can be used an alternative for a restriction endonuclease or meganuclease for the site-specific DNA cleavage in vitro.
- the sequence specificity of the complex is dictated by the crRNA sequence which can be engineered to address a desirable DNA target.
- the DNA cleavage activity of the in vitro assembled Cas9-crRNA complex was assayed on the plasmid substrates pSP1 and pUC18.
- the pSP1 plasmid contained a proto-spacer1 sequence flanked by the 5′-NGGNG-3′ PAM sequence. Proto-spacer1 sequence was not present in pUC18. Reactions on pUC18 and pSP1 plasmids (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) were conducted at 37° C.
- reaction mixtures typically contained 3.0 nM of supercoiled plasmid DNA.
- the reactions were initiated by mixing 50 ⁇ l volumes of Cas9-crRNA complex and plasmid DNA (1:1 v/v ratio) in a reaction buffer. Aliquots were removed at timed intervals and quenched with phenol/chloroform.
- the aqueous phase was mixed with loading dye solution (0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol) and reaction products analyzed by electrophoresis through agarose ( FIG. 16 ).
- loading dye solution 0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol
- reaction products analyzed by electrophoresis through agarose ( FIG. 16 ).
- loading dye solution 0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol
- Reaction product analysis revealed that in vitro assembled Cas9-crRNA complex cleaved both strands of the oligoduplex at fixed position, inside the proto-spacer, after the 37th nucleotide from the 5′-terminus, 3 nt upstream of the PAM sequence 5′-NGGNG-3′ leaving blunt ends ( FIG. 17 ).
- Synthetic 42 nt oligoribonucleotide is comprised of 20 nt of identical to the spacer1 of CRISPR3 region at the 5′ terminus and 22 nt of repeat sequence at the 3′ end. More specifically, tracrRNA and CRISPR RNA transcripts were obtained as described in Example 1. To generate the Cas9-crRNA complex the 6 ⁇ His-tagged Cas9 protein (“6 ⁇ His” disclosed as SEQ ID NO: 23) was mixed with tracrRNA and CRISPR RNA transcript, or 42 nt synthetic crRNA, at 1:0.5:1 molar ratio and incubated in a buffer containing 10 mM Tris-HCl (pH 7.5 at 37° C.), 100 mM NaCl at 37° C.
- the final concentrations of the components in the assembly mix were the following: 100 nM of 6 ⁇ His-tagged Cas9 protein (“6 ⁇ His” disclosed as SEQ ID NO: 23), 50 nM of CRISPR RNA or 42 nt synthetic crRNA, 100 nM of tracrRNA.
- Cas9-crRNA complex guided by the crRNA sequence cleaves DNA at the specific site to generate blunt ends.
- Cas9-crRNA complex can be used an alternative for a restriction endonuclease or meganuclease for the site-specific DNA cleavage in vitro.
- the sequence specificity of the complex is dictated by the crRNA sequence which can be engineered to address a desirable DNA target.
- the DNA cleavage activity of the in vitro assembled Cas9-crRNA complex was assayed on the plasmid substrates pSP1 and pUC18.
- the pSP1 plasmid contained a proto-spacer1 sequence flanked by the 5′-NGGNG-3′ PAM sequence. Proto-spacer1 sequence was not present in pUC18. Reactions on plasmid substrates (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) were conducted at 37° C.
- reaction mixtures typically contained 3.0 nM of supercoiled plasmid DNA.
- the reactions were initiated by mixing 50 ⁇ l volumes of Cas9-crRNA complex and plasmid DNA (1:1 v/v ratio) in a reaction buffer. Aliquots were removed at timed intervals and quenched with phenol/chloroform. The aqueous phase was mixed with loading dye solution (0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol) and reaction products analyzed by electrophoresis through agarose ( FIG. 18 ).
- Reaction product analysis revealed that in vitro assembled Cas9-crRNA complex cleaved both strands of the oligoduplex at fixed position, inside the proto-spacer, after the 37th nucleotide form the 5′-end, 3 nt upstream of the PAM sequence 5′-NGGNG-3′ leaving blunt ends ( FIG. 19 ).
- FIG. 20B we describe an interchangeable spacer cassette which allows to produce crRNA carrying a nucleotide sequence against any desirable DNA target to be used for assembly of the Cas9-crRNA complex described in Examples 1 and 2 ( FIG. 20B ).
- the cassette caries a single repeat-spacer-repeat unit which allows insertion of the oligoduplex carrying the new spacer sequence required to generate a desired crRNA.
- To engineer a cassette first we constructed a cassette containing a leader sequence, a repeat sequence and a unique Sapl recognition site in the vicinity of the repeat sequence followed by BamHI site ( FIG. 20C ).
- the distance between Sapl and AatII restriction sites is 775 bp, while the distance between the putative Cas9-crRNA complex cleavage sites located in the spacers N1 and N2 is 612 by ( FIG. 21A ).
- the crRNA1 and crRNA2 PCR fragments containing T7 promoter at the proximal end were obtained from the corresponding interchangeable spacer cassette plasmids and used to produce by in vitro transcription CRISPR RNA transcripts carrying sequences matching spacer N1 or spacer N2 sequences.
- the catalytically active complexes of Cas9 with crRNA1 and crRNA2 were assembled for DNA cleavage as described in Example 1.
- Cas9-crRNA complex may be used to prepare a vector for cloning procedure.
- cleavage products obtained by the Cas9-crRNA complex can be re-ligated by DNA ligase.
- DNA ligase We purified linear pSP1 cleavage product from agarose gel and re-ligated it using DNA ligase. After transformation of E. coli cells by the ligation mix, five individual clones were selected from resulting transformants, plasmid DNA was purified and subjected to sequencing.
- FIG. 21A Next we analyzed cleavage of pUC18 plasmid with Cas9 complex loaded with crRNA1 and crRNA2 described in Example 5 ( FIG. 21A ).
- pUC18 was cleaved with one complex, purified and re-ligated. Sequencing of 10 clones in each case confirmed, that sequence of cleaved and re-ligated plasmid was identical to the sequence of the non-treated plasmid ( FIG. 21C ). This experiment suggests that additional mutations are not introduced after cleavage by Cas9-crRNA complex and ligation, and the Cas9-crRNA complex can be used for cloning experiments.
- the 2 ⁇ g pUC18 was incubated with the mix of separately assembled Cas9-RNA complexes (250 nM each) containing different crRNAs for 1 hour at 37° C. in 100 ⁇ l reaction volume (10 mM Tris-HCl (pH 7.5 at 37° C.), 100 mM NaCl, 1 mM DTT and 10 mM MgCl 2 ). Obtained vector fragment was purified from agarose gel using GeneJET gel extraction Kit (Thermo Fisher scientific) and divided in to two equal parts. One part of pre-cleaved vector was dephosphorylated with the FastAP alkaline phosphatase while another part was untreated.
- Cas9-crRNA may be addressed to cleave targets in long DNA molecules, including phage A, E. coli and human genomic DNAs.
- Cas9-RNA complex to cleave specific sites in ⁇ bacteriophage (48 kb), E. coli BL-21 strain (4.6 Mb) and human (3.2 Gb) genomic DNAs.
- Cas9-crRNA complex was assembled as described in Examples 2 and 3.
- ⁇ DNA cleavage reactions were initiated by mixing ⁇ DNA (Thermo Fisher Scientific) with assembled Cas9-RNA complex (1:1 v/v ratio) and incubating at 37° C. Final reaction mixture contained 2 ⁇ g ⁇ DNA, 50 nM Cas9-RNA complex, 10 mM Tris-HCl (pH 7.5 at 37° C.), 100 mM NaCl, 1 mM DTT and 10 mM MgCl 2 in 100 ⁇ l reaction volume. Aliquots were removed at timed intervals and quenched with phenol/chloroform.
- the aqueous phase was mixed with 3 ⁇ loading dye solution (0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol) and reaction products analyzed by electrophoresis through agarose gels and ethidium bromide staining.
- 3 ⁇ loading dye solution 0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol
- reaction products analyzed by electrophoresis through agarose gels and ethidium bromide staining.
- the analysis of linear ⁇ phage genomic DNA cleavage products in agarose gel confirmed that ⁇ 40 by length DNA is efficiently cleaved at a single site ( FIG. 22A ).
- E. coli BL21 (DE3) strain was isolated using the Genomic DNA purification kit (Thermo Fisher Scientific).
- E. coli genomic DNA was combined with assembled Cas9-RNA complex (1:1 v/v ratio) and incubated for 3 hours at 37° C.
- Final reaction mixture contained 30 ⁇ g genomic DNA, 1 ⁇ M Cas9-RNA complex, 10 mM Tris-HCl (pH 7.5 at 37° C.), 100 mM NaCl, 1 mM DTT and 10 mM MgCl 2 in 300 ⁇ l reaction volume.
- the membrane was prehybridized with 6 ⁇ SSC buffer containing 0.5% SDS and 100 ⁇ g/ml denatured salmon sperm DNA (Amresco) for 1 h at 65° C.
- the hybridization probe was generated by PCR using the genomic E. coli BL21(DE3) DNA as a template yielding 397 by product. 5′-ends were dephosphorylated with FastAP phosphatase (Thermo Fisher Scientific) and radiolabelled by incubating with [ ⁇ - 32 P]ATP (Hartmann Analytic) and T4 PNK (Thermo Fisher Scientific).
- the labeled probe was purified using GeneJET PCR Purification Kit (Thermo Fisher Scientific), denatured by heating to 95° C.
- the probe was designed to target DNA fragment containing a target (a proto-spacer) for the Cas9-RNA complex ( FIG. 22B ).
- the distance between two Pstl targets is ⁇ 1500 bp, while the distance between proto-spacer and left Pstl target is 466 bp.
- After cleavage with Cas9 complex we detected only 466 by DNA fragment ( FIG. 22C ), which means that all DNA targets were cleaved by Cas9 protein in the desired position.
- Cas9-crRNA cleavage products of human genomic DNA we used DNA extracted from human brain. Human genomic DNA was combined with assembled Cas9-crRNA complex (1:1 v/v ratio) and incubated for 30 min at 37° C. Final reaction mixture contained 1 ⁇ g genomic DNA, 100 nM Cas9, 10 mM Tris-HCl (pH 7.5 at 37° C.), 100 mM NaCl, 1 mM DTT and 10 mM MgCl 2 in 100 ⁇ l reaction volume.
- Cas9-crRNA-HS1 (SEQ ID NO: 13) and Cas9-crRNA-H52 (SEQ ID NO: 14) complexes were assembled to target RASGEF1C or ARL15 loci, respectively.
Landscapes
- Life Sciences & Earth Sciences (AREA)
- Health & Medical Sciences (AREA)
- Chemical & Material Sciences (AREA)
- Genetics & Genomics (AREA)
- Engineering & Computer Science (AREA)
- Organic Chemistry (AREA)
- Zoology (AREA)
- Wood Science & Technology (AREA)
- Bioinformatics & Cheminformatics (AREA)
- Molecular Biology (AREA)
- Biotechnology (AREA)
- General Engineering & Computer Science (AREA)
- Biomedical Technology (AREA)
- Microbiology (AREA)
- Biochemistry (AREA)
- General Health & Medical Sciences (AREA)
- Biophysics (AREA)
- Physics & Mathematics (AREA)
- Plant Pathology (AREA)
- Proteomics, Peptides & Aminoacids (AREA)
- Immunology (AREA)
- Mycology (AREA)
- Crystallography & Structural Chemistry (AREA)
- Medicinal Chemistry (AREA)
- Analytical Chemistry (AREA)
- Chemical Kinetics & Catalysis (AREA)
- Cell Biology (AREA)
- General Chemical & Material Sciences (AREA)
- Micro-Organisms Or Cultivation Processes Thereof (AREA)
- Enzymes And Modification Thereof (AREA)
- Peptides Or Proteins (AREA)
- Preparation Of Compounds By Using Micro-Organisms (AREA)
- Medicines That Contain Protein Lipid Enzymes And Other Medicines (AREA)
- Measuring Or Testing Involving Enzymes Or Micro-Organisms (AREA)
Abstract
Isolation or in vitro assembly of the Cas9-crRNA complex of the Streptococcus thermophilus CRISPR3/Cas system and use for cleavage of DNA bearing a nucleotide sequence complementary to the crRNA and a proto-spacer adjacent motif. Methods for site-specific modification of a target DNA molecule using an RNA-guided DNA endonuclease comprising at least one RNA sequence and at least one of an RuvC active site motif and an HNH active site motif; for conversion of Cas9 polypeptide into a nickase cleaving one strand of double-stranded DNA by inactivating one of the active sites (RuvC or HNH) in the polypeptide by at least one point mutation; for assembly of active polypeptide-polyribonucleotides complex in vivo or in vitro; and for re-programming a Cas9-crRNA complex specificity in vitro or using a cassette containing a single repeat-spacer-repeat unit.
Description
- This applications claims priority to co-pending U.S. application Ser. Nos. 61/613,373 filed Mar. 20, 2012, and 61/625,420 filed Apr. 17, 2012, each of which is expressly incorporated by reference herein in its entirety.
- Clustered Regularly Interspaced Short Palindromic Repeats (CRISPR) together with cas (CRISPR-associated) genes comprise an adaptive immune system that provides acquired resistance against invading foreign nucleic acids in bacteria and archaea (Barrangou et al., 2007. Science 315:1709-12). CRISPR consists of arrays of short conserved repeat sequences interspaced by unique variable DNA sequences of similar size called spacers, which often originate from phage or plasmid DNA (Barrangou et al., 2007. Science 315:1709-12; Bolotin et al., 2005. Microbiology 151:2551-61; Mojica et al., 2005. J Mol Evol 60:174-82). The CRISPR-Cas system functions by acquiring short pieces of foreign DNA (spacers) which are inserted into the CRISPR region and provide immunity against subsequent exposures to phages and plasmids that carry matching sequences (Barrangou et al., 2007. Science 315:1709-12; Brouns et al., 2008. Science 321: 960-4) The CRISPR-Cas immunity is generally carried out through three stages, referred to as i) adaptation/immunization/spacer acquisition, ii) CRISPR expression/crRNA biogenesis, iii) interference/immunity. (Horvath & Barrangou, 2010. Science 327:167-70; Deveau et al., 2010. Annu Rev Microbiol. 64:475-93;Marraffini & Sontheimer, 2010. Nat Rev Genet 11,181-90; Bhaya et al., Annu Rev Genet 45:273-97; Wiedenheft et al., 2012. Nature 482:331-338). Here, we specifically focus on the interference/immunity step which enables crRNA-mediated silencing of foreign nucleic acids.
- The highly diverse CRISPR-Cas systems are categorized into three major types, which are further subdivided into ten subtypes, based on core element content and sequences (Makarova et al., 2011. Nat Rev Microbiol 9:467-77). The structural organization and function of nucleoprotein complexes involved in crRNA-mediated silencing of foreign nucleic acids differ between distinct CRISPR/Cas types (Wiedenheft et al., 2012. Nature 482:331-338). In the Type I-E system, as exemplified by Escherichia coli, crRNAs are incorporated into a multisubunit effector complex called Cascade (CRISPR-associated complex for antiviral defence) (Brouns et al., 2008. Science 321: 960-4), which binds to the target DNA and triggers degradation by the signature Cas3 protein (Sinkunas et al.,2011. EMBO J 30:1335-42; Beloglazova et al., 2011. EMBO J 30:616-27). In Type III CRISPR/Cas systems of Sulfolobus solfataricus and Pyrococcus furiosus, Cas RAMP module (Cmr) and crRNA complex recognize and cleave synthetic RNA in vitro (Hale et al., 2012. Mol Cell 45:292-302; Zhang et al., 2012. Mol Cell, 45:303-13) while the CRISPR/Cas system of Staphylococcus epidermidis targets DNA in vivo (Marraffini & Sontheimer, Science. 322:1843-5).
- RNP complexes involved in DNA silencing by Type II CRISPR/Cas systems, more specifically in the CRISPR3/Cas system of Streptococcus thermophilus DGCC7710 (Horvath & Barrangou, 2010. Science 327:167-70), consists of four cas genes cas9, cas1, cas2, and csn2, that are located upstream of 12 repeat-spacer units (
FIG. 1A ). Cas9 (formerly named cas5 or csn1) is the signature gene for Type II systems (Makarova et al., 2011. Nat Rev Microbiol 9:467-77). In the closely related S. thermophilus CRISPR1/Cas system, disruption of cas9 abolishes crRNA-mediated DNA interference (Barrangou et al., 2007. Science 315:1709-12). We have shown recently that the S. thermophilus CRISPR3/Cas system can be transferred into Escherichia coli, and that this heterologous system provides protection against plasmid transformation and phage infection, de novo (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82). The interference against phage and plasmid DNA provided by S. thermophilus CRISPR3 requires the presence, within the target DNA, of a proto-spacer sequence complementary to the spacer-derived crRNA, and a conserved PAM (Proto-spacer Adjacent Motif) sequence, NGGNG, located immediately downstream the proto-spacer (Deveau et al., 2008. J Bacteriol 190:1390-400; Horvath et al., 2008. J Bacteriol 190:1401-12; Mojica et al., 2009. Microbiology 155:733-40). Single point mutations in the PAM or defined proto-spacer positions allow the phages or plasmids to circumvent CRISPR-mediated immunity (Deveau et al., 2008. J Bacteriol 190:1390-400; Garneau et al., 2010. Nature 468:67-71; Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82). We have established that in the heterologous system, cas9 is the sole cas gene necessary for CRISPR-encoded interference (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82), suggesting that this protein is involved in crRNA processing and/or crRNA-mediated silencing of invasive DNA. Cas9 of S. thermophilus CRISPR3/Cas system is a large multi-domain protein comprised of 1,409 aa residues (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82). It contains two nuclease domains, a RuvC-like nuclease domain near the amino terminus, and a HNH-like nuclease domain in the middle of the protein. Mutational analysis has established that interference provided in vivo by Cas9 requires both the RuvC- and HNH-motifs (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82). - Isolation of the Cas9-crRNA complex of the S. thermophilus CRISPR3/Cas system as well as complex assembly in vitro from separate components and demonstration that it cleaves both synthetic oligodeoxynucleotide and plasmid DNA bearing a nucleotide sequence complementary to the crRNA, in a PAM-dependent manner, is provided. Furthermore, we provide experimental evidence that the PAM is recognized in the context of double-stranded DNA and is critical for in vitro DNA binding and cleavage. Finally, we show that the Cas9 RuvC- and HNH-active sites are responsible for the cleavage of opposite DNA strands. Taken together, our data demonstrate that the Cas9-crRNA complex functions as an RNA-guided endonuclease which uses RNA for the target site recognition and Cas9 for DNA cleavage. The simple modular organization of the Cas9-crRNA complex, where specificity for DNA targets is encoded by a small crRNA and the cleavage machinery consists of a single, multidomain Cas protein, provides a versatile platform for the engineering of universal RNA-guided DNA endonucleases. Indeed, we provide evidence that by altering the RNA sequence within the Cas9-crRNA complex, programmable endonucleases can be designed both for in vitro and in vivo applications, and we provide a proof of concept for this novel application. These findings pave the way for the development of novel molecular tools for RNA-directed DNA surgery.
- A method for the site-specific modification of a target DNA molecule through contacting under suitable conditions, a target polydeoxynucleotide molecule; and an RNA-guided DNA endonuclease comprising at least one RNA sequence and at least one of an RuvC active site motif and an HNH active site motif; to result in the target polydeoxynucleotide molecule modified in a region that is determined by the complimentary binding of the RNA sequence to the target DNA molecule is provided. The method includes incubating under suitable conditions a composition that includes a target double stranded polydeoxynucleotide or single stranded polydeoxynucleotide; wherein a double stranded polydeoxynucleotide contains a short proto-spacer adjacent motif (PAM), which is non-obligatory for a single stranded polydeoxynucleotide; and where PAM comprises a 5′-NGGNG-3′ sequence; a polyribonucleotide (crRNA) comprising a 3′ and 5′ regions wherein the 3′ region comprises at least 22 nt of the repeat present in a microbe containing CRISPR locus and 5′-region comprises of at least 20 nt of the spacer sequence immediately downstream of the repeat in the CRISPR locus, which is substantially complementary, optionally complementary, to a portion of the target polynucleotide, a polypeptide wherein the amino acid sequence of polypeptide and amino acid sequence of SEQ ID NO: 1 have at least 80% identity, isolated from S. thermophilus, or genetically modified microorganism, including a genetically modified E. coli, or wherein the polypeptide is produced by a method selected from recombinant DNA technology or chemical synthesis; a polyribonucleotide tracrRNA of nucleotide sequence SEQ ID NO: 5 (or have at least 80% identity) comprising a 5′ and 3′ regions wherein the 5′ region is comprised of at least 22 nucleotides is complementary to the 22
nucleotides 3′ region of crRNA, and 3′ region. Wherein polyribonucleotides are produced by in vitro transcription or chemical synthesis. Wherein, suitable conditions means conditions in vitro or in vivo where reaction might occur. - A method for the conversion of Cas9 polypeptide into a nickase, cleaving only one strand of double-stranded DNA, by inactivating one of the active sites (RuvC or HNH) in the polypeptide by at least on point mutation, exemplified by D31A (SEQ ID NO: 2), N891A (SEQ ID NO: 3) and H868A (SEQ ID NO: 4) point mutations, is provided. RuvC motif mutant cleaves only bottom DNA strand in respect to 5′NGGNG-3′ motif, while HNH motif mutant cleaves top strand.
- Polypeptide-polyribonucleotides complex might be isolated from a genetically modified microbe (for example Escherichia coli or Streptoccocus thermophilus), or assembled in vitro from separate components. In the genetically modified microbe components of the complex might be encoded on the one, two or three separate plasmids containing host promoters of the genetically modified microbe or promoters from a native host genome.
- A method for assembly of active polypeptide-polyribonucleotides complex in vitro, comprising incubating the components of the complex under conditions suitable for complex assembly is provided. The complex might be assembled using three or four components. Method for three components assembly comprises incubating the Cas9 polypeptide, 78 nt tracrRNA polyribonucleotide (SEQ ID NO: 5), and 42 nt crRNA polyribonucleotide (5′-NNNNNNNNNNNNNNNNNNNNGUUUUAGAGCUGUGUUGUUUCG-3′) (SEQ ID NO: 15) under conditions suitable for complex assembly. Method for four components assembly comprises incubating the Cas9 polypeptide; 102 nt tracrRNA polyribonucleotide (SEQ ID NO: 6); polyribonucleotide containing
sequence 5′-NNNNNNNNNNNNNNNNNNNNGUUUUAGAGCUGUGUUGUUUCG-3′ (SEQ ID NO: 15) and flanking regions and RNase III polypeptide, cleaving double stranded RNA polynucleotide. The examples forpolyribonucleotide containing sequence 5′-NNNNNNNNNNNNNNNNNNNNGUUUUAGAGCUGUGUUGUUUCG-3′ (SEQ ID NO: 15) are SEQ ID NO: 8, SEQ ID NO: 9, SEQ ID NO: 10, SEQ ID NO: 11 and SEQ ID NO: 12). Examples of source for suitable RNaseIII include Escherichia coli or Streptococcus thermophilus. - A method for re-programming of a Cas9-crRNA complex specificity by mixing separate components or using a cassette containing a single repeat-spacer-repeat unit is provided. Any sequence might be inserted between two repeats in the cassette using suitable restriction endonucleases. Cassette might be used to target sequences in vivo, or to produce RNA ribonucleotide suitable for complex assembly in vitro.
-
FIG. 1 shows Cas9 protein co-purifies with crRNA. (A) Schematic representation of CRISPR3/Cas system of S. thermophilus. Four cas genes (cas9, cas1, cas2, csn2) are located upstream of the CRISPR repeat-spacer array, consisting of 13 repeat (R) sequences and 12 unique spacers (S1-S12). The tracrRNA, required for crRNA maturation in Type II CRISPR systems (Deltcheva et al., 2011. Nature 471:602-7), is located upstream the cas9 gene and encoded on the opposite DNA strand (showed by an arrow) in respect to the other elements of CRISPR3/Cas system. (B) Schematic representation of heterologous loci in two plasmids used for the co-expression of the Cas9-crRNA complex. E. coli RR1 strain contained pCas9(−)1SP (encoding Cas1, Cas2, Csn2, SP1 and tracrRNA) and pASKIBA-Cas9 (encoding Strep-tagged version of Cas9) plasmids. (C) Northern analysis of Cas9-crRNA complexes using anti-crDNA oligonucleotide as a probe. M1-84 nt oligodeoxynucleotide corresponding to the spacer S1-repeat unit; M2-42 nt synthetic oligoribonucleotide corresponding to the predicted S. thermophilus CRISPR3 crRNA (SeeFIG. 4 ); crRNA (wt)-crRNA isolated from the wt Cas9 complex; K1-crRNA (wt) treated with Dnase I for 15 min; K2-crRNA (wt) treated with RNasel for 15 min, D31A-crRNA purified from the Cas9 D31A mutant complex; N891A-crRNA purified from the Cas9 N891A mutant complex. -
FIG. 2 shows DNA cleavage by Cas9-crRNA complexes obtained by Cas9 co-expression with full length CRISPR locus. (A) Schematic representation of CRISPR/Cas locus of recombinant pCas9(−) plasmid carrying indigenous 12 spacer-repeat array of SthCRISPR3/Cas system and pASKIBA-Cas9 plasmid carrying cas9 gene with a Strep-tag at the C-terminus. (B) Oligoduplex cleavage assay. Both pCas9(−) and pASKIBA-Cas9 plasmids were co-expressed in E. coli, Cas9-crRNA complexes were purified and subjected to cleavage analysis using SP1 (first proto-spacer) and SP2 (second proto-spacer) oligoduplexes labeled with 33P at the 5′-end of the (+) strand. Reaction products were analysed on PAA gel. -
FIG. 3 shows immunity against plasmid transformation in E. coli cells provided by the SthCRISPR3/Cas system. (A) Schematic representation of CRISPR/Cas locus of recombinant plasmid pCRISPR3 carrying indigenous 12 spacer-repeat array of SthCRISPR3/Cas system and engineered pCRISPR3-SP1 plasmid carrying 1 spacer-repeat unit. (B) Interference of plasmid transformation by SthCRISPR3/Cas system in E. coli cells. Escherichia coli RR1 recipient strains carrying plasmids pACYC184, pCRISPR3 or pCRISPR3-SP1, were transformed with plasmid pSP1 carrying proto-spacers and PAM or pUC18 (1). Transformation efficiency is expressed as cfu per nanogram of plasmid DNA (mean±SD). -
FIG. 4 shows comparison of Type IIA CRISPR/Cas systems from S. thermophilus DGCC7710, LMD-9 and S. pyogenes SF370 strains. (A) Schematic organization of the CRISPR/Cas systems. Nucleotide sequences corresponding to the tracrRNA required for the crRNA maturation in of S. pyogenes (2) are present in LMD-9 and DGCC7710. Percentage of identical and similar (in parenthesis) residues between corresponding protein sequences that are connected by dashed lines. (B). Alignment of the conserved repeat sequences and tracrRNA. Corresponding sequences from DGCC7710 and LMD-9 are identical. Nucleotide positions which are identical in all three strains are labeled with an asterisk below aligned sequences. (B) disclosesSEQ ID NOS 50, 50-52, and 52-53, respectively, in order of appearance. (C) Comparison of crRNA sequences. The sequence and length of S. pyogenes crRNA was determined by deep sequencing analysis (2). The approximate length of crRNA from S. thermophilus LMD-9 (2) and DGCC7710 (this work) strains were determined by the northern blot analysis. (C) discloses SEQ ID NOS 54-56, respectively, in order of appearance. -
FIG. 5 shows Cas9-crRNA complex cleaves in vitro double-stranded DNA within a proto-spacer. (A) Oligoduplex substrate used in the cleavage assay. 55 nt oligoduplex SP1 contains the proto-spacer1(red letters), PAM (blue letters) and 10 nt flanking sequences on both sides identical to those in pSP1 plasmid. In the SP1 oligoduplex DNA strand complimentary to the 5′-terminal fragment of crRNA (red letters) is named (+)strand, an opposite DNA strand is named (−)strand. (A) disclosesSEQ ID NOS 31, 7, and 34, respectively, in order of appearance. (B) Oligoduplex SP1 cleavage. 2.5 nM of Cas9-crRNA complex and 1 nM SP1 oligoduplex labeled with 33P at the 5′-end of either (+) or (−) strand were incubated in the reaction buffer (10 mM Tris-HCl pH=7.5, 10 mM NaCl, 10 mM MgCl2, 0.1 mg/ml BSA) at 37° C. for varied time intervals (30 s to 10 min) and reaction products analysed in the 20% PAA gel. Lanes M1 and M2 contain chemically synthesized 5′-end 33P-labeled 37 nt and 18 nt oligodeoxynucleotides corresponding to the cleavage products of (−) and (+) DNA strands, respectively. Cleavage positions are designated by arrows. (B) discloses SEQ ID NO: 31. (C) Schematic representation of pSP1 plasmid (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) used in the plasmid cleavage assay. (C) discloses SEQ ID NO: 57. (D) pSP1 plasmid cleavage. Agarose gel analysis of pSP1 cleavage products (left panel). SC—super-coiled plasmid DNA, OC—open circular DNA nicked at one of the strands, FLL—full length linear DNA cut at both strands. Final reaction mixtures at 37° C. contained 2.5 nM of pSP1 plasmid and 2.5 nM of Cas9-crRNA complex in the reaction buffer (section B). Direct sequencing electropherograms (right panel) of (+) (upper part) and (−) (lower part) strands of pSP1 plasmid cleavage product. The non-templated addition of adenine (T in the reverse complement sequence shown here) at the extremity of sequence is a sequencing artefact caused by the polymerase. (D) disclosesSEQ ID NOS 58, 59, 58, and 60, respectively, in order of appearance. -
FIG. 6 shows DNA binding and cleavage analysis of Cas9-Chis protein lacking crRNA. Electrophoretic mobility shift analysis (EMSA) of Cas9-Chis protein binding to (A) the double stranded SP1 oligoduplex and (B) the single stranded s(+)SP1 oligonucleotide. Electrophoretic mobility shift experiments were performed in the binding buffer (40 mM Tris-acetate, pH 8.3 at 25 C, 0.1 EDTA, 0.1 mg/ml BSA, 10% v/v glycerol). The reactions contained 0.5 nM of the 33P-labelled oligoduplex, and the protein at concentrations as indicated above each lane. (C). Oligonucleotide cleavage assay. 5 nM of Cas9-Chis protein was incubated in the reaction buffer (10 mM Tris-HCl, pH=7.5, 10 mM NaCl, 10 mM MgCl2, 0.1 mg/ml BSA) at 37° C. with 1 nM oligonucleotide. SP1 oligoduplex was labeled with 33P at the 5′-end of the (+) or (−) strand. Single stranded oligonucleotide s(+)SP1 was labeled with 33P at the 5′-end. -
FIG. 7 shows reprograming of Cas9-crRNA complex. (A) Schematic representation of heterologous loci in two plasmids used for reprogramming of Cas9-crRNA complex. pCas(−)SPN were constructed from pCas9(−) plasmid (SeeFIG. 2 ), by inserting new spacer sequence (SN) (5′-CC ACC CAG CAA AAT TCG GTT TTC TGG CTG-3′ (SEQ ID NO: 16)) and inactivating Cas9 gene as described in (1). (B) Agarose gel analysis of plasmid DNA cleavage products. pSP1 and pSP1+SPN (pSP1 plasmid with inserted new proto-spacer and PAM over AatII site were incubated at 2.5 nM concentration with 2 nM of Cas9-crRNA complex in the reaction buffer (10 mM Tris-HCl pH=7.5, 10 mM NaCl, 10 mM MgCl2, 0.1 mg/ml BSA) at 37° C. for varied time intervals and reaction products analysed in the agarose gel. SC—super-coiled plasmid DNA, OC—open circular DNA nicked at one of DNA strands, FLL—full length linear DNA cut at both strands. (C) Oligoduplex SP1 cleavage. 2.5 nM of Cas9-crRNA complex and 1 nM SPN oligoduplex (Table S2) labeled with 33P at the 5′-end of either (+) or (−)strand were incubated in the reaction buffer (10 mM Tris-HCl pH=7.5, 10 mM NaCl, 10 mM MgCl2, 0.1 mg/ml BSA) at 37° C. M1-18 nt length marker Lanes M1 and M2 contain chemically synthesized 5′-end 33P-labeled 18 nt and 37 nt oligodeoxynucleotides corresponding to the cleavage products of (+) and (−) DNA strands, respectively. (D) Schematic representation of SPN oligoduplex substrate and cleavage products. SPN oligoduplex contains the new proto-spacer (red letters), PAM (blue letters). Cleavage positions are designated by arrows. (D) discloses SEQ ID NO: 39. -
FIG. 8 shows impact of spacer length on CRISPR-encoded immunity. (A) Schematic representation of shortened versions of proto-spacers inserted in the transformed plasmids. (A) disclosesSEQ ID NOS 7 and 61-66, respectively, in order of appearance. (B) Effect of proto-spacer length on the plasmid transformation efficiency. Transformation efficiency is expressed as cfu per nanogram of plasmid DNA (mean±SD). (C). Schematic representation of oligoduplexes used in the in vitro cleavage and binding experiments. (C) discloses SEQ ID NOS 31 and 38, respectively, in order of appearance. (D) Time courses of the 27 by oligoduplex (full length protospacer SP1, filled circles) and the 20 by oligoduplex (truncated protospacer SP1-20, square) cleavage by the Cas9-crRNA complex. (E) Electrophoretic mobility shift assay of SP1 and SP1-20 oligoduplex binding by the Cas9-crRNA complex. -
FIG. 9 shows PAM is required for in vitro DNA binding and cleavage by the Cas9-crRNA complex. (A) Agarose gel analysis of plasmid DNA cleavage products. Three different plasmids: PAM+Proto-spacer+ (pSP1 plasmid containing both the proto-spacer and PAM), PAM-Protospacer-(pUC18 plasmid containing multiple PAMs but no protospacer) and PAM-Protospacer+ (pSP1-pΔ (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) containing a proto-spacer without PAM) were incubated at 2.5 nM concentration with 2 nM of Cas9-crRNA complex in the reaction buffer (10 mM Tris-HCl pH=7.5, 10 mM NaCl, 10 mM MgCl2, 0.1 mg/ml BSA) at 37° C. for varied time intervals and reaction products analysed in the agarose gel. SC—super-coiled plasmid DNA, OC—open circular DNA nicked at one of DNA strands, FLL—full length linear DNA cut at both strands. (B) Time courses of (+)strand hydrolysis in the single-stranded and double-stranded oligodeoxynucleotides. Reactions containing 2 nM Cas9-crRNA and 1 nM of oligodeoxynucleotide were conducted at 37° C. in the reaction buffer (section A). SP1 (filled circles) and SP1-pΔ (open squares) oligoduplexes were used as dsDNA. s(+)SP1 (open triangles) and s(+) SP1-pΔ (filled squeres) were used as ssDNA. (C) and (D) dsDNA and ssDNA (+)strand) binding by Cas9-crRNA complex. The reactions contained 0.5 nM of the 33P-labelled ssDNA or dsDNA oligonucleotide, and the protein at concentrations as indicated above each lane. After 15 min at room temperature, the samples were subjected to PAGE for 2 h and analysed as described in ‘Materials and Methods’ -
FIG. 10 shows RNA binding and cleavage analysis of Cas9-crRNA complex. (A) - Electrophoretic mobility shift analysis (EMSA) of Cas9-crRNA complex binding to 84 nt RNA fragment containing proto-spacer-1, PAM and 24 nt flanking sequences on both sides. Left panel: RNA (−) strand; center panel: RNA (+) strand; right panel: double stranded RNA. RNA fragments used for analysis were generated by in vitro transcription (TranscriptAid™ T7 High Yield Transcription Kit, Fermentas) from PCR fragments with inserted T7 promoter at the front end of RNA coding sequence. PCR fragments coding (+) and (−) RNA strands were obtained from pSP1 plasmid (1) with following primer pairs accordingly: 5′
taatacgactcactataGggtaccgagctcgaattg 3′ (SEQ ID NO: 17)/5′ GGGAAACAGCTATGACCATGATTACGAATTC-3′ (SEQ ID NO: 18) and 5′gggtaccgagctcgaattgaaattcTAAACG 3′ (SEQ ID NO: 19)/5′taatacgactcactataGggAAACAGCTATGACCATGATTACG 3′ (SEQ ID NO: 20) (T7 RNA polymerase promoter underlined, transcription start on bold). The reactions contained 1 nM of the 33P-labelled RNA fragment, and the protein at concentrations as indicated above each lane. After 15 min at room temperature, the samples were subjected to PAGE for 2 h and analyzed as described in ‘Materials and Methods’. (B) RNA cleavage assay. 2.5 nM of Cas9-crRNA complex was incubated in the reaction buffer (10 mM Tris-HCl pH=7.5, 10 mM NaCl, 10 mM MgCl2, 0.1 mg/ml BSA,) at 37° C. in the presence of 1 nM (+) and (−) RNA strands(left panel) or double stranded RNA labeled on (+) or (−) strand (right panel). Reaction products were analysed on denaturing PAA gel. -
FIG. 11 shows RuvC and HNH active site motifs of Cas9 contribute to the cleavage of opposite DNA strands. (A) Localization of the conserved active site motifs within Cas9 protein. Amino acid residues identified as crucial for Cas9 in vivo activity (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) are indicated. (B). Agarose gel analysis of pSP1 plasmid cleavage by Cas9 and mutant proteins. Reactions were performed as described in and ‘Materials and Methods’ (C) Strand preference of D31A mutant. Reactions were performed as described inFIG. 2 and ‘Materials and Methods’. D31 mutant cleaves only (+)strand of SP1 oligoduplex. (C) discloses SEQ ID NOS 31. (D) Strand preference of N891A mutant. N891 mutant cleaves only (−)strand of SP1 oligoduplex. Cleavage positions are designated by arrows. (D) discloses SEQ ID NOS 31. -
FIG. 12 shows properties of Cas9 active site mutant-crRNA complexes. (A) Direct sequencing of reaction products obtained with Cas9 mutant D31A (RuvC-like active site motif). (A) discloses SEQ ID NOS 58, 59, 58, and 58, respectively, in order of appearance. (B) Direct sequencing of reaction products obtained with Cas9 N891A mutant (HNH-like active site motif). (B) disclosesSEQ ID NOS 58, 58, 58, and 60, respectively, in order of appearance. (C) SP1 oligoduplex binding by the wt Cas9-crRNA and active site mutant complexes. (D) Cleavage of (+)SP1 strand by Cas9-crRNA mutant complexes. -
FIG. 13 shows molecular mass of the wt Cas9-Chis protein. Gel filtration experiments were carried out at roomtemperature using Superdex 200 10/300 GL column (GE healthcare) pre-equilibrated with 10 mM sodium phosphate (pH 7.4) buffer containing 500 mM sodium chloride. The apparent Mw of Cas9 (black triangle) were calculated by interpolation from the standard curve obtained using a set of proteins of known Mw (black circles) (Bio-Rad Gel Filtration Standards). -
FIG. 14 shows schematic arrangement and mechanism of crRNA-directed DNA cleavage by the Cas9-crRNA complex. Domain architecture of Cas9 is shown schematically on the top. Cas9-crRNA complex binds to the dsDNA containing PAM. crRNA binds to the complementary (+)strand resulting in DNA strand separation and the R-loop formation. In the ternary complex RuvC active site of Cas9 is positioned at the scissile phosphate on the unpaired (−)strand, while HNH active site is located at the scissile phosphate on the DNA (+)strand bound to crRNA. Coordinated action of both active sites results in thedouble strand break 3 nt away from the 5′-NGGNG-5′ PAM generating blunt end DNA.FIG. 14 discloses SEQ ID NOS. 31 and 7, respectively, in order of appearance. -
FIG. 15 shows native electrophoresis of Cas9-crRNA and cleavage products. The protein at concentrations as indicated above each lane, where incubated in the reaction buffer (10 mM Tris-HCl pH=7.5, 10 mM NaCl, 10 mM MgCl2, 0.1 mg/ml BSA) at 37° C. for 30 min in the presence of 0.5 nM SP1 oligoduplex. Samples was mixed with loading dye solution (0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol) and analysed by non-denaturing PAGE. The gel lanes marked M—melted form of cleavage reactions products. The cartoons in each side of the gel illustrate protein-DNA complexes and DNA that correspond to each band, while cartoons below the gel illustrate major substrate form after reaction. -
FIG. 16 shows plasmid DNA cleavage by Cas9-crRNA complex. (A) pSP1 and pUC18 plasmid DNA cleavage. Cas9-crRNA complex was incubated with pSP1 and pUC18 plasmids in a reaction buffer provided in the Example 1. pSP1 plasmid contained a proto-spacer1 sequence flanked by the the 5′-NGGNG-3′ PAM sequence. Proto-spacer1 sequence was not present in pUC18. Reaction products were analysed in the agarose gel. Under these conditions pSP1 plasmid is converted into a linear form while pUC18 plasmid lacking proto-spacer1 sequence is resistant to cleavage. (B) pSP1 cleavage reactions in the absence of one of the components. In the reaction mixes lacking one of the components (Cas9, crRNA or tracrRNA, respectively) pSP1 plasmid is not cleaved. SC—super-coiled plasmid DNA, OC—open circular DNA nicked at one of DNA strands, FLL—full length linear DNA cut at both strands. -
FIG. 17 shows DNA oligoduplex cleavage by Cas9-crRNA complex. The strand of oligoduplex which is complementary to crRNA is marked as (+) strand, while the other strand—(−) strand. To monitor cleavage reactions either (+) or (−) strand of the oligoduplex was P33-labeled at the 5′-terminus. M1 and M2 are synthetic oligonucleotide markers corresponding to the 37 nt of (−) strand and 18 nt of (+) strand which were used to determine the size of the cleavage products and map the cleavage position. Cas9 protein cleaves both strands of oligoduplex inside the proto-spacer, after the 37th nucleotide, 3 nt upstream of the PAM (5′-NGGNG-3′) leaving blunt ends. Both strands of non-specific substrate (K1 and K2) are not cleaved when incubated with Cas9-crRNA complex for 30 min.FIG. 17 discloses SEQ ID NO: 31. -
FIG. 18 shows plasmid DNA cleavage by Cas9-crRNA complex assembled in the absence of RNaseIII. Cas9-crRNA complex was incubated with pSP1 plasmid and reaction products analysed in the agarose gels. The pSP1 plasmid is resistant for cleavage in the presence of complex assembled without crRNA (left panel). The pSP1 plasmid is converted into linear form in the presence of complex assembled using synthetic 42 nt crRNA (no RNAseIII) (middle panel). The pSP1 plasmid is converted into a mixture of linear and circular DNA forms in the presence of complex assembled using CRISPR RNA transcript (no RNAseIII) (right panel). -
FIG. 19 shows DNA oligoduplex cleavage by Cas9-crRNA complex. The strand of oligoduplex which is complementary to crRNA is marked as (+) strand, while the other strand—(−) strand. To monitor cleavage reaction either (+) or (−) strand of the oligoduplex was P33-labeled at the 5′-terminus. M1 and M2 are synthetic oligonucleotide markers corresponding to the 37 nt of (−) strand and 18 nt of (+) strand which were used to determine the size of the cleavage products and map the cleavage position. Cas9 protein cleaves both strands of oligoduplex inside the proto-spacer, after the 37th nucleotide form the 5′-end, 3 nt upstream of the PAM (5′-NGGNG-3′) leaving blunt ends. Both strands of non-specific substrate (K1 and K2) are not cleaved when incubated with Cas9-crRNA complex for 30 min.FIG. 19 discloses SEQ ID NO: 31. -
FIG. 20 shows (A) Schematic representation of the CRISPR3/Cas system of S. thermophilus DGCC7710. Four cas genes (cas9, cas1, cas2, csn2) are located upstream of the CRISPR repeat-spacer array, consisting of 13 repeat (R) sequences and 12 unique spacers (S1-S12). The tracrRNA, required for crRNA maturation in Type II CRISPR/Cas systems (Deltcheva et al.,2011. Nature 471, 602-7), is located upstream the cas9 gene and encoded on the opposite DNA strand (shown by an arrow) with respect to the other elements of this system. (B) The pathways for a new spacer insertion in to CRISPR region and CRISPR RNA synthesis. Synthetic oligoduplex encoding desired spacer sequence and containing Sapl and Eco31I restriction compatible ends was inserted between two repeats. The CRISPR region was amplified using PCR. The new spacer encoding CRISPR RNA was obtained by In vitro transcription. (C) In vitro assembly of Cas9-RNA complex. The CRISPR RNA and tracrRNA transcripts were assembled in to duplex. The Cas9 protein was first pre-incubated with RNA duplex, followed by the subsequent incubation with RNAseIII to generate a catalytically competent Cas9-RNA complex. -
FIG. 21 shows A. Schematic representation of pUC18 plasmid. The distance between Sapl and AatII restriction sites is 775 bp, while the distance between two spacers is 612 bp. B. pUC18 plasmid cleavage by re-programed Cas9-crRNA complexes. “1”—pUC18 plasmid; “2”—pUC18 cleaved with AatII; “3”—pUC18 cleaved with complex containing crRNA matching proto-spacer1; “4”—pUC18 cleaved with Sapl; “5”—pUC18 cleaved with complex containing crRNA matching proto-spacer2; “6”—pUC18 cleaved with AatII and Sapl; “7”—pUC18 cleaved with mix of the complexes used in theline -
FIG. 22 shows genomic DNA cleavage with in vitro assembled Cas9-RNA complex. (A) Agarose gel analysis of linear A DNA cleavage products. Phage A DNA was incubated with Cas9-RNA complex in the reaction buffer for various time intervals. The target site for Cas9-RNA complex is located 8 kb away from the cos site. (B). Probe selection for Southern blot experiments. Genomic DNA was fragmented by treating with Pstl enzyme. The proto-spacer is located between two Pstl sites. If genomic DNA is cleaved with Cas9-RNA complex, 466 by fragment should be detected. Otherwise the probe will hybridize with 1499 by length fragment. (C) Southern blot analysis of genomic DNA fragments. C line—E. coli genomic DNA fragmented with Pstl. Cas9-RNA—genomic DNA was incubated with Cas9-RNA complex before fragmentation. (D). Human genomic DNA cleavage by Cas9-crRNA complex. Relative amount of intact DNA DNA fragments were estimated by qPCR. - The following non-limiting examples further describe the methods, compositions, uses, and embodiments.
- In this example, we have isolated the Cas9-crRNA complex of S. thermophilus CRISPR3/Cas system and demonstrate that it cuts in a PAM dependent manner both synthetic oligodeoxynucleotide and plasmid DNA bearing a nucleotide sequence complementary to the crRNA. Furthermore, we provide experimental evidence that PAM is recognized in the context of double-stranded DNA and is critical for in vitro DNA binding and cleavage. Finally, we show that RuvC and HNH- motifs of Cas9 contribute to the cleavage of opposite DNA strands. Taken together, our data demonstrate that Cas9-crRNA complex functions as RNA-guided endonuclease which uses RNA module for the target site recognition and employs two separate active sites in the protein module for DNA cleavage. These findings pave the way for engineering of programable Cas9-crRNA complexes as universal RNA-guided endonucleases.
- DNA manipulations. Genomic DNA of Streptococcus thermophilus DGCC7710 strain was used as a template in PCR reactions to clone cas9. To generate a pASKIBA3-Cas9 plasmid which was used for the expression of the C-terminal Strep-tagged Cas9 protein variant, PCR fragment amplified with following primers: 5′-ACGTCTCAAATGTTGTTTAATAAGTGTATAATAATTTC-3′ (SEQ ID NO: 21) and 5′-ACGTCTCCGCGCTACCCTCTCCTAGTTTG-3′ (SEQ ID NO: 22) was cloned into the pASK-IBA3 expression vector via Esp3l sites. To generate a pBAD-Cas9 plasmid which was used for the expression of the C-terminal 6× His-tagged Cas9 protein variant (“6× His” disclosed as SEQ ID NO: 23), PCR fragment amplified with the following primer pair: 5′-ACGTCTCACATGACTAAGCCATACTCAATTGGAC-3′ (SEQ ID NO: 24) and 5′-ACTCGAGACCCTCTCCTAGTTTGGCAA-3′ (SEQ ID NO: 25) was cloned into the pBAD24-Chis expression vector via NcoI and XhoI sites. Full sequencing of cas9 gene in pASKIBA3-Cas9 and pBAD-Cas9 plasmids revealed no difference with the original cas9 sequence. To obtain plasmids pCas9(−)SP1 (
FIG. 1B ) and pCRISPR3-SP1 (FIG. 2A ), bearing a single spacer1, PCR fragment amplified from pCRISPR3 plasmid with the following primer pair:5′GACCACTTATTGAGGTAAATGAG 3′ (SEQ ID NO: 26)/5′ CAAACCAGGATCCAAGCTAATACAGCAG-3′ (SEQ ID NO: 27) ((BamHI (GGATCC) sites is underlined) was cloned into pCas9(−) and pCRISPR3 plasmids (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82), respectively. - Expression and purification of Cas9 protein and Cas9-crRNA complex. 6xHis-tagged (“6× His” disclosed as SEQ ID NO: 23) version of Cas9 protein was expressed and purified using a scheme described for the Cas3 protein from S. thermophilus CRISPR4/Cas system (Sinkunas et al.,2011. EMBO J 30:1335-42). For purification of the Cas9-crRNA complex, Strep-tagged version of the Cas9 protein was expressed in E. coli RR1 strain, bearing pCas9(−)SP1 plasmid (
FIG. 1B ). LB broth was supplemented with Ap (100 μg/ml) and Cm (10 μ/ml. E. coli cells for the Cas9-crRNA complex isolation were grown in two steps. First, 4 ml of cells culture were grown at 37° C. to OD600 of ˜0.5, and expression induced by adding 0.2 μg/ml of anhydrotetracycline (AHT) (Sigma). After for 4 h, 1/400 of the pre-induced culture was inoculated into fresh LB medium supplemented with Ap (100 μg/ml), Cm (12 μg/ml) and AHT (0.2 μg/ml) and was grown at 37° C. overnight. Harvested cells were disrupted by sonication and cell debris removed by centrifugation. The supernatant was loaded onto the 1 ml StrepTrap HP column (GE Healthcare) and eluted with 2.5 mM of desthiobiotin. Approximately 1.5 μg of the Cas9 protein was obtained in a single run from 1 L of E. coli culture. The fractions containing Cas9 were stored at +4° C. for several days. The homogeneity of protein preparations was estimated by SDS-PAGE. Protein concentrations in the Cas9-crRNA complexes were determined by densitometric analysis of SDS-PAGE gels containing samples of Strep-Tactin purified Cas9 proteins along with known amounts of His-tagged Cas9 protein. The concentration of the Cas9-crRNA complexes is expressed as Cas9 protein concentration assuming that Cas9 is a monomer and binds crRNA in a complex with 1:1 stoichiometry. - Northern blot analysis. Cas9-bound RNA was isolated from Strep-Tactin purified Cas9, co-expressed with pCas9(−)SP1 plasmid using the miRNeasy Mini kit (Qiagen). Northern blots were performed by running RNA on a 10% polyacrylamide gel with 7 M urea in 20 mM MOPS/
NaOH pH 8 buffer. The RNA was transferred to a SensiBlot™ Plus Nylon Membrane (Fermentas) by semi-dry blotting using a Trans-blot SD (Bio-Rad). RNA was cross-linked to the membrane with 0.16 M l-ethyl-3-(3-dimethylaminopropyl) carbodiimide (EDC) (Pierce)/0.13 M 1-methylimidazole (Sigma)pH 8 at 60° C. for 1 h. The membrane was pre-hybridized with 2×SSC buffer containing 1% SDS and 0.1 mg/ml denatured DNA from fish testes (Ambion) for 1 h at 40° C. Blots were probed for 12 h with a 32P-5′-labelled 42 nt anti-crRNA DNA oligonucleotide containing 20 nt of spacer1 and 22 nt of the repeat sequence (5′-TCGAAACAACACAGCTCTAAAACTGTCCTCTTCCTCTTTAGC-3′ (SEQ ID NO: 28)). The blots were washed 3× for 15 min with 0.2×SSC buffer containing 0.2% SDS, and were visualized using phosphorimaging. A 42 nt synthetic oligoribonucleotide (5′-CGCUAAAGAGGAAGAGGACAGUUUUAGAGCUGUGUUGUUUCG-3′ (SEQ ID NO: 7)) and 84 nt DNA oligonucleotide. - Oligonucleotide substrates. All oligonucleotide substrates used in this study are given in Table 1. Oligodeoxyribonucleotides were purchased from Metabion (Martinsried, Germany). The 5′-ends of oligonucleotides were radiolabelled using PNK (Fermentas) and [y-33P]ATP (Hartmann Analytic). Duplexes were made by annealing two oligonucleotides with complementary sequences (SP1, SP1-Δp, SP2). Radioactive label was introduced at the 5′ end of individual DNA strand prior to the annealing with unlabelled strand.
- Reactions with oligonucleotide substrates. Reactions were typically carried out by adding 2 nM of Cas9-crRNA complex to 1 nM labeled oligonucleotide in 10 mM Tris-HCl (pH 7.5 at 37° C.), 10 mM NaCl, 0.1 mg/ml BSA and 10 mM MgCl2 at 37° C. Aliquots were removed at timed intervals and quenched with loading dye (95% v/v formamide, 0.01% bromphenol blue, 25 mM EDTA, pH 9.0) and subjected to denaturing gel electrophoresis through 20% polyacrylamide followed by a FLA-5100 phosphorimager (Fujilm) detection.
- Reactions with plasmid substrates. Reactions on pUC18 plasmid and its derivatives (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) were conducted at 37° C. in the buffer used for reactions on oligonucleotide substrates. Reaction mixtures typically contained 2.5 nM supercoiled plasmid and 2 nM of Cas9-crRNA complex. The reactions were initiated by adding protein to the mixture of the other components. Aliquots were removed at timed intervals and quenched with phenol/chloroform. The aqueous phase was mixed with loading dye solution (0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol) and analyzed by electrophoresis through agarose.
- Plasmid cleavage position determination. To achieve complete cleavage of plasmid substrate, 8 nM of Cas9-crRNA complex was incubated with 2.5 nM of supercoiled plasmid in the reaction buffer at 37° C. for 10 min. Reaction products were purified and concentrated using GeneJET PCR Purification Kit (Fermentas). Spacer1 surrounding region of Cas9 linearized and nicked plasmids were directly sequenced with the following primers: 5′-ccgcatcaggcgccattcgcc-3′ (SEQ ID NO: 29) (sequencing of (+)strand) and 5′-gcgaggaagcggaagagcgccc-3′ (SEQ ID NO: 30) (sequencing of (−)strand).
- Binding assay. Increasing amounts of protein-crRNA complex were mixed with 0.5 nM of 33P-labeled double-stranded and single-stranded DNA substrates (Table 1) in the binding buffer (40 mM Tris-acetate, pH 8.3 at 25 C, 0.1 EDTA, 0.1 mg/ml BSA, 10% v/v glycerol) and incubated for 15 min at room temperature. Free DNA and protein-DNA complexes were separated on the non-denaturing 8% polyacrylamide gel (ratio of acrylamide/N,N′-methylenebisacrylamide 29:1) using 40 mM Tris-acetate (pH 8.3) supplemented with 0.1 mM EDTA as the running buffer. Electrophoresis was run at room temperature for 3 h at 6 V/cm.
- Mutagenesis. The mutants D31A and N891A were obtained by the site-directed mutagenesis as previously described (Tamulaitis et al., 2007. Nucleic Acids Res 35:4792-9). Sequencing of the entire gene for each mutant confirmed that only the designed mutation had been introduced.
-
TABLE 1 Oligonucleotide substrates. Proto-spacer sequence is underlined, PAM is on bold. Oligonucleotide Sequence Specification SP1 5′-GCTCGAATTGAAATTCTAAACGCTAAAGAGGAAGAGGACATGGTGAATTCGTAAT-3 55 bp oligoduplex (SEQ ID NO: 31) 3′-CGAGCTTAACTTTAAGATTTGCGATTTCTCCTTCTCCTGTACCACTTAAGCATTA-5′ substrate containing proto-spacer1 and PAM SP1-pΔ 5′-GCTCGAATTGAAATTCTAAACGCTAAAGAGGAAGAGGACAAATTCGTAAT-3′ 50 bp oligoduplex (SEQ ID NO: 32) 3′-CGAGCTTAACTTTAAGATTTGCGATTTCTCCTTCTCCTGTTTAAGCATTA-5′ substrate containing proto-spacer2 SP2 5′-GCTCGAATTGTACTGCTGTATTAGCTTGGTTGTTGGTTTGTGGTGAATTCGTAAT-3′ 55 bp oligoduplex (SEQ ID NO: 33) 3′-CGAGCTTAACATGACGACATAATCGAACCAACAACCAAACACCACTTAAGCATTA-5′ substrate containing proto-spacer2 and PAM (oligoduble without proto-spacer1) s(+) SP1 5′-ATTACGAATTCACCATGTCCTCTTCCTCTTTAGCGTTTAGAATTTCAATTCGAGC-3′ 55 nt ssDNA (SEQ ID NO: 34) oligonucleotide substrate (+) strand of SP1 oligoduplex s(+) SP1-p 5′-ATTACGAATTTGTCCTCTTCCTCTTTAGCGTTTAGAATTTCAATTCGAGC-3′ 50 nt ssDNA (SEQ ID NO. 35) oligonucleotide substrate (+) strand of SP1-Δ oligoduplex s(+) SP2 5′-ATTACGAATTCACCACAAACCAACAACCAAGCTAATACAGCAGTACAATTCGAGC-3′ 55 nt ssDNA (SEQ ID NO: 36) oligonucleotide substrate (+) strand of SP2 oligoduplex s(−) SP1 5′-GCTCGAATTGAAATTCTAAACGCTAAAGAGGAAGAGGACATGGTGAATTCGTAAT-3′ 55 nt ssDNA (SEQ ID NO: 37) oligonucleotide substrate, ) strand of SP1 oligoduplx SP1-20 5′-GCTCGAATTGCGCTAAAGAGGAAGAGGACATGGTGAATTCGTAAT-3 45 nt oligoduplex (SEQ ID NO: 38) 3′-CGAGCTTAACGCGATTTCTCCTTCTCCTGTACCACTTAAGCATTA-5′ substrate containing 2 nt of proto-spacerl and PAM SPN 5′-GCTCGAATTGCCACCCAGCAAAATTCGGTTTTCTGGCTGATGGTGAATTCGTAAT-3′ 55 by oligoduplex (SEQ ID NO: 39) 3′-CGAGCTTAACGGTGGGTCGTTTTAAGCCAAAAGACCGACTACCACTTAAGCATTA-5 substrate containing proto-spacerN and PAM indicates data missing or illegible when filed - Expression and purification of the Cas9-crRNA complex. The cas9 gene from the CRISR3 system of S. thermophilus DGCC7710 strain was cloned into the pASK-IBA3 vector to produce a construct encoding a Cas9 protein fusion containing a C-terminal Strep(II)-tag (
FIG. 1B ). Initially, we have tried to purify Cas9-crRNA complex from E. coli strain RR1 expressing Cas9 protein on the pASK-IBA3 vector and other Cas proteins (except Cas9) on pCas9(−) plasmid (Sapranauskas et al, 2011). pCas9(−) also contained a complete CRISPR3 array comprised of 12 spacer-repeat units (FIG. 2A ). To achieve simultaneous transcription of all target genes we performed cas9 gene expression in two steps. First, we induced Cas9 expression in a small volume of E. coli culture and after 4 h transferred an aliquot of pre-induced culture into a larger volume of fresh LB media already containing inductor and incubated overnight. Cas9 protein complex was purified from the crude cell extract using Strep-Tactin Sepharose. We managed to isolate a small amount of the Cas9-crRNA complex which showed only traces of nucleolytic activity on the oligoduplex SP1 containing a proto-spacer1 and PAM. We assumed that low cleavage activity could be due to the intrinsic heterogeneity of Cas9-crRNA complexes resulting from the transcription of 12 spacer-repeat units. If all spacer-repeat units are uniformly transcribed into a mature crRNA, the concentration of the Cas9 complex containing crRNA against spacer-1 will make 1/12th fraction of the total Cas9-crRNA concentration. The cleavage activity of the Cas9-crRNA preparation against the SP2 oligoduplex containing a proto-spacer-2 and PAM is consistent with the heterogeneity of Cas9-crRNA complexes (FIG. 2B ). To increase the yield of the specific Cas9-crRNA complex we engineered a pCas9(−)SP1 plasmid which contains a single R-spacer1-R unit in the CRISPR array (FIG. 1B ). Plasmid transformation interference assay confirmed that the CRISPR3/Cas system carrying a single spacer1 prevents plasmid pSP1 transformation in E. coli with the same efficiency as the CRISPR3/Cas system carrying a complete CRISPR region (FIG. 3B ). We have isolated Cas9-crRNA complex following the procedure described above and analysed crRNA bound to Cas9 protein. - Cas9 protein co-purifies with crRNA. CRISPR3/Cas system of S. thermophilus belongs to the Type IIA subtype (former Nmeni or CASS4) of CRISPR/Cas systems (Makarova et al., 2011. Nat Rev Microbiol 9:467-77). It has been shown that in the Type IIA CRISPR/Cas system of Streptococcus pyogenes trans-encoded small RNA (tracrRNA) and bacterial RNaseIII are involved in the generation of crRNA (Deltcheva et al., 2011. Nature 471:602-7). Streptococcus pyogenes crRNA is only 42 nt in length and has no “5′-handle” which is conserved in crRNA's from Type I and III CRISPR systems (Hale et al., 2009. Cell 139:945-56; Jore et al., 2011. Nat Struct Mol Biol 18:529-36). According to the northern blot analysis crRNA of similar length is generated in the S. thermophilus LMD-9 CRISPR3/Cas system (Makarova et al., 2011. Nat Rev Microbiol 9:467-77), which is almost identical to the CRISPR3/Cas system of DGCC7710 strain (
FIGS. 4A and B). We assumed that crRNA isolated from the Cas9-crRNA complex expressed in the heterologous E. coli strain (FIG. 1 ) may have the same length (FIG. 4 ). Therefore, to probe nucleic acids extracted from the Strep-Tactin purified Cas9 complex we used 42 nt anti-crRNA DNA oligonucleotide comprised of 22 nt region corresponding to the 3′-end of the repeat sequence and 20 nt at the 5′-end of SP1 fragment. Nucleic acid present in the Cas9 complex hybridized with anti-crRNA oligonucleotide, and was sensitive to RNAse but not DNAse treatment (FIG. 1C ). The size of extracted crRNA was identical to the 42 nt synthetic oligoribonucleotide corresponding to the putative crRNA of the CRISPR3 system of S. thermophilus DGCC7710 strain (FIG. 3A ,FIG. 4C ). Taken together, these data confirm that Cas9 Strep-tag protein co-purifies with 42 nt crRNA, which is derived from CRISPR3 region. - Cas9 protein cleaves double-stranded DNA within a proto-spacer. To test in vitro activity of purified Cas9-crRNA complex we first used the SP1 oligoduplex (Table 1) containing the proto-spacer sequence identical to spacer SP1 in the CRISPR3 array, the
PAM sequence 5′-TGGTG-3′ downstream of the proto-spacer, and 10 nt flanking sequences from pSP1 plasmid (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) (FIG. 5A ). The oligoduplex strand complementary to crRNA is named (+)strand, while the opposite duplex strand is called the ( )strand. To monitor cleavage reaction either (+) or (−)strand of the SP1 oligoduplex was P33-labeled at the 5′-terminus. Data shown inFIG. 5B demonstrate that the Cas9-crRNA complex cleaves both strands of oligoduplex at fixed position. Mapping of the cleavage position using synthetic oligonucleotides as size markers revealed that the Cas9-crRNA complex cuts both strands of the SP1 oligoduplex within the proto-spacer 3 nt upstream of the PAM (FIG. 5B ) leaving blunt ends. It is worth to note, that no cleavage is observed after the 2 h incubation of the SP1 oligoduplex with the Cas9 protein lacking crRNA (FIG. 6C ). - To test whether the Cas9-crRNA complex can locate the proto-spacer and cut DNA in vitro in long DNA substrates mimicking in vivo invading foreign DNA we analyzed cleavage of pSP1 plasmid (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) (
FIG. 5C ) carrying proto-spacer1 and PAM. In the presence of Cas9-crRNA complex supercoiled form of pSP1 plasmid was converted into a linear form (FIG. 5D ), while pUC18 plasmid lacking proto-spacer1 was not cleaved. This means that both strands of the pSC1 plasmid were cleaved specifically within the proto-spacer region. We used direct sequencing to determine the ends of linear DNA form formed after the Cas9-crRNA cleavage. Sequencing results confirmed that cleavage of plasmid DNA occurred 3 nt away from 5′-NGGNG-3′ PAM sequence similarly to the SP1 oligoduplex cleavage (FIG. 5D ). The cleavage positions identified in the in vitro experiments (FIG. 4 ) for the CRISPR3/Cas system of S. thermophilus are identical to those determined in the in vivo cleavage experiments for the CRISPR1/Cas system in S. thermophilus (Garneau et al., 2010. Nature 468:67-71). To check if Cas9-crRNA induced cleavage occurs at the same position in other proto-spacer sequences, we analysed cleavage of the SP2 oligoduplex carrying a protospacer-2 and PAM sequences by the heterogeneous Cas9-crRNA complex isolated from the host carrying 12 spacer-repeat units. We have found that this heterogeneous Cas9-crRNA complex cuts (+)strand of SP2 oligoduplex exactly at the same position as in the SP1 oligoduplex. - Cas9-crRNA cleavage specificity is directed by the crRNA sequence. To demonstrate directly that Cas9-crRNA complex specificity can be re-programmed by changing crRNA in the ribonucleoprotein complex we inserted a new spacer (SN) instead of spacer S1 in the CRISPR region generating pCas(−)SN plasmid containing only a minimal CRISPR region and tracrRNA encoding sequence (
FIG. 7 ), co-expressed this plasmid together with pASKIBA-Cas9 and purified Cas9-crRNA complex. The cleavage specificity of Cas9-crRNA complex was analysed using plasmids pSP1+SPN and pSP1. pSP1+SPN plasmid containing the proto-spacer sequence matching the SN spacer in the CRISPR region, was linearized by the Cas9-crRNA complex, while pSP1 plasmid which lacks complimentary sequence remained intact (FIG. 7B ). To determine the cleavage position within the SPN spacer sequence, we performed experiments with SPN oligoduplex, containing proto-spacer complementary to spacer SN and PAM (FIG. 7D ). Oligoduplex cleavage assay confirmed (FIG. 7C and D) that Cas9-crRNA complex with re-engineered specificity cleaves both DNA strands within the SN proto-spacer 3 nt upstream of the PAM identically to other Cas9-crRNA complexes. - The length of the spacer in the CRISPR3 region of S. thermophilus is 30 nt. According to the data provided in the
FIG. 1C , the mature crRNA copurified with the Cas9 protein is comprised of 42 nt. It means that only 20 nt of crRNA is complementary to the (+)strand of proto-spacer. To assess whether 5′-end of proto-spacer is important for the plasmid interference by the CRISPR3 system of S. thermophilus we engineered plasmids pSP1-27, pSP1-23, pSP1-19, pSP1-15, pSP1-11 with the 5′-truncated proto-spacer1 (the length of proto-spacer 27 bp, 23 bp, 19 bp, 15 bp, 11 bp, respectively), and analyzed transformation efficiency of the recipient strain containing pCRISPR3 (FIG. 8B ). Plasmids containing 4 or 7 by truncations at the 5′ end of proto-spacer1, had no effect on the recipient strain ability to interfere with plasmid transformation. Shorter versions of proto-spacer (11, 15, 19 bp) abolished recipient strain ability to prevent plasmid transformation. These data shows that 5′ end of the proto-spacer, which has no complementarity to mature crRNA is not important for CRISPR3/Cas function. In full support to the in vivo experiments, the SP1-20 oligoduplex containing only 20 nt of the protospacer-1 is efficiently cleaved by Cas9-crRNA (FIGS. 8D and E). - PAM is required for DNA binding and cleavage by Cas9-crRNA. Plasmids carrying a proto-spacer but not PAM (pSP1-pΔ) or multiple PAM's but no proto-spacer (pUC18) are resistant for Cas9-crRNA cleavage (
FIG. 8A ). Hence, in accordance with in vivo data both PAM and proto-spacer are required for double-stranded DNA cleavage by Cas9-crRNA complex (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82). To find out, whether PAM is recognized in a context of a double-stranded or a single-stranded DNA, we analyzed Cas9-crRNA binding and cleavage of oligodeoxynucleotides i) SP1 (containing both proto-spacer and PAM), ii) SP1-Δp (contains only proto-spacer), and iii) SP2 (contains only PAM). The (+)strands of these oligodeoxynucleotides were used as single-stranded DNA substrates (s(+)SP1, s(+)SP1-Δp, s(+)SP2, accordingly) (Table 1). - Consistent with the plasmid cleavage experiments, oligoduplexes which have only proto-spacer, but not PAM are not cut by Cas9-crRNA (
FIG. 9B ). On the other hand, (+)strand in the single-stranded form is cut at the similar rate independently whether it has or has not PAM (FIG. 9B ). These data clearly show that PAM is required only for a double-stranded but not for a single-stranded DNA cleavage. - To test if PAM is important for DNA binding by the Cas9-crRNA complex, electrophoretic mobility shift experiments were performed. To avoid cleavage, binding experiments were performed in the absence of Mg2+ ions which are necessary for cleavage. Cas9-crRNA showed different binding patterns for double-stranded and single-stranded oligonucleotides. In the case of the SP1 oligoduplex a low mobility complex is observed already at 1 nM concentration (
FIG. 9C ). On the other hand, no binding is observed under the same experimental conditions for oligoduplexes without PAM (SP1-Δp) or without proto-spacer (SP2). Moreover, no low mobility complex is observed in the case of Cas9 protein without crRNA (FIG. 6A ), confirming that crRNA is important for complex formation. Thus, taken together binding experiments clearly show that the Cas9 protein complex is unable to bind double-stranded DNA in the absence of PAM, even if it contains crRNA complementary to proto-spacer. To put it into other words, double-stranded DNA substrates lacking PAM are not cleaved because PAM is required for Cas9-crRNA binding. - On the other hand, single-stranded oligonucleotides ((+)strand) are bound by Cas9-crRNA with the same affinity independently of the PAM presence (
FIG. 9D ). Again, no binding was observed for single-stranded DNA oligonucleotide without proto-spacer (FIG. 9D ), or for Cas9 protein lacking crRNA (FIG. 6C ). Taken together these data indicate that Cas9-crRNA complex discriminates PAM only in the double-stranded but not a single-stranded DNA. - Since some Type III CRISPR systems provide RNA rather than DNA interference, we have studied RNA binding and cleavage by the Cas9-crRNA complex. The Cas9-crRNA did not cleave specifically either single-stranded RNA, or double-stranded RNA bearing a proto-spacer and PAM (
FIG. 10B).This finding confirms confirms once more that DNA is a primary target for the CRISPR3/Cas system of S. thermophilus. Cas9-crRNA complex binds a complementary RNA containing a proto-spacer, but this interaction is probably functionally not important, because single stranded RNA is not cleaved specifically by Cas9 within a proto-spacer. - Mutagenesis of Cas9 protein RuvC and HNH motifs. Plasmid transformation experiments indicate that RuvC and HNH motifs (
FIG. 11A ) are important for Cas9 function (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82). To test if these motifs are involved in the target DNA cleavage, we expressed and purified D31A and N891A mutants following procedure described for wt Cas9. Both mutants co-purified with crRNA identical to crRNA in the wt Cas9 complex (FIG. 11C ). To test whether mutant proteins retained cleavage activity, we monitored pSP1 plasmid cleavage by mutant Cas9-crRNA complexes. Surprisingly, instead of linear reaction product observed for the wt Cas9 protein, both mutants produced nicked DNA form (FIG. 11B ) indicating that both active sites mutants cleave only one DNA strand of plasmid substrate within a proto-spacer. - To determine whether mutant proteins exhibit a strand preference, we analysed D31A and N891A mutant cleavage of the SP1 oligoduplex. RuvC active site mutant (D31A) cut (+)strand of oligoduplex at the same position as wt Cas9-crRNA protein, while the (−)strand stayed intact (
FIG. 11C ). And vice versa, HNH active site mutant (N891A) cleaved only (−)strand, but not (+)strand of the SP1 oligoduplex (FIG. 11D ). Taken together these data indicate that RuvC and HNH active sites act on opposite DNA strands to generate a double strand break. To test, whether the same cleavage pattern is conserved during the plasmid DNA cleavage, we sequenced proto-spacer regions of nicked plasmids. Run-off sequence data confirmed that RuvC active site mutant cut only (+) DNA strand while HNH/McrA mutant—only (−)strand (FIGS. 12A and B). Furthermore, we found that RuvC mutant cleaved (+)strand of a single-stranded DNA but no such cleavage was detected for the HNH mutant (FIG. 12D ). - To test whether mutations altered DNA-binding affinity of mutant protein-crRNA complexes, DNA binding was studied using the electrophoretic mobility shift assay. Both mutant protein-crRNA complexes bound oligoduplex SP1 with the same affinity as wild type protein (
FIG. 12C .). Thus, mutations in the putative active sites of Cas9 have no significant effect on double-stranded DNA-binding properties of the Cas9-crRNA complex. Since 42 nt crRNA was present in the mutant protein complexes (FIG. 12C ), we conclude that mutant Cas9-crRNA complexes lost ability to cut one of the target DNA strand due to active site mutation. Since Cas9-HisTag protein is a monomer in solution(FIG. 13 ), it is likely that Cas9 protein is functional as a monomer and uses two active sites for the cleavage of opposite DNA strands. Similar strategy is exploited by some restriction endonucleases (Armalyte et al., 2005. J Biol Chem 280: 41584-94). - Cas9-crRNA complex of CRISPR3/Cas system of S. thermophilus is crRNA-guided endonuclease. This work demonstrates that Cas9-crRNA complex of CRISPR3/Cas system of S. thermophilus is crRNA-directed endonuclease which cuts both DNA strands in the presence of Mg2+-ions within a
protospacer 3 nt downstream of the PAM sequence to produce blunt end cleavage products. Sequence specificity of the Cas9-crRNA complex is dictated by the 42 nt crRNA which include ˜20 nt fragment complementary to the proto-spacer sequence in the target DNA. In this respect the mature crRNA in the Cas9 complex of CRISPR3/Cas system of S. thermophilus is similar to crRNA of Streptoccocus pyogenes which has a 3′-handle of repeat sequence but lacks part of the spacer sequence and 5′-handle corresponding to the repeat fragment (Deltcheva et al, 2011). Therefore, crRNA present in the Cas9-crRNA complex of CRISPR3/Cas system of S. thermophilus is complementary only to the part of the proto-spacer sequence distal to PAM. Not surprisingly, truncation of the 3′-end of the proto-spacer sequence by 10 nucleotides has no effect on Cas9-crRNA cleavage of synthetic oligoduplexes or plasmid DNA (FIG. 8 ). - The cleavage machinery of Cas9-crRNA complex resides in the Cas9 protein which provides two active sites for the phosphodiester bond cleavage. The RuvC- and HNH-like active sites of Cas9 protein are located on different domains and act independently on individual DNA strands. Alanine replacement of the active site residues in the RuvC- and HNH-motifs transforms Cas9-crRNA complex into a strand-specific nicking endonucleases similar to the nicking enzymes (Chan et al., 2011. Nucleic Acids Res 39:1-18). Consistent with in vivo studies, a functional activity of the Cas9-crRNA complex in vitro is absolutely dependent on the presence of the proto-spacer adjacent motif NGGNG upstream of the proto-spacer sequence. Data presented in the
FIG. 3 show that PAM is required for Cas9-crRNA binding to the double-stranded DNA. If PAM sequence is missing in double-stranded DNA, the Cas9-crRNA complex does not bind such DNA even if it contains a complementary proto-spacer sequence. On the other hand, Cas9-crRNA does not display DNA binding if PAM (or multiple PAM's) is present but proto-spacer sequence is absent. Thus, in consistence with the in vivo data, both PAM and proto-spacer sequences are necessary prerequisite for double-stranded DNA binding and subsequent cleavage. Contrary to the Cas9-crRNA binding to the double-stranded DNA, PAM sequence motif has no effect on the single-stranded DNA binding by: a single-stranded oligodeoxynucleotide containing proto-spacer with or without PAM sequence is bound equally well but with lower affinity than double-stranded DNA. In the presence of Mg2+ ions Cas9 cuts single-stranded DNA bound to the crRNA using its HNH-active site. - Mechanism of DNA interference in the Type II systems. Our results establish a simple model for the mechanism of double-stranded DNA cleavage by Cas9-crRNA complex in the S. thermophilus CRISPR3/Cas system (
FIG. 14 ). Cas9-crRNA complexes using a mechanism that yet has to be defined locates and binds to a proto-spacer sequence within the double-stranded DNA in a PAM-dependent process. It is possible that PAM in the double-stranded DNA serves as an initiation site (signal) for the strand separation and promotes subsequent pairing of crRNA to the complementary (+)strand of DNA. It remains to be established whether a Cas9 protein module or Cas9-bound crRNA (for example, using nucleotides in the conserved the “3′-handle” of the conserved repeat sequence) recognizes the PAM sequence. Despite of the lack of these mechanistic details, our data clearly demonstrate that PAM is recognized by Cas9-crRNA in the context of double-stranded DNA. The Cas9-crRNA binding to the target sequence in the ds DNA presumably results in the R-loop structure where (−)strand is displaced and the complementary (+) DNA strand is paired to the crRNA. In the presence of Mg2+ ions phosphodiester bond cleavage occurs on bothstrands 3 nt 5′-upstream of the PAM sequence to generate blunt DNA ends. DNA cleavage analysis by the RuvC- or HNH-motif mutants demonstrate that RuvC- and HNH-like active sites of Cas9 protein act on the (−) and (+)strands, respectively. Therefore, in the catalytically competent the Cas9-crRNA complex, the N-terminal domain containing the catalytic D31A residue of the RuvC motif is positioned at the displaced (−) DNA strand, while the central part of Cas9 containing the HNH motif is located in the vicinity of the scissile phosphodiester bond of (+) DNA strand paired to crRNA. After DNA cleavage Cas9-crRNA remains bound to the reaction products (FIG. 15 ). Taken together data presented here suggest a first molecular mechanism for the DNA interference step by the CRISPR3/Cas system of S. thermophilus. Since cas9 is a signature gene (Makarova et al., 2011. Nat Rev Microbiol 9:467-77) for Type IIA and Type IIB systems the cleavage mechanism proposed here is likely to be conserved in other Type IIA and Type IIB systems. Stand-alone versions of Cas9-like proteins which are not a part of the CRISPR system were identified by bioinformatics (Makarova et al., 2011. Biol Direct 6: 38). In the light of the data provided here we suggest that these proteins can provide interference against foreign DNA similarly to Cas9 if loaded with small crRNA molecules which may be generated through the pathway different from CRISPR. - Comparison to other RNA interference complexes. The mechanism proposed here for the double-stranded DNA cleavage by the Cas9-crRNA complex differs significantly from that for the Type I-E (former Ecoli or CASS2) system (Jore et al., 2011. Nat Struct Mol Biol 18:529-36). In the E. coli system crRNA and Cas proteins assemble into a large ribonucleoprotein complex named Cascade that facilitates target recognition by enhancing sequence-specific hybridization between the CRISPR RNA and complementary target sequences (Jore et al., 2011. Nat Struct Mol Biol 18:529-36). Target recognition is dependent on PAM and governed by the “seed” crRNA sequence located at the 5′-end of the spacer region (Semenova et al., 2011. Proc Natl Acad Sci USA 108:10098-103). However, while Cascade-crRNA complex alone is able to bind double-stranded DNA containing PAM and proto-spacer, it requires an accessory Cas3 protein for DNA cleavage. Cas3 is a single-stranded DNA nuclease and helicase which is able to cleave single-stranded DNA producing multiple cuts (Sinkunas et al.,2011. EMBO J 30:1335-42). The mechanistic details of the Cas3 action on a proper biological substrate (e.g., Cascade-crRNA bound to the double-stranded DNA in the R-loop like complex) have yet to be established. However, it has been demonstrated recently that Cas3 of M. jannaschii alone is able to cut both DNA strands in the synthetic substrate mimicking R-loop (Beloglazova et al., 2011. EMBO J 30:616-27). It is proposed that Cas3 may follow similar mechanism for DNA cleavage in the presence of Cascade-crRNA complex. Thus, current data clearly show that mechanistic details of the interference step for the Type I-E system differs from that of CRISPR3 system both by the catalytic machinery and mechanism and complexity.
- In the III-B subtype CRISPR systems present in many archea and some bacteria, Cas module RAMP (Cmr) proteins and cRNA assemble into the effector complex that targets invading RNA (Hale et al., 2009. Cell 139:945-56; Hale et al., 2012. Mol Cell 45:292-302). In Pyroccus furiosus RNA silencing complex comprised of six Cmr1-6 proteins and crRNA binds to the target RNA and cuts it at fixed distance in respect to 3′-end the psiRNA. The cleavage activity depends on Mg2+-ions however individual Cmr protein(-s) responsible for target RNA cleavage has yet to be identified. The effector complex of Sulfolobus solfataricus comprised of seven Cmr1-7 proteins and crRNA cuts invading RNA in an endonucleolytic reaction at UA dinucleotides (Zhang et al., 2012. Mol Cell 45: 303-13). Importantly, both Cmr-crRNA complexes perform RNA cleavage in a PAM independent manner.
- The data provided here show that Cas9-crRNA complex of CRISPR3 system is so far the most simple DNA interference system comprised of a single Cas9 protein bound to the crRNA molecule. The simple modular organization of the Cas9-crRNA complex where specificity for DNA target is encoded by the crRNA and cleavage machinery is brought by the Cas protein provides a versatile platform for engineering of universal RNA-guided DNA endonucleases.
- In Vitro assembly of Cas9-crRNA Complex from 4 Components
- In this example we demonstrate that the catalytically active Cas9-crRNA complex can be assembled in vitro by mixing 4 individual components: the C-terminal 6× His-tagged variant of Cas9 protein (“6× His” disclosed as SEQ ID NO: 23), tracrRNA transcript (SEQ ID NO: 5), CRISPR RNA transcript (SEQ ID NO: 8) and E. coli RNAseIII (Abgene). Cas9 protein is first pre-incubated with tracrRNA and CRISPR RNA transcripts, followed by the subsequent incubation with RNAseIII to generate a catalytically competent Cas9-crRNA complex which is used for the site-specific DNA cleavage.
- More specifically, RNA fragments required for complex assembly were produced by in vitro transcription (TranscriptAid™ T7 High Yield Transcription Kit, Fermentas) of PCR-generated fragment containing a T7 promoter at the proximal end of RNA coding sequence. PCR-generated DNA fragments encoding CRISPR RNA and tracrRNA were produced using pCas9(−)SP1 plasmid as a template with a following primer pair: 5′-taatacgactcactataGggtagaaaagatatcctacgagg-3′ (SEQ ID NO: 40)/5′-CAACAACCAAGCTAATACAGCAG-3′ (SEQ ID NO: 41) and 5′-aaaaacaccgaatcggtgccac-3′ (SEQ ID NO: 42)/5′-taatacgactcactataGggTAATAATAATTGTGGTTTGAAACCATTC-3′ (SEQ ID NO: 43) (T7 RNA polymerase promoter underlined, transcription start shown in bold). The 150 nt CRISPR RNA transcript is comprised of 102 nt Repeat-Spacerl-Repeat sequences flanked by the 23 nt upstream and 25 nt downstream regions required for primer annealing. The 105 nt transcript of tracrRNA is comprised of a 38 nt stretch partially complimentary to the S. thermophilus DCGG7710 CRISPR3 repeat sequence fragment (anti-repeat sequence), flanked by the 16 nt upstream and 51 nt downstream region. RNA fragments produced by in vitro transcription were purified using RNeasy MinElute Cleanup Kit (Qiagen).
- For in vitro assembly of catalytically competent Cas9-crRNA complex, the 6× His-tagged Cas9 protein (“6× His” disclosed as SEQ ID NO: 23) was mixed with CRISPR RNA and tracrRNA transcripts at 1:0.5:1 molar ratio and pre-incubated in a buffer containing 10 mM Tris-HCl (pH 7.5 at 37° C.), 100 mM NaCl at 37° C. for 30 min followed by addition of RNAseIII (Ambion), MgCl2 and DTT and subsequent incubation for additional 30 min. The final concentrations of the components in the assembly mix were the following: 100 nM of 6× His-tagged Cas9 protein (“6× His” disclosed as SEQ ID NO: 23), 50 nM of CRISPR RNA, 100 nM of tracrRNA, 50 nM RNAseIII, 10 mM MgCl2 and 1 mM DTT.
- Below we provide experimental evidences that in vitro assembled Cas9-crRNA complex guided by the crRNA sequence cleaves DNA at the specific site to generate blunt ends. In this respect Cas9-crRNA complex can be used an alternative for a restriction endonuclease or meganuclease for the site-specific DNA cleavage in vitro. The sequence specificity of the complex is dictated by the crRNA sequence which can be engineered to address a desirable DNA target.
- First, the DNA cleavage activity of the in vitro assembled Cas9-crRNA complex was assayed on the plasmid substrates pSP1 and pUC18. The pSP1 plasmid contained a proto-spacer1 sequence flanked by the 5′-NGGNG-3′ PAM sequence. Proto-spacer1 sequence was not present in pUC18. Reactions on pUC18 and pSP1 plasmids (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) were conducted at 37° C. in the 10 mM Tris HCl (pH 7.5 at 37° C.), 50 mM NaCl, 0.05 mg/ml BSA, 0.5 mM DTT and 10 mM MgCl2. Reaction mixtures typically contained 3.0 nM of supercoiled plasmid DNA. The reactions were initiated by mixing 50 μl volumes of Cas9-crRNA complex and plasmid DNA (1:1 v/v ratio) in a reaction buffer. Aliquots were removed at timed intervals and quenched with phenol/chloroform. The aqueous phase was mixed with loading dye solution (0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol) and reaction products analyzed by electrophoresis through agarose (
FIG. 16 ). To check whether the pSP1 plasmid pre-cleaved by Cas9-crRNA complex can be re-ligated, we purified linear pSP1 cleavage product from agarose gel using GeneJET gel extraction Kit (Fermentas) and re-ligated using T4 DNA ligase (Fermentas). After transformation of E. coli cells by the ligation mix, five individual clones were selected from resulting transformants, plasmid DNA was purified and subjected to sequencing using the following primers: 5′-ccgcatcaggcgccattcgcc-3′ (SEQ ID NO: 29) (sequencing of (+)strand) and 5′-gcgaggaagcggaagagcgccc-3′ (SEQ ID NO: 30) (sequencing of (−)strand). Sequence analysis revealed that the DNA sequence of the pSP1 plasmid in the locus that was cleaved by Cas9-crRNA complex and re-ligated was identical to the sequence of the non-treated plasmid. E. coli transformation by the ligation mix in the absence of T4 DNA ligase did not produce transformants indicating that no traces of supercoiled plasmid are co-purified with the linear reaction product. - Next, the cleavage activity of the in vitro assembled Cas9-crRNA complex was assayed on a synthetic 55 by oligodeoxynucleotide duplex SP1 containing a proto-spacer sequence matching to the spacer sequence of crRNA (
FIG. 17 ). Reactions conditions were identical to those described above for the plasmid DNA cleavage, except that 1 nM of oligoduplex was used. Reaction product analysis revealed that in vitro assembled Cas9-crRNA complex cleaved both strands of the oligoduplex at fixed position, inside the proto-spacer, after the 37th nucleotide from the 5′-terminus, 3 nt upstream of thePAM sequence 5′-NGGNG-3′ leaving blunt ends (FIG. 17 ). - In Vitro Assembly of Cas9-crRNA Complex from 3 Components
- In this example we demonstrate that active Cas9-crRNA complex can be assembled in vitro by mixing 3 individual components: the C-terminal 6× His-tagged variant of Cas9 protein (“6× His” disclosed as SEQ ID NO: 23), tracrRNA transcript provided in Example 1 (SEQ ID NO: 5 and SEQ ID NO: 6), and CRISPR RNA transcript (SEQ ID NO: 8) provided in Example 1 or synthetic crRNA (SEQ ID NO: 7) which corresponds to the putative crRNA of CRISPR3/Cas system of S. thermophilus DGCC7710 strain.
Synthetic 42 nt oligoribonucleotide is comprised of 20 nt of identical to the spacer1 of CRISPR3 region at the 5′ terminus and 22 nt of repeat sequence at the 3′ end. More specifically, tracrRNA and CRISPR RNA transcripts were obtained as described in Example 1. To generate the Cas9-crRNA complex the 6× His-tagged Cas9 protein (“6× His” disclosed as SEQ ID NO: 23) was mixed with tracrRNA and CRISPR RNA transcript, or 42 nt synthetic crRNA, at 1:0.5:1 molar ratio and incubated in a buffer containing 10 mM Tris-HCl (pH 7.5 at 37° C.), 100 mM NaCl at 37° C. for 1 h. The final concentrations of the components in the assembly mix were the following: 100 nM of 6× His-tagged Cas9 protein (“6× His” disclosed as SEQ ID NO: 23), 50 nM of CRISPR RNA or 42 nt synthetic crRNA, 100 nM of tracrRNA. - Below we provide experimental evidences that in vitro assembled Cas9-crRNA complex guided by the crRNA sequence cleaves DNA at the specific site to generate blunt ends. In this respect Cas9-crRNA complex can be used an alternative for a restriction endonuclease or meganuclease for the site-specific DNA cleavage in vitro. The sequence specificity of the complex is dictated by the crRNA sequence which can be engineered to address a desirable DNA target.
- First, the DNA cleavage activity of the in vitro assembled Cas9-crRNA complex was assayed on the plasmid substrates pSP1 and pUC18. The pSP1 plasmid contained a proto-spacer1 sequence flanked by the 5′-NGGNG-3′ PAM sequence. Proto-spacer1 sequence was not present in pUC18. Reactions on plasmid substrates (Sapranauskas et al., 2011. Nucleic Acids Res 39:9275-82) were conducted at 37° C. in the 10 mM Tris-HCl (pH 7.5 at 37° C.), 50 mM NaCl, 0.05 mg/ml BSA, 0.5 mM of DTT and 10 mM MgCl2. Reaction mixtures typically contained 3.0 nM of supercoiled plasmid DNA. The reactions were initiated by mixing 50 μl volumes of Cas9-crRNA complex and plasmid DNA (1:1 v/v ratio) in a reaction buffer. Aliquots were removed at timed intervals and quenched with phenol/chloroform. The aqueous phase was mixed with loading dye solution (0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol) and reaction products analyzed by electrophoresis through agarose (
FIG. 18 ). - Next, the cleavage activity of the in vitro assembled Cas9-crRNA complex was assayed on a synthetic 55 by oligodeoxynucleotide duplex SP1 containing a a proto-spacer sequence matching to the spacer sequence of crRNA (
FIG. 19 ). Reactions conditions were identical to those described above for the plasmid DNA cleavage, except that 1 nM of oligoduplex was used. Reaction product analysis revealed that in vitro assembled Cas9-crRNA complex cleaved both strands of the oligoduplex at fixed position, inside the proto-spacer, after the 37th nucleotide form the 5′-end, 3 nt upstream of thePAM sequence 5′-NGGNG-3′ leaving blunt ends (FIG. 19 ). - Interchangeable Spacer Cassette for the Re-Programing of the Cas9-crRNA Complex Specificity.
- In this example we describe an interchangeable spacer cassette which allows to produce crRNA carrying a nucleotide sequence against any desirable DNA target to be used for assembly of the Cas9-crRNA complex described in Examples 1 and 2 (
FIG. 20B ). The cassette caries a single repeat-spacer-repeat unit which allows insertion of the oligoduplex carrying the new spacer sequence required to generate a desired crRNA. To engineer a cassette, first we constructed a cassette containing a leader sequence, a repeat sequence and a unique Sapl recognition site in the vicinity of the repeat sequence followed by BamHI site (FIG. 20C ). To generate CRISPR region containing the unique desired spacer, we inserted a synthetic oligoduplex containing a unique spacer sequence and a repeat unit into the plasmid precleaved with Sapl and BamHI restriction enzymes. Using this cassette we produced crRNA transcripts which contained nucleotide sequences complementary to the proto-spacers N1 and N2 present in pUC18 plasmid (see below). - As proof of the principle demonstration, we used an interchangeable spacer cassette to generate crRNA1 and crRNA2 which were engineered to target pUC18 plasmid at proto-spacer1 and proto-spacer2, respectively, incorporated crRNA1 and crRNA2 into Cas9 complex as described in the Example 1 and used these complexes for the cleavage of pUC18 plasmid. The proto-spacer N1 is located near the Sapl restriction endonuclease site, while the proto-spacer N2 is in the vicinity of AatII site. The distance between Sapl and AatII restriction sites is 775 bp, while the distance between the putative Cas9-crRNA complex cleavage sites located in the spacers N1 and N2 is 612 by (
FIG. 21A ). The crRNA1 and crRNA2 PCR fragments containing T7 promoter at the proximal end were obtained from the corresponding interchangeable spacer cassette plasmids and used to produce by in vitro transcription CRISPR RNA transcripts carrying sequences matching spacer N1 or spacer N2 sequences. The catalytically active complexes of Cas9 with crRNA1 and crRNA2 were assembled for DNA cleavage as described in Example 1. In vitro assembled complexes containing either crRNA1 or crRNA2 linearized pUC18 plasmid (FIG. 21B ). When both complexes were incubated with the pUC18plasmid, two DNA fragments (2074 and 612 bp) were obtained (FIG. 21B ), indicating that plasmid cleavage occurred at sites targeted by the crRNA molecules present in the complexes. - Cloning Procedure Using Cas9-crRNA Complex.
- In this example we demonstrate that Cas9-crRNA complex may be used to prepare a vector for cloning procedure. First we demonstrated that cleavage products obtained by the Cas9-crRNA complex can be re-ligated by DNA ligase. We purified linear pSP1 cleavage product from agarose gel and re-ligated it using DNA ligase. After transformation of E. coli cells by the ligation mix, five individual clones were selected from resulting transformants, plasmid DNA was purified and subjected to sequencing. Sequence analysis revealed that the DNA sequence of the pSP1 plasmid in the locus that was cleaved by Cas9-RNA complex and re-ligated was identical to the sequence of the non-treated plasmid. E. coli transformation by the ligation mix in the absence of T4 DNA ligase did not produce transformants indicating that no traces of supercoiled plasmid are co-purified with the linear reaction product. This result illustrates, that the DNA ends generated by the Cas9 cleavage are substrates for T4 DNA ligase, and therefore must contain a phosphate at the 5′ terminus and a free OH group at the 3′ terminus (Lehman 1974. Science 186:790-7).
- Next we analyzed cleavage of pUC18 plasmid with Cas9 complex loaded with crRNA1 and crRNA2 described in Example 5 (
FIG. 21A ). First, pUC18 was cleaved with one complex, purified and re-ligated. Sequencing of 10 clones in each case confirmed, that sequence of cleaved and re-ligated plasmid was identical to the sequence of the non-treated plasmid (FIG. 21C ). This experiment suggests that additional mutations are not introduced after cleavage by Cas9-crRNA complex and ligation, and the Cas9-crRNA complex can be used for cloning experiments. When both complexes were incubated with the pUC18 plasmid, two DNA fragments (2074 and 612 bp) were obtained (FIG. 21B ), indicating that plasmid cleavage occurred at sites targeted by the crRNA molecules present in the complexes. To demonstrate that the pUC18 plasmid cleaved with Cas9-RNA complexes is suitable for a genetic engineering we cloned PCR fragment containing a promoter and a tetracycline resistance gene from the pACYC184 plasmid to the pUC18 vector pre-cleaved with the Cas9 complex mix containing both crRNA1 or crRNA2. The clones were selected on the media enriched by tetracycline and ampicillin. Sequencing of 4 selected clones confirmed that the intact PCR fragment was inserted into a desired position ((FIG. 21C ). - More specifically, the 2 μg pUC18 was incubated with the mix of separately assembled Cas9-RNA complexes (250 nM each) containing different crRNAs for 1 hour at 37° C. in 100 μl reaction volume (10 mM Tris-HCl (pH 7.5 at 37° C.), 100 mM NaCl, 1 mM DTT and 10 mM MgCl2). Obtained vector fragment was purified from agarose gel using GeneJET gel extraction Kit (Thermo Fisher scientific) and divided in to two equal parts. One part of pre-cleaved vector was dephosphorylated with the FastAP alkaline phosphatase while another part was untreated. 1282 by insert containing a promoter and a tetracycline resistance gene was obtained from the pACYC184 plasmid by PCR. After purification using the GeneJET PCR Purification Kit (Thermo Fisher scientific), a solution containing the PCR fragment was divided in to two parts. One part was phosphorylated with T4 polynucleotide kinase (Thermo Fisher scientific) while another part remained untreated. Untreated vector was ligated with the untreated PCR fragment, while a dephosphorylated vector was ligated with a phosphorylated fragment using the T4 DNA ligase (Thermo Fisher scientific). Clones were selected on a media supplemented with 100 μg/ml of Ap and 25 μg/ml Tc.
- Cleavage of Long DNA Substrates by Cas9 crRNA Complex.
- In this example we demonstrate that Cas9-crRNA may be addressed to cleave targets in long DNA molecules, including phage A, E. coli and human genomic DNAs.
- More specifically, we addressed Cas9-RNA complex to cleave specific sites in λ bacteriophage (48 kb), E. coli BL-21 strain (4.6 Mb) and human (3.2 Gb) genomic DNAs. Cas9-crRNA complex was assembled as described in Examples 2 and 3. We used 42 nt long synthetic crRNAs, 150 nt pre-crRNAs and tracrRNAs synthesized using in vitro transcription from templates generated as described in Example 4.
- λ DNA cleavage reactions were initiated by mixing λ DNA (Thermo Fisher Scientific) with assembled Cas9-RNA complex (1:1 v/v ratio) and incubating at 37° C. Final reaction mixture contained 2 μg λ DNA, 50 nM Cas9-RNA complex, 10 mM Tris-HCl (pH 7.5 at 37° C.), 100 mM NaCl, 1 mM DTT and 10 mM MgCl2 in 100 μl reaction volume. Aliquots were removed at timed intervals and quenched with phenol/chloroform. The aqueous phase was mixed with 3× loading dye solution (0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol) and reaction products analyzed by electrophoresis through agarose gels and ethidium bromide staining. The analysis of linear λ phage genomic DNA cleavage products in agarose gel confirmed that ˜40 by length DNA is efficiently cleaved at a single site (
FIG. 22A ). - DNA from E. coli BL21 (DE3) strain was isolated using the Genomic DNA purification kit (Thermo Fisher Scientific). For cleavage assay, E. coli genomic DNA was combined with assembled Cas9-RNA complex (1:1 v/v ratio) and incubated for 3 hours at 37° C. Final reaction mixture contained 30 μg genomic DNA, 1 μM Cas9-RNA complex, 10 mM Tris-HCl (pH 7.5 at 37° C.), 100 mM NaCl, 1 mM DTT and 10 mM MgCl2 in 300 μl reaction volume. Following incubation, 30 μl of FastDigest Pstl (Thermo Fisher Scientific) was added and the reaction mix was incubated for additional 16 hours at 37° C. The reaction was terminated by heating the reaction mixture for 30 min at 55° C. with Proteinase K (0.5 mg/ml; Thermo Fisher Scientific) and SDS (0.5%, w/v) followed by 30 min incubation at room temperature with RNase A (0.25 mg/ml; Thermo Fisher Scientific). After phenol/chloroform extraction, DNA was precipitated by isopropanol and dissolved in TE buffer (10 mM Tris-HCl, pH 8.0 and 1 mM EDTA). 10 μg of DNA was mixed with 3× loading dye solution (0.01% bromphenol blue and 75 mM EDTA in 50% v/v glycerol) and electrophoresed on 1% agarose gel.
- To analyse Cas9-crRNA cleavage products of E. coli genomic DNA, we designed a probe against DNA fragment containing a Cas9-RNA complex target (a proto-spacer) (
FIG. 22B ) and performed Southern blot analysis. Southern blot analysis was performed as described in (Sambrook et al, 1989. Molecular Cloning: A Laboratory Manual) with the following modifications. Fractionated DNA was transferred from agarose gel onto SensiBlot Plus Nylon membrane (Thermo Fisher Scientific) via semi-dry transfer. DNA was denatured and fixed on the membrane by placing it on paper towel saturated with 0.4 M NaOH for 10 min, rinsed with 2×SSC and air dried. The membrane was prehybridized with 6×SSC buffer containing 0.5% SDS and 100 μg/ml denatured salmon sperm DNA (Amresco) for 1 h at 65° C. The hybridization probe was generated by PCR using the genomic E. coli BL21(DE3) DNA as a template yielding 397 by product. 5′-ends were dephosphorylated with FastAP phosphatase (Thermo Fisher Scientific) and radiolabelled by incubating with [Ξ-32P]ATP (Hartmann Analytic) and T4 PNK (Thermo Fisher Scientific). The labeled probe was purified using GeneJET PCR Purification Kit (Thermo Fisher Scientific), denatured by heating to 95° C. for 5 min, rapidly cooled on ice and added directly to the prehybridization solution. The membrane was probed for 16 hours at 65° C. and washed twice with 2×SSC, 0.5% SDS and twice with 2×SSC, 0.1% SDS at room temperature, air dried and visualized by phosphorimaging (FLA-5100; Fujifilm). - The probe was designed to target DNA fragment containing a target (a proto-spacer) for the Cas9-RNA complex (
FIG. 22B ). The distance between two Pstl targets is ˜1500 bp, while the distance between proto-spacer and left Pstl target is 466 bp. After cleavage with Cas9 complex we detected only 466 by DNA fragment (FIG. 22C ), which means that all DNA targets were cleaved by Cas9 protein in the desired position. These data clearly demonstrates that Cas9 protein effectively finds targets in very long and complex molecules such as viral and bacterial DNA. - To analyze Cas9-crRNA cleavage products of human genomic DNA we used DNA extracted from human brain. Human genomic DNA was combined with assembled Cas9-crRNA complex (1:1 v/v ratio) and incubated for 30 min at 37° C. Final reaction mixture contained 1 μg genomic DNA, 100 nM Cas9, 10 mM Tris-HCl (pH 7.5 at 37° C.), 100 mM NaCl, 1 mM DTT and 10 mM MgCl2 in 100 μl reaction volume. Cas9-crRNA-HS1 (SEQ ID NO: 13) and Cas9-crRNA-H52 (SEQ ID NO: 14) complexes were assembled to target RASGEF1C or ARL15 loci, respectively. Cleavage products were analyzed using qPCR (
FIG. 22D ). After treatment with Cas9-crRNA complex, the amount of intact DNA targets decreased more than 25 times. The analysis of the results obtained from qPCR data revealed that Cas9-RNA complexes cleave human genomic DNA efficiently in the desired loci. These data clearly demonstrates that Cas9 protein effectively finds targets in very long and complex molecules such as viral, bacterial and mammal DNA. - The application contains a Sequence Listing which has been submitted in ASCII format and is hereby incorporated by reference in its entirety. The ASCII copy, created on Mar. 13, 2013, is named 078981.4_SL.txt and is 63.6 kilobytes in size.
- The embodiments shown and described in the specification are only specific embodiments of inventors who are skilled in the art and are not limiting in any way. Therefore, various changes, modifications, or alterations to those embodiments may be made without departing from the spirit of the invention in the scope of the following claims. The references cited are expressly incorporated by reference herein in their entirety.
Claims (12)
1-78. (canceled)
79. A Cas9-crRNA complex comprising:
a. a Cas9 protein;
b. a tracrRNA transcript; and
c. a CRISPR RNA transcript that is engineered to guide the Cas9-crRNA complex to a target DNA sequence for site specific modification of the target DNA sequence,
wherein (a), (b), and (c) are assembled in vitro.
80-113. (canceled)
114. The Cas9-crRNA complex of claim 79 , wherein the crRNA comprises an approximately 20 nucleotide fragment complementary to a proto-spacer sequence in the target DNA sequence.
115. The Cas9-crRNA complex of claim 79 , wherein the target DNA sequence is a plasmid DNA.
116. The Cas9-crRNA complex of claim 79 , wherein the target DNA sequence is a human genomic DNA.
117. The Cas9-crRNA complex of claim 79 , wherein the Cas9 protein comprises a fusion polypeptide comprising at least one additional amino acid sequence.
118. The Cas9-crRNA complex of claim 117 , wherein the additional amino acid sequence is used for purification of the fusion polypeptide by affinity chromatography.
119. The Cas9-crRNA complex of claim 79 , wherein the Cas9 protein contains a point mutation in the RuvC active site motif.
120. The Cas9-crRNA complex of claim 119 , wherein the point mutation is D31A.
121. The Cas9-crRNA complex of claim 79 , wherein the Cas9 protein contains a point mutation in the HNH active site motif.
122. The Cas9-crRNA complex of claim 121 , wherein the point mutation is N891A.
Priority Applications (1)
Application Number | Priority Date | Filing Date | Title |
---|---|---|---|
US14/683,443 US20150240261A1 (en) | 2012-03-20 | 2015-04-10 | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
Applications Claiming Priority (5)
Application Number | Priority Date | Filing Date | Title |
---|---|---|---|
US201261613373P | 2012-03-20 | 2012-03-20 | |
US201261625420P | 2012-04-17 | 2012-04-17 | |
PCT/LT2013/000006 WO2013141680A1 (en) | 2012-03-20 | 2013-03-15 | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
US201414385241A | 2014-09-15 | 2014-09-15 | |
US14/683,443 US20150240261A1 (en) | 2012-03-20 | 2015-04-10 | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
Related Parent Applications (2)
Application Number | Title | Priority Date | Filing Date |
---|---|---|---|
PCT/LT2013/000006 Continuation WO2013141680A1 (en) | 2012-03-20 | 2013-03-15 | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
US14/385,241 Continuation US9637739B2 (en) | 2012-03-20 | 2013-03-15 | RNA-directed DNA cleavage by the Cas9-crRNA complex |
Publications (1)
Publication Number | Publication Date |
---|---|
US20150240261A1 true US20150240261A1 (en) | 2015-08-27 |
Family
ID=48050947
Family Applications (8)
Application Number | Title | Priority Date | Filing Date |
---|---|---|---|
US14/385,241 Active US9637739B2 (en) | 2012-03-20 | 2013-03-15 | RNA-directed DNA cleavage by the Cas9-crRNA complex |
US14/385,857 Abandoned US20150050699A1 (en) | 2012-03-20 | 2013-03-20 | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
US14/683,443 Abandoned US20150240261A1 (en) | 2012-03-20 | 2015-04-10 | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
US14/743,764 Abandoned US20150291961A1 (en) | 2012-03-20 | 2015-06-18 | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
US15/834,578 Active US11555187B2 (en) | 2012-03-20 | 2017-12-07 | RNA-directed DNA cleavage by the Cas9-crRNA complex |
US16/148,783 Active US10844378B2 (en) | 2012-03-20 | 2018-10-01 | RNA-directed DNA cleavage by the Cas9-crRNA complex |
US17/857,480 Pending US20230123754A1 (en) | 2012-03-20 | 2022-07-05 | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
US18/065,006 Pending US20230272394A1 (en) | 2012-03-20 | 2022-12-13 | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
Family Applications Before (2)
Application Number | Title | Priority Date | Filing Date |
---|---|---|---|
US14/385,241 Active US9637739B2 (en) | 2012-03-20 | 2013-03-15 | RNA-directed DNA cleavage by the Cas9-crRNA complex |
US14/385,857 Abandoned US20150050699A1 (en) | 2012-03-20 | 2013-03-20 | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
Family Applications After (5)
Application Number | Title | Priority Date | Filing Date |
---|---|---|---|
US14/743,764 Abandoned US20150291961A1 (en) | 2012-03-20 | 2015-06-18 | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
US15/834,578 Active US11555187B2 (en) | 2012-03-20 | 2017-12-07 | RNA-directed DNA cleavage by the Cas9-crRNA complex |
US16/148,783 Active US10844378B2 (en) | 2012-03-20 | 2018-10-01 | RNA-directed DNA cleavage by the Cas9-crRNA complex |
US17/857,480 Pending US20230123754A1 (en) | 2012-03-20 | 2022-07-05 | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
US18/065,006 Pending US20230272394A1 (en) | 2012-03-20 | 2022-12-13 | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
Country Status (16)
Country | Link |
---|---|
US (8) | US9637739B2 (en) |
EP (2) | EP3594341A1 (en) |
JP (3) | JP6423338B2 (en) |
CN (2) | CN104520429B (en) |
BR (1) | BR112014023353A2 (en) |
CA (2) | CA2867849C (en) |
DK (1) | DK2828386T3 (en) |
EA (1) | EA029544B1 (en) |
ES (1) | ES2749108T3 (en) |
HK (1) | HK1206392A1 (en) |
HU (1) | HUE046295T2 (en) |
IN (1) | IN2014DN07846A (en) |
MX (2) | MX370435B (en) |
PL (1) | PL2828386T3 (en) |
PT (1) | PT2828386T (en) |
WO (1) | WO2013142578A1 (en) |
Cited By (29)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
US9888673B2 (en) | 2014-12-10 | 2018-02-13 | Regents Of The University Of Minnesota | Genetically modified cells, tissues, and organs for treating disease |
US10000772B2 (en) | 2012-05-25 | 2018-06-19 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
WO2018226900A2 (en) | 2017-06-06 | 2018-12-13 | Zymergen Inc. | A htp genomic engineering platform for improving fungal strains |
WO2018226880A1 (en) | 2017-06-06 | 2018-12-13 | Zymergen Inc. | A htp genomic engineering platform for improving escherichia coli |
US10166255B2 (en) | 2015-07-31 | 2019-01-01 | Regents Of The University Of Minnesota | Intracellular genomic transplant and methods of therapy |
US10190137B2 (en) | 2013-11-07 | 2019-01-29 | Editas Medicine, Inc. | CRISPR-related methods and compositions with governing gRNAS |
US10428319B2 (en) | 2017-06-09 | 2019-10-01 | Editas Medicine, Inc. | Engineered Cas9 nucleases |
US10731181B2 (en) | 2012-12-06 | 2020-08-04 | Sigma, Aldrich Co. LLC | CRISPR-based genome modification and regulation |
US10844378B2 (en) | 2012-03-20 | 2020-11-24 | Vilnius University | RNA-directed DNA cleavage by the Cas9-crRNA complex |
US10851380B2 (en) | 2012-10-23 | 2020-12-01 | Toolgen Incorporated | Methods for cleaving a target DNA using a guide RNA specific for the target DNA and Cas protein-encoding nucleic acid or Cas protein |
US10912797B2 (en) | 2016-10-18 | 2021-02-09 | Intima Bioscience, Inc. | Tumor infiltrating lymphocytes and methods of therapy |
US11053515B2 (en) | 2019-03-08 | 2021-07-06 | Zymergen Inc. | Pooled genome editing in microbes |
US11053506B2 (en) | 2019-03-08 | 2021-07-06 | Zymergen Inc. | Iterative genome editing in microbes |
US11066663B2 (en) | 2018-10-31 | 2021-07-20 | Zymergen Inc. | Multiplexed deterministic assembly of DNA libraries |
US11078481B1 (en) | 2016-08-03 | 2021-08-03 | KSQ Therapeutics, Inc. | Methods for screening for cancer targets |
US11078483B1 (en) | 2016-09-02 | 2021-08-03 | KSQ Therapeutics, Inc. | Methods for measuring and improving CRISPR reagent function |
US11098325B2 (en) | 2017-06-30 | 2021-08-24 | Intima Bioscience, Inc. | Adeno-associated viral vectors for gene therapy |
US11236313B2 (en) | 2016-04-13 | 2022-02-01 | Editas Medicine, Inc. | Cas9 fusion molecules, gene editing systems, and methods of use thereof |
US11371030B2 (en) | 2017-05-31 | 2022-06-28 | The University Of Tokyo | Modified Cas9 protein and use thereof |
US11390884B2 (en) | 2015-05-11 | 2022-07-19 | Editas Medicine, Inc. | Optimized CRISPR/cas9 systems and methods for gene editing in stem cells |
US11414657B2 (en) | 2015-06-29 | 2022-08-16 | Ionis Pharmaceuticals, Inc. | Modified CRISPR RNA and modified single CRISPR RNA and uses thereof |
US11499151B2 (en) | 2017-04-28 | 2022-11-15 | Editas Medicine, Inc. | Methods and systems for analyzing guide RNA molecules |
US11530396B2 (en) | 2017-09-05 | 2022-12-20 | The University Of Tokyo | Modified CAS9 protein, and use thereof |
US11597924B2 (en) | 2016-03-25 | 2023-03-07 | Editas Medicine, Inc. | Genome editing systems comprising repair-modulating enzyme molecules and methods of their use |
US11667911B2 (en) | 2015-09-24 | 2023-06-06 | Editas Medicine, Inc. | Use of exonucleases to improve CRISPR/CAS-mediated genome editing |
US11680268B2 (en) | 2014-11-07 | 2023-06-20 | Editas Medicine, Inc. | Methods for improving CRISPR/Cas-mediated genome-editing |
US11866726B2 (en) | 2017-07-14 | 2024-01-09 | Editas Medicine, Inc. | Systems and methods for targeted integration and genome editing and detection thereof using integrated priming sites |
US11911415B2 (en) | 2015-06-09 | 2024-02-27 | Editas Medicine, Inc. | CRISPR/Cas-related methods and compositions for improving transplantation |
US12110545B2 (en) | 2017-01-06 | 2024-10-08 | Editas Medicine, Inc. | Methods of assessing nuclease cleavage |
Families Citing this family (346)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
CA2798703A1 (en) | 2010-05-10 | 2011-11-17 | The Regents Of The University Of California | Endoribonuclease compositions and methods of use thereof |
US11951140B2 (en) | 2011-02-04 | 2024-04-09 | Seed Health, Inc. | Modulation of an individual's gut microbiome to address osteoporosis and bone disease |
US11844720B2 (en) | 2011-02-04 | 2023-12-19 | Seed Health, Inc. | Method and system to reduce the likelihood of dental caries and halitosis |
US11951139B2 (en) | 2015-11-30 | 2024-04-09 | Seed Health, Inc. | Method and system for reducing the likelihood of osteoporosis |
US11523934B2 (en) | 2011-02-04 | 2022-12-13 | Seed Health, Inc. | Method and system to facilitate the growth of desired bacteria in a human's mouth |
US11191665B2 (en) | 2011-02-04 | 2021-12-07 | Joseph E. Kovarik | Method and system for reducing the likelihood of a porphyromonas gingivalis infection in a human being |
US11998479B2 (en) | 2011-02-04 | 2024-06-04 | Seed Health, Inc. | Method and system for addressing adverse effects on the oral microbiome and restoring gingival health caused by sodium lauryl sulphate exposure |
US10687975B2 (en) | 2011-02-04 | 2020-06-23 | Joseph E. Kovarik | Method and system to facilitate the growth of desired bacteria in a human's mouth |
US10583033B2 (en) | 2011-02-04 | 2020-03-10 | Katherine Rose Kovarik | Method and system for reducing the likelihood of a porphyromonas gingivalis infection in a human being |
CA2853829C (en) | 2011-07-22 | 2023-09-26 | President And Fellows Of Harvard College | Evaluation and improvement of nuclease cleavage specificity |
WO2014163886A1 (en) | 2013-03-12 | 2014-10-09 | President And Fellows Of Harvard College | Method of generating a three-dimensional nucleic acid containing matrix |
US11021737B2 (en) | 2011-12-22 | 2021-06-01 | President And Fellows Of Harvard College | Compositions and methods for analyte detection |
GB201122458D0 (en) | 2011-12-30 | 2012-02-08 | Univ Wageningen | Modified cascade ribonucleoproteins and uses thereof |
BR112014026294B1 (en) | 2012-04-25 | 2021-11-23 | Regeneron Pharmaceuticals, Inc | METHOD FOR MODIFYING A TARGET GENOME LOCUS IN A MOUSE EMBRYO STEM CELL(ES) |
WO2014018423A2 (en) * | 2012-07-25 | 2014-01-30 | The Broad Institute, Inc. | Inducible dna binding proteins and genome perturbation tools and applications thereof |
DK2931898T3 (en) | 2012-12-12 | 2016-06-20 | Massachusetts Inst Technology | CONSTRUCTION AND OPTIMIZATION OF SYSTEMS, PROCEDURES AND COMPOSITIONS FOR SEQUENCE MANIPULATION WITH FUNCTIONAL DOMAINS |
US8697359B1 (en) * | 2012-12-12 | 2014-04-15 | The Broad Institute, Inc. | CRISPR-Cas systems and methods for altering expression of gene products |
ES2701749T3 (en) | 2012-12-12 | 2019-02-25 | Broad Inst Inc | Methods, models, systems and apparatus to identify target sequences for Cas enzymes or CRISPR-Cas systems for target sequences and transmit results thereof |
BR112015013786B1 (en) * | 2012-12-12 | 2022-03-15 | President And Fellows Of Harvard College | crispr-cas component systems, methods and compositions for sequence manipulation |
RU2721275C2 (en) | 2012-12-12 | 2020-05-18 | Те Брод Инститьют, Инк. | Delivery, construction and optimization of systems, methods and compositions for sequence manipulation and use in therapy |
WO2014093694A1 (en) * | 2012-12-12 | 2014-06-19 | The Broad Institute, Inc. | Crispr-cas nickase systems, methods and compositions for sequence manipulation in eukaryotes |
IL300461A (en) | 2012-12-12 | 2023-04-01 | Harvard College | Engineering and optimization of improved systems, methods and enzyme compositions for sequence manipulation |
ES2536353T3 (en) | 2012-12-12 | 2015-05-22 | The Broad Institute, Inc. | Systems engineering, methods and guide compositions optimized for sequence manipulation |
CA2895155C (en) | 2012-12-17 | 2021-07-06 | President And Fellows Of Harvard College | Rna-guided human genome engineering |
AU2014207618A1 (en) | 2013-01-16 | 2015-08-06 | Emory University | Cas9-nucleic acid complexes and uses related thereto |
DK2971167T3 (en) | 2013-03-14 | 2019-11-04 | Caribou Biosciences Inc | COMPOSITIONS AND PROCEDURES FOR TARGETING NUCLEIC ACID WITH NUCLEIC ACID |
AU2014228981B2 (en) | 2013-03-15 | 2019-11-28 | The General Hospital Corporation | Using truncated guide RNAs (tru-gRNAs) to increase specificity for RNA-guided genome editing |
WO2014204578A1 (en) | 2013-06-21 | 2014-12-24 | The General Hospital Corporation | Using rna-guided foki nucleases (rfns) to increase specificity for rna-guided genome editing |
US10760064B2 (en) | 2013-03-15 | 2020-09-01 | The General Hospital Corporation | RNA-guided targeting of genetic and epigenomic regulatory proteins to specific genomic loci |
US9902973B2 (en) | 2013-04-11 | 2018-02-27 | Caribou Biosciences, Inc. | Methods of modifying a target nucleic acid with an argonaute |
ES2888250T3 (en) | 2013-04-16 | 2022-01-03 | Regeneron Pharma | Targeted modification of the rat genome |
ES2670531T3 (en) * | 2013-05-29 | 2018-05-30 | Cellectis S.A. | A method to produce an accurate DNA cleavage using the nickase activity of Cas9 |
US11414695B2 (en) * | 2013-05-29 | 2022-08-16 | Agilent Technologies, Inc. | Nucleic acid enrichment using Cas9 |
US20140356956A1 (en) | 2013-06-04 | 2014-12-04 | President And Fellows Of Harvard College | RNA-Guided Transcriptional Regulation |
CA3176690A1 (en) | 2013-06-04 | 2014-12-11 | President And Fellows Of Harvard College | Rna-guided transcriptional regulation |
EP3011030B1 (en) | 2013-06-17 | 2023-11-08 | The Broad Institute, Inc. | Optimized crispr-cas double nickase systems, methods and compositions for sequence manipulation |
KR20160030187A (en) | 2013-06-17 | 2016-03-16 | 더 브로드 인스티튜트, 인코퍼레이티드 | Delivery and use of the crispr-cas systems, vectors and compositions for hepatic targeting and therapy |
EP3011033B1 (en) | 2013-06-17 | 2020-02-19 | The Broad Institute, Inc. | Functional genomics using crispr-cas systems, compositions methods, screens and applications thereof |
CN106062197A (en) * | 2013-06-17 | 2016-10-26 | 布罗德研究所有限公司 | Delivery, engineering and optimization of tandem guide systems, methods and compositions for sequence manipulation |
WO2014204729A1 (en) | 2013-06-17 | 2014-12-24 | The Broad Institute Inc. | Delivery, use and therapeutic applications of the crispr-cas systems and compositions for targeting disorders and diseases using viral components |
KR102481330B1 (en) | 2013-07-10 | 2022-12-23 | 프레지던트 앤드 펠로우즈 오브 하바드 칼리지 | Orthogonal cas9 proteins for rna-guided gene regulation and editing |
US11306328B2 (en) | 2013-07-26 | 2022-04-19 | President And Fellows Of Harvard College | Genome engineering |
US10421957B2 (en) | 2013-07-29 | 2019-09-24 | Agilent Technologies, Inc. | DNA assembly using an RNA-programmable nickase |
US9163284B2 (en) | 2013-08-09 | 2015-10-20 | President And Fellows Of Harvard College | Methods for identifying a target site of a Cas9 nuclease |
US9359599B2 (en) | 2013-08-22 | 2016-06-07 | President And Fellows Of Harvard College | Engineered transcription activator-like effector (TALE) domains and uses thereof |
MX361154B (en) | 2013-08-22 | 2018-11-28 | Pioneer Hi Bred Int | Genome modification using guide polynucleotide/cas endonuclease systems and methods of use. |
US9340800B2 (en) | 2013-09-06 | 2016-05-17 | President And Fellows Of Harvard College | Extended DNA-sensing GRNAS |
US9388430B2 (en) | 2013-09-06 | 2016-07-12 | President And Fellows Of Harvard College | Cas9-recombinase fusion proteins and uses thereof |
US9737604B2 (en) | 2013-09-06 | 2017-08-22 | President And Fellows Of Harvard College | Use of cationic lipids to deliver CAS9 |
EP3988649A1 (en) | 2013-09-18 | 2022-04-27 | Kymab Limited | Methods, cells and organisms |
WO2015065964A1 (en) | 2013-10-28 | 2015-05-07 | The Broad Institute Inc. | Functional genomics using crispr-cas systems, compositions, methods, screens and applications thereof |
WO2015066119A1 (en) | 2013-10-30 | 2015-05-07 | North Carolina State University | Compositions and methods related to a type-ii crispr-cas system in lactobacillus buchneri |
WO2015070193A1 (en) * | 2013-11-11 | 2015-05-14 | Liu Oliver | Compositions and methods for targeted gene disruption in prokaryotes |
US9074199B1 (en) | 2013-11-19 | 2015-07-07 | President And Fellows Of Harvard College | Mutant Cas9 proteins |
WO2015075056A1 (en) * | 2013-11-19 | 2015-05-28 | Thermo Fisher Scientific Baltics Uab | Programmable enzymes for isolation of specific dna fragments |
US10787684B2 (en) | 2013-11-19 | 2020-09-29 | President And Fellows Of Harvard College | Large gene excision and insertion |
WO2015079056A1 (en) | 2013-11-28 | 2015-06-04 | Haplogen Genomics Gmbh | Somatic human cell line mutations |
BR112016013400B1 (en) | 2013-12-11 | 2023-02-14 | Regeneron Pharmaceuticals, Inc. | IN VITRO METHOD TO MODIFY A GENOME AT A GENOMIC LOCUS OF INTEREST IN A PLURIPOTENT CELL |
SI3080279T1 (en) | 2013-12-11 | 2019-01-31 | Regeneron Pharmaceuticals, Inc. | Methods and compositions for the targeted modification of a genome |
WO2015089486A2 (en) | 2013-12-12 | 2015-06-18 | The Broad Institute Inc. | Systems, methods and compositions for sequence manipulation with optimized functional crispr-cas systems |
EP3653704A1 (en) | 2013-12-12 | 2020-05-20 | The Broad Institute, Inc. | Compositions and methods of use of crispr-cas systems in nucleotide repeat disorders |
WO2015089427A1 (en) | 2013-12-12 | 2015-06-18 | The Broad Institute Inc. | Crispr-cas systems and methods for altering expression of gene products, structural information and inducible modular cas enzymes |
WO2015089364A1 (en) | 2013-12-12 | 2015-06-18 | The Broad Institute Inc. | Crystal structure of a crispr-cas system, and uses thereof |
US20150166984A1 (en) | 2013-12-12 | 2015-06-18 | President And Fellows Of Harvard College | Methods for correcting alpha-antitrypsin point mutations |
KR20160089527A (en) | 2013-12-12 | 2016-07-27 | 더 브로드 인스티튜트, 인코퍼레이티드 | Delivery, use and therapeutic applications of the crispr-cas systems and compositions for genome editing |
CN106029886B (en) | 2013-12-19 | 2021-02-05 | 阿迈瑞斯公司 | Method for genomic integration |
US11826388B2 (en) | 2013-12-20 | 2023-11-28 | Seed Health, Inc. | Topical application of Lactobacillus crispatus to ameliorate barrier damage and inflammation |
US11969445B2 (en) | 2013-12-20 | 2024-04-30 | Seed Health, Inc. | Probiotic composition and method for controlling excess weight, obesity, NAFLD and NASH |
US11672835B2 (en) | 2013-12-20 | 2023-06-13 | Seed Health, Inc. | Method for treating individuals having cancer and who are receiving cancer immunotherapy |
US12005085B2 (en) | 2013-12-20 | 2024-06-11 | Seed Health, Inc. | Probiotic method and composition for maintaining a healthy vaginal microbiome |
US11998574B2 (en) | 2013-12-20 | 2024-06-04 | Seed Health, Inc. | Method and system for modulating an individual's skin microbiome |
US11980643B2 (en) | 2013-12-20 | 2024-05-14 | Seed Health, Inc. | Method and system to modify an individual's gut-brain axis to provide neurocognitive protection |
US11529379B2 (en) | 2013-12-20 | 2022-12-20 | Seed Health, Inc. | Method and system for reducing the likelihood of developing colorectal cancer in an individual human being |
US11833177B2 (en) | 2013-12-20 | 2023-12-05 | Seed Health, Inc. | Probiotic to enhance an individual's skin microbiome |
US11839632B2 (en) | 2013-12-20 | 2023-12-12 | Seed Health, Inc. | Topical application of CRISPR-modified bacteria to treat acne vulgaris |
US11642382B2 (en) | 2013-12-20 | 2023-05-09 | Seed Health, Inc. | Method for treating an individual suffering from bladder cancer |
WO2015103153A1 (en) | 2013-12-31 | 2015-07-09 | The Regents Of The University Of California | Cas9 crystals and methods of use thereof |
MX2016009243A (en) * | 2014-01-14 | 2017-03-08 | Lam Therapeutics Inc | Mutagenesis methods. |
US10787654B2 (en) | 2014-01-24 | 2020-09-29 | North Carolina State University | Methods and compositions for sequence guiding Cas9 targeting |
EP4063503A1 (en) | 2014-02-11 | 2022-09-28 | The Regents of the University of Colorado, a body corporate | Crispr enabled multiplexed genome engineering |
CN106232814B (en) * | 2014-02-13 | 2021-05-11 | 宝生物工程(美国)有限公司 | Methods of depleting target molecules from an initial collection of nucleic acids, and compositions and kits for practicing same |
JP2017506893A (en) | 2014-02-18 | 2017-03-16 | デューク ユニバーシティ | Viral replication inactivating composition and method for producing and using the same |
EP3957735A1 (en) | 2014-03-05 | 2022-02-23 | Editas Medicine, Inc. | Crispr/cas-related methods and compositions for treating usher syndrome and retinitis pigmentosa |
DK3116997T3 (en) | 2014-03-10 | 2019-08-19 | Editas Medicine Inc | CRISPR / CAS-RELATED PROCEDURES AND COMPOSITIONS TO TREAT LEVER'S CONGENITAL AMAUROSIS 10 (LCA10) |
US11141493B2 (en) | 2014-03-10 | 2021-10-12 | Editas Medicine, Inc. | Compositions and methods for treating CEP290-associated disease |
US11339437B2 (en) | 2014-03-10 | 2022-05-24 | Editas Medicine, Inc. | Compositions and methods for treating CEP290-associated disease |
WO2015148863A2 (en) | 2014-03-26 | 2015-10-01 | Editas Medicine, Inc. | Crispr/cas-related methods and compositions for treating sickle cell disease |
CA2944978C (en) | 2014-04-08 | 2024-02-13 | North Carolina State University | Methods and compositions for rna-directed repression of transcription using crispr-associated genes |
GB201406970D0 (en) | 2014-04-17 | 2014-06-04 | Green Biologics Ltd | Targeted mutations |
GB201406968D0 (en) * | 2014-04-17 | 2014-06-04 | Green Biologics Ltd | Deletion mutants |
WO2015183026A1 (en) * | 2014-05-28 | 2015-12-03 | 주식회사 툴젠 | Method for separating target dna using inactivated target-specific nuclease |
WO2015184262A1 (en) | 2014-05-30 | 2015-12-03 | The Board Of Trustees Of The Leland Stanford Junior University | Compositions and methods of delivering treatments for latent viral infections |
MX2016016133A (en) | 2014-06-06 | 2017-08-04 | Regeneron Pharma | Methods and compositions for modifying a targeted locus. |
CA2953362A1 (en) | 2014-06-23 | 2015-12-30 | The General Hospital Corporation | Genomewide unbiased identification of dsbs evaluated by sequencing (guide-seq) |
DK3354732T3 (en) * | 2014-06-23 | 2020-04-06 | Regeneron Pharma | NUCLEASE MEDIATED DNA COLLECTION |
CN107002093B (en) | 2014-06-26 | 2021-06-25 | 瑞泽恩制药公司 | Methods and compositions for targeted genetic modification, and methods of use of these compositions |
CN106687594A (en) | 2014-07-11 | 2017-05-17 | 纳幕尔杜邦公司 | Compositions and methods for producing plants resistant to glyphosate herbicide |
EP4079847A1 (en) | 2014-07-30 | 2022-10-26 | President And Fellows Of Harvard College | Cas9 proteins including ligand-dependent inteins |
EP4194557A1 (en) | 2014-08-06 | 2023-06-14 | Institute for Basic Science | Genome editing using campylobacter jejuni crispr/cas system-derived rgen |
US11071289B2 (en) | 2014-08-14 | 2021-07-27 | Biocytogen Boston Corp | DNA knock-in system |
CA2958292A1 (en) * | 2014-08-19 | 2016-02-25 | President And Fellows Of Harvard College | Rna-guided systems for probing and mapping of nucleic acids |
CA2959070C (en) | 2014-08-27 | 2020-11-10 | Caribou Biosciences, Inc. | Methods for increasing cas9-mediated engineering efficiency |
EP3633032A3 (en) | 2014-08-28 | 2020-07-29 | North Carolina State University | Novel cas9 proteins and guiding features for dna targeting and genome editing |
WO2016036754A1 (en) | 2014-09-02 | 2016-03-10 | The Regents Of The University Of California | Methods and compositions for rna-directed target dna modification |
CA2956487A1 (en) | 2014-09-12 | 2016-03-17 | E. I. Du Pont De Nemours And Company | Generation of site-specific-integration sites for complex trait loci in corn and soybean, and methods of use |
CN107205353B (en) | 2014-09-26 | 2021-03-19 | 谱赛科美国股份有限公司 | Single Nucleotide Polymorphism (SNP) markers for stevia |
EP3207124B1 (en) | 2014-10-15 | 2019-06-26 | Regeneron Pharmaceuticals, Inc. | Methods and compositions for generating or maintaining pluripotent cells |
AU2015335618B2 (en) | 2014-10-24 | 2018-02-01 | Avectas Limited | Delivery across cell plasma membranes |
US9816080B2 (en) | 2014-10-31 | 2017-11-14 | President And Fellows Of Harvard College | Delivery of CAS9 via ARRDC1-mediated microvesicles (ARMMs) |
KR20160059994A (en) | 2014-11-19 | 2016-05-27 | 기초과학연구원 | A method for regulation of gene expression by expressing Cas9 protein from the two independent vector |
NZ731962A (en) | 2014-11-21 | 2022-07-01 | Regeneron Pharma | Methods and compositions for targeted genetic modification using paired guide rnas |
WO2016089433A1 (en) | 2014-12-03 | 2016-06-09 | Agilent Technologies, Inc. | Guide rna with chemical modifications |
EP3230451B1 (en) | 2014-12-12 | 2021-04-07 | The Broad Institute, Inc. | Protected guide rnas (pgrnas) |
BR112017011510B1 (en) * | 2014-12-17 | 2023-12-05 | Proqr Therapeutics Ii B.V. | OLIGONUCLEOTIDE CONSTRUCT FOR THE SITE-DIRECTED EDITING OF AN ADENOSINE NUCLEOTIDE INTO A TARGET RNA SEQUENCE IN A EUKARYOTIC CELL AND USE THEREOF |
WO2016100819A1 (en) | 2014-12-19 | 2016-06-23 | Regeneron Pharmaceuticals, Inc. | Methods and compositions for targeted genetic modification through single-step multiple targeting |
WO2016100857A1 (en) | 2014-12-19 | 2016-06-23 | Regeneron Pharmaceuticals, Inc. | Stem cells for modeling type 2 diabetes |
CN107406875B (en) | 2014-12-20 | 2021-12-07 | 阿克生物公司 | Compositions and methods for targeted subtraction, enrichment, and segmentation of nucleic acids using CRISPR/Cas system proteins |
SG11201704272YA (en) | 2014-12-31 | 2017-06-29 | Synthetic Genomics Inc | Compositions and methods for high efficiency in vivo genome editing |
EP3242938B1 (en) | 2015-01-09 | 2020-01-08 | Bio-Rad Laboratories, Inc. | Detection of genome editing |
EA039511B1 (en) | 2015-01-27 | 2022-02-04 | Инститьют Оф Дженетикс Энд Девелопментал Байолоджи, Чайниз Акэдеми Оф Сайенсиз | Method for conducting site-specific modification on entire plant via gene transient expression |
CA2975166C (en) | 2015-01-28 | 2020-01-14 | Pioneer Hi-Bred International, Inc. | Crispr hybrid dna/rna polynucleotides and methods of use |
US9944912B2 (en) | 2015-03-03 | 2018-04-17 | The General Hospital Corporation | Engineered CRISPR-Cas9 nucleases with altered PAM specificity |
EA038896B1 (en) | 2015-03-16 | 2021-11-03 | Институт Генетики И Биологии Развития Академии Наук Китая | Method of conducting site-directed modification of plant genomes using non-inheritable materials |
EP3553178A1 (en) | 2015-03-27 | 2019-10-16 | E. I. du Pont de Nemours and Company | Soybean u6 small nuclear rna gene promoters and their use in constitutive expression of small rna genes in plants |
ES2884838T3 (en) | 2015-04-06 | 2021-12-13 | Univ Leland Stanford Junior | Chemically modified guide RNA for CRISPR / CAS-mediated gene regulation |
JP2018522249A (en) | 2015-04-24 | 2018-08-09 | エディタス・メディシン、インコーポレイテッド | Evaluation of CAS 9 molecule / guide RNA molecule complex |
EP3292219B9 (en) | 2015-05-04 | 2022-05-18 | Ramot at Tel-Aviv University Ltd. | Methods and kits for fragmenting dna |
DE112016002056T5 (en) | 2015-05-06 | 2018-02-08 | Snipr Technologies Limited | Modifying microbial populations and modifying microbiomas |
AU2016265560B2 (en) * | 2015-05-15 | 2022-07-28 | Pioneer Hi-Bred International, Inc. | Rapid characterization of Cas endonuclease systems, PAM sequences and guide RNA elements |
CN107709555A (en) * | 2015-05-15 | 2018-02-16 | 达尔马科恩有限公司 | The unidirectional of synthesis for the gene editing of Cas9 mediations leads RNA |
EP3095870A1 (en) | 2015-05-19 | 2016-11-23 | Kws Saat Se | Methods for the in planta transformation of plants and manufacturing processes and products based and obtainable therefrom |
EP4039816A1 (en) | 2015-05-29 | 2022-08-10 | North Carolina State University | Methods for screening bacteria, archaea, algae, and yeast using crispr nucleic acids |
US10117911B2 (en) | 2015-05-29 | 2018-11-06 | Agenovir Corporation | Compositions and methods to treat herpes simplex virus infections |
JP2018516984A (en) | 2015-05-29 | 2018-06-28 | アジェノビア コーポレーション | Compositions and methods for cell targeted HPV treatment |
US10883103B2 (en) | 2015-06-02 | 2021-01-05 | Monsanto Technology Llc | Compositions and methods for delivery of a polynucleotide into a plant |
WO2016196887A1 (en) | 2015-06-03 | 2016-12-08 | Board Of Regents Of The University Of Nebraska | Dna editing using single-stranded dna |
WO2016196655A1 (en) * | 2015-06-03 | 2016-12-08 | The Regents Of The University Of California | Cas9 variants and methods of use thereof |
JP2018521642A (en) | 2015-06-12 | 2018-08-09 | ロンザ ウォカーズビル インコーポレーティッド | A method for nuclear reprogramming using synthetic transcription factors |
FI3307872T3 (en) | 2015-06-15 | 2023-10-16 | Univ North Carolina State | Methods and compositions for efficient delivery of nucleic acids and rna-based antimicrobials |
WO2016205759A1 (en) | 2015-06-18 | 2016-12-22 | The Broad Institute Inc. | Engineering and optimization of systems, methods, enzymes and guide scaffolds of cas9 orthologs and variants for sequence manipulation |
RU2752834C2 (en) | 2015-06-18 | 2021-08-09 | Те Брод Инститьют, Инк. | Crispr enzyme mutations reducing non-targeted effects |
US9580727B1 (en) | 2015-08-07 | 2017-02-28 | Caribou Biosciences, Inc. | Compositions and methods of engineered CRISPR-Cas9 systems using split-nexus Cas9-associated polynucleotides |
WO2017028768A1 (en) | 2015-08-14 | 2017-02-23 | Institute Of Genetics And Developmental Biology, Chinese Academy Of Sciences | Method for obtaining glyphosate-resistant rice by site-directed nucleotide substitution |
JP6986509B2 (en) | 2015-08-19 | 2021-12-22 | アーク バイオ, エルエルシー | Nucleic acid capture using a nucleic acid guided nuclease-based system |
JP6799586B2 (en) | 2015-08-28 | 2020-12-16 | ザ ジェネラル ホスピタル コーポレイション | Genetic manipulation CRISPR-Cas9 nuclease |
US9512446B1 (en) | 2015-08-28 | 2016-12-06 | The General Hospital Corporation | Engineered CRISPR-Cas9 nucleases |
US9926546B2 (en) | 2015-08-28 | 2018-03-27 | The General Hospital Corporation | Engineered CRISPR-Cas9 nucleases |
US11453864B2 (en) | 2015-09-08 | 2022-09-27 | University Of Massachusetts | DNase H activity of Neisseria meningitidis Cas9 |
EP3347467B1 (en) | 2015-09-11 | 2021-06-23 | The General Hospital Corporation | Full interrogation of nuclease dsbs and sequencing (find-seq) |
US11286480B2 (en) | 2015-09-28 | 2022-03-29 | North Carolina State University | Methods and compositions for sequence specific antimicrobials |
WO2017059313A1 (en) | 2015-09-30 | 2017-04-06 | The General Hospital Corporation | Comprehensive in vitro reporting of cleavage events by sequencing (circle-seq) |
WO2017066707A1 (en) | 2015-10-14 | 2017-04-20 | Life Technologies Corporation | Ribonucleoprotein transfection agents |
JP7067793B2 (en) | 2015-10-23 | 2022-05-16 | プレジデント アンド フェローズ オブ ハーバード カレッジ | Nucleobase editing factors and their use |
US9677090B2 (en) | 2015-10-23 | 2017-06-13 | Caribou Biosciences, Inc. | Engineered nucleic-acid targeting nucleic acids |
MX2018005611A (en) | 2015-11-03 | 2018-11-09 | Harvard College | Method and apparatus for volumetric imaging of a three-dimensional nucleic acid containing matrix. |
WO2017079428A1 (en) | 2015-11-04 | 2017-05-11 | President And Fellows Of Harvard College | Site specific germline modification |
WO2017081288A1 (en) | 2015-11-11 | 2017-05-18 | Lonza Ltd | Crispr-associated (cas) proteins with reduced immunogenicity |
KR101906491B1 (en) * | 2015-11-30 | 2018-12-05 | 기초과학연구원 | Composition for Genome Editing comprising Cas9 derived from F. novicida |
NZ742040A (en) * | 2015-12-04 | 2019-08-30 | Caribou Biosciences Inc | Engineered nucleic-acid targeting nucleic acids |
US9988624B2 (en) | 2015-12-07 | 2018-06-05 | Zymergen Inc. | Microbial strain improvement by a HTP genomic engineering platform |
US11208649B2 (en) | 2015-12-07 | 2021-12-28 | Zymergen Inc. | HTP genomic engineering platform |
WO2017100376A2 (en) | 2015-12-07 | 2017-06-15 | Zymergen, Inc. | Promoters from corynebacterium glutamicum |
WO2017112620A1 (en) | 2015-12-22 | 2017-06-29 | North Carolina State University | Methods and compositions for delivery of crispr based antimicrobials |
JP7449646B2 (en) * | 2015-12-30 | 2024-03-14 | アヴェクタス リミテッド | Vector-free delivery of gene editing proteins and compositions to cells and tissues |
SG11201805792PA (en) | 2016-01-11 | 2018-08-30 | Univ Leland Stanford Junior | Chimeric proteins and methods of regulating gene expression |
JP7012645B2 (en) | 2016-01-11 | 2022-01-28 | ザ ボード オブ トラスティーズ オブ ザ レランド スタンフォード ジュニア ユニバーシティー | Chimeric proteins and immunotherapeutic methods |
ES2919953T3 (en) | 2016-01-27 | 2022-07-29 | Oncorus Inc | Oncolytic viral vectors and uses thereof |
US11326161B2 (en) | 2016-02-18 | 2022-05-10 | President And Fellows Of Harvard College | Methods and systems of molecular recording by CRISPR-Cas system |
US11530253B2 (en) | 2016-02-25 | 2022-12-20 | The Children's Medical Center Corporation | Customized class switch of immunoglobulin genes in lymphoma and hybridoma by CRISPR/CAS9 technology |
JP2019507610A (en) | 2016-03-04 | 2019-03-22 | インドア バイオテクノロジーズ インコーポレイテッド | Fel d1 knockout and related compositions and methods based on CRISPR-Cas genome editing |
EP3433364A1 (en) | 2016-03-25 | 2019-01-30 | Editas Medicine, Inc. | Systems and methods for treating alpha 1-antitrypsin (a1at) deficiency |
JP7259182B2 (en) | 2016-04-25 | 2023-04-18 | プレジデント アンド フェローズ オブ ハーバード カレッジ | Hybridization chain reaction method for in situ molecular detection |
CN105907785B (en) * | 2016-05-05 | 2020-02-07 | 苏州吉玛基因股份有限公司 | Application of chemically synthesized crRNA in CRISPR/Cpf1 system in gene editing |
EP3458595A2 (en) | 2016-05-18 | 2019-03-27 | Amyris, Inc. | Compositions and methods for genomic integration of nucleic acids into exogenous landing pads |
CN113831407B (en) | 2016-05-20 | 2024-06-11 | 瑞泽恩制药公司 | Methods for disrupting immune tolerance using multiple guide RNAs |
PT3272867T (en) | 2016-06-02 | 2019-12-04 | Sigma Aldrich Co Llc | Using programmable dna binding proteins to enhance targeted genome modification |
GB201609811D0 (en) | 2016-06-05 | 2016-07-20 | Snipr Technologies Ltd | Methods, cells, systems, arrays, RNA and kits |
US10767175B2 (en) | 2016-06-08 | 2020-09-08 | Agilent Technologies, Inc. | High specificity genome editing using chemically modified guide RNAs |
US11293021B1 (en) | 2016-06-23 | 2022-04-05 | Inscripta, Inc. | Automated cell processing methods, modules, instruments, and systems |
CA3029254A1 (en) | 2016-06-24 | 2017-12-28 | The Regents Of The University Of Colorado, A Body Corporate | Methods for generating barcoded combinatorial libraries |
EP3474849A4 (en) | 2016-06-27 | 2020-07-29 | The Broad Institute, Inc. | Compositions and methods for detecting and treating diabetes |
KR102345898B1 (en) | 2016-06-30 | 2022-01-03 | 지머젠 인코포레이티드 | Methods for generating glucose permeabilization enzyme libraries and uses thereof |
KR102345899B1 (en) | 2016-06-30 | 2021-12-31 | 지머젠 인코포레이티드 | Methods for generating bacterial hemoglobin libraries and uses thereof |
SG11201901305YA (en) | 2016-07-29 | 2019-03-28 | Regeneron Pharma | Mice comprising mutations resulting in expression of c-truncated fibrillin-1 |
CA3032822A1 (en) | 2016-08-02 | 2018-02-08 | Editas Medicine, Inc. | Compositions and methods for treating cep290 associated disease |
IL308426A (en) | 2016-08-03 | 2024-01-01 | Harvard College | Adenosine nucleobase editors and uses thereof |
AU2017308889B2 (en) | 2016-08-09 | 2023-11-09 | President And Fellows Of Harvard College | Programmable Cas9-recombinase fusion proteins and uses thereof |
US11542509B2 (en) | 2016-08-24 | 2023-01-03 | President And Fellows Of Harvard College | Incorporation of unnatural amino acids into proteins using base editing |
US20190225974A1 (en) | 2016-09-23 | 2019-07-25 | BASF Agricultural Solutions Seed US LLC | Targeted genome optimization in plants |
WO2018067546A1 (en) | 2016-10-03 | 2018-04-12 | President And Fellows Of Harvard College | Delivery of therapeutic rnas via arrdc1-mediated microvesicles |
JP7399710B2 (en) | 2016-10-14 | 2023-12-18 | ザ ジェネラル ホスピタル コーポレイション | Epigenetically regulated site-specific nucleases |
CN110214180A (en) | 2016-10-14 | 2019-09-06 | 哈佛大学的校长及成员们 | The AAV of nucleobase editing machine is delivered |
GB201617559D0 (en) | 2016-10-17 | 2016-11-30 | University Court Of The University Of Edinburgh The | Swine comprising modified cd163 and associated methods |
CN109906030B (en) | 2016-11-04 | 2022-03-18 | 安健基因公司 | Genetically modified non-human animals and methods for producing heavy chain-only antibodies |
US9816093B1 (en) | 2016-12-06 | 2017-11-14 | Caribou Biosciences, Inc. | Engineered nucleic acid-targeting nucleic acids |
WO2018209712A1 (en) * | 2017-05-19 | 2018-11-22 | Tsinghua University | Engineering of a minimal sacas9 crispr/cas system for gene editing and transcriptional regulation optimized by enhanced guide rna |
WO2018119359A1 (en) | 2016-12-23 | 2018-06-28 | President And Fellows Of Harvard College | Editing of ccr5 receptor gene to protect against hiv infection |
EP3569708A4 (en) | 2017-01-13 | 2020-09-09 | Jichi Medical University | Aav vector for disrupting clotting-related factor gene on liver genome |
CN108314736B (en) * | 2017-01-18 | 2021-08-31 | 李燕强 | Method for promoting RNA degradation |
CA3047429A1 (en) | 2017-01-23 | 2018-07-26 | Regeneron Pharmaceuticals, Inc. | Hsd17b13 variants and uses thereof |
US11898179B2 (en) | 2017-03-09 | 2024-02-13 | President And Fellows Of Harvard College | Suppression of pain by gene editing |
WO2018165629A1 (en) | 2017-03-10 | 2018-09-13 | President And Fellows Of Harvard College | Cytosine to guanine base editor |
WO2018170184A1 (en) | 2017-03-14 | 2018-09-20 | Editas Medicine, Inc. | Systems and methods for the treatment of hemoglobinopathies |
IL269458B2 (en) | 2017-03-23 | 2024-02-01 | Harvard College | Nucleobase editors comprising nucleic acid programmable dna binding proteins |
WO2018195129A1 (en) | 2017-04-17 | 2018-10-25 | University Of Maryland, College Park | Embryonic cell cultures and methods of using the same |
MX2019012567A (en) | 2017-04-20 | 2020-02-13 | Egenesis Inc | Methods for generating genetically modified animals. |
US11591589B2 (en) | 2017-04-21 | 2023-02-28 | The General Hospital Corporation | Variants of Cpf1 (Cas12a) with altered PAM specificity |
US11732251B2 (en) | 2017-04-24 | 2023-08-22 | Dupont Nutrition Biosciences Aps | Anti-CRISPR polynucleotides and polypeptides and methods of use |
WO2018209158A2 (en) | 2017-05-10 | 2018-11-15 | Editas Medicine, Inc. | Crispr/rna-guided nuclease systems and methods |
US11560566B2 (en) | 2017-05-12 | 2023-01-24 | President And Fellows Of Harvard College | Aptazyme-embedded guide RNAs for use with CRISPR-Cas9 in genome editing and transcriptional activation |
US20200140842A1 (en) | 2017-05-25 | 2020-05-07 | The General Hospital Corporation | Bipartite base editor (bbe) architectures and type-ii-c-cas9 zinc finger editing |
CN109963944A (en) | 2017-06-20 | 2019-07-02 | 江苏恒瑞医药股份有限公司 | It is external to knock out crRNA used in the method and this method of target gene in T cell |
US9982279B1 (en) | 2017-06-23 | 2018-05-29 | Inscripta, Inc. | Nucleic acid-guided nucleases |
US10011849B1 (en) | 2017-06-23 | 2018-07-03 | Inscripta, Inc. | Nucleic acid-guided nucleases |
HUE058668T2 (en) | 2017-06-30 | 2022-09-28 | Inscripta Inc | Automated cell processing methods, modules, instruments, and systems |
RU2771110C2 (en) | 2017-07-26 | 2022-04-26 | Онкорус, Инк. | Oncolytic viral vectors and their application |
JP2020534795A (en) | 2017-07-28 | 2020-12-03 | プレジデント アンド フェローズ オブ ハーバード カレッジ | Methods and Compositions for Evolving Base Editing Factors Using Phage-Supported Continuous Evolution (PACE) |
US20190032156A1 (en) | 2017-07-31 | 2019-01-31 | Regeneron Pharmaceuticals, Inc. | Methods and compositions for assessing crispr/cas-induced recombination with an exogenous donor nucleic acid in vivo |
CN110891420B (en) | 2017-07-31 | 2022-06-03 | 瑞泽恩制药公司 | CAS transgenic mouse embryonic stem cell, mouse and application thereof |
EP3585160A2 (en) | 2017-07-31 | 2020-01-01 | Regeneron Pharmaceuticals, Inc. | Crispr reporter non-human animals and uses thereof |
AU2018320865B2 (en) | 2017-08-23 | 2023-09-14 | The General Hospital Corporation | Engineered CRISPR-Cas9 nucleases with altered PAM specificity |
US10738327B2 (en) | 2017-08-28 | 2020-08-11 | Inscripta, Inc. | Electroporation cuvettes for automation |
EP3676376A2 (en) | 2017-08-30 | 2020-07-08 | President and Fellows of Harvard College | High efficiency base editors comprising gam |
EP4276185A3 (en) | 2017-09-29 | 2024-02-21 | Regeneron Pharmaceuticals, Inc. | Rodents comprising a humanized ttr locus and methods of use |
CA3074927A1 (en) | 2017-09-30 | 2019-04-04 | Inscripta, Inc. | Flow through electroporation instrumentation |
EP3694993A4 (en) | 2017-10-11 | 2021-10-13 | The General Hospital Corporation | Methods for detecting site-specific and spurious genomic deamination induced by base editing technologies |
JP2021500036A (en) | 2017-10-16 | 2021-01-07 | ザ ブロード インスティテュート, インコーポレーテッドThe Broad Institute, Inc. | Use of adenosine base editing factors |
CN111448313A (en) | 2017-11-16 | 2020-07-24 | 阿斯利康(瑞典)有限公司 | Compositions and methods for improving the effectiveness of Cas 9-based knock-in strategies |
AU2019207409B2 (en) | 2018-01-12 | 2023-02-23 | Basf Se | Gene underlying the number of spikelets per spike qtl in wheat on chromosome 7a |
EP3755792A4 (en) | 2018-02-23 | 2021-12-08 | Pioneer Hi-Bred International, Inc. | Novel cas9 orthologs |
WO2019178426A1 (en) | 2018-03-14 | 2019-09-19 | Editas Medicine, Inc. | Systems and methods for the treatment of hemoglobinopathies |
AU2019239880B2 (en) | 2018-03-19 | 2023-11-30 | Regeneron Pharmaceuticals, Inc. | Transcription modulation in animals using CRISPR/Cas systems |
US10760075B2 (en) | 2018-04-30 | 2020-09-01 | Snipr Biome Aps | Treating and preventing microbial infections |
EP3775159A4 (en) | 2018-03-29 | 2022-01-19 | Inscripta, Inc. | Automated control of cell growth rates for induction and transformation |
WO2019195738A1 (en) | 2018-04-06 | 2019-10-10 | Children's Medical Center Corporation | Compositions and methods for somatic cell reprogramming and modulating imprinting |
US10376889B1 (en) | 2018-04-13 | 2019-08-13 | Inscripta, Inc. | Automated cell processing instruments comprising reagent cartridges |
JP7460539B2 (en) | 2018-04-17 | 2024-04-02 | ザ ジェネラル ホスピタル コーポレイション | IN VITRO sensitive assays for substrate selectivity and sites of binding, modification, and cleavage of nucleic acids |
US10526598B2 (en) | 2018-04-24 | 2020-01-07 | Inscripta, Inc. | Methods for identifying T-cell receptor antigens |
US10501738B2 (en) | 2018-04-24 | 2019-12-10 | Inscripta, Inc. | Automated instrumentation for production of peptide libraries |
US10858761B2 (en) | 2018-04-24 | 2020-12-08 | Inscripta, Inc. | Nucleic acid-guided editing of exogenous polynucleotides in heterologous cells |
WO2019222545A1 (en) | 2018-05-16 | 2019-11-21 | Synthego Corporation | Methods and systems for guide rna design and use |
EP3813974A4 (en) | 2018-06-30 | 2022-08-03 | Inscripta, Inc. | Instruments, modules, and methods for improved detection of edited sequences in live cells |
US11142740B2 (en) | 2018-08-14 | 2021-10-12 | Inscripta, Inc. | Detection of nuclease edited sequences in automated modules and instruments |
US10752874B2 (en) | 2018-08-14 | 2020-08-25 | Inscripta, Inc. | Instruments, modules, and methods for improved detection of edited sequences in live cells |
US10532324B1 (en) | 2018-08-14 | 2020-01-14 | Inscripta, Inc. | Instruments, modules, and methods for improved detection of edited sequences in live cells |
BR112021003545A2 (en) | 2018-08-29 | 2021-05-18 | Amyris, Inc. | cells and methods for selection-based assay |
AU2019363487A1 (en) | 2018-08-30 | 2021-04-15 | Inscripta, Inc. | Improved detection of nuclease edited sequences in automated modules and instruments |
US20210198642A1 (en) | 2018-09-07 | 2021-07-01 | Astrazeneca Ab | Compositions and methods for improved nucleases |
EP3861120A4 (en) | 2018-10-01 | 2023-08-16 | North Carolina State University | Recombinant type i crispr-cas system |
WO2020076976A1 (en) | 2018-10-10 | 2020-04-16 | Readcoor, Inc. | Three-dimensional spatial molecular indexing |
US11851663B2 (en) | 2018-10-14 | 2023-12-26 | Snipr Biome Aps | Single-vector type I vectors |
US10604746B1 (en) | 2018-10-22 | 2020-03-31 | Inscripta, Inc. | Engineered enzymes |
US11214781B2 (en) | 2018-10-22 | 2022-01-04 | Inscripta, Inc. | Engineered enzyme |
JP2022505440A (en) | 2018-11-01 | 2022-01-14 | キージーン ナムローゼ フェンノートシャップ | Dual guide RNA for CRISPR / Cas genome editing in plant cells |
CA3117768A1 (en) | 2018-11-28 | 2020-06-04 | Keygene N.V. | Targeted enrichment by endonuclease protection |
KR20200071198A (en) | 2018-12-10 | 2020-06-19 | 네오이뮨텍, 인코퍼레이티드 | Development of new adoptive T cell immunotherapy by modification of Nrf2 expression |
JP2022514493A (en) | 2018-12-14 | 2022-02-14 | パイオニア ハイ-ブレッド インターナショナル, インコーポレイテッド | A novel CRISPR-CAS system for genome editing |
KR20210105914A (en) | 2018-12-20 | 2021-08-27 | 리제너론 파마슈티칼스 인코포레이티드 | Nuclease-mediated repeat expansion |
WO2020163396A1 (en) | 2019-02-04 | 2020-08-13 | The General Hospital Corporation | Adenine dna base editor variants with reduced off-target rna editing |
US10982200B2 (en) | 2019-02-14 | 2021-04-20 | Metagenomi Ip Technologies, Llc | Enzymes with RuvC domains |
EP3924477A4 (en) * | 2019-02-14 | 2023-03-29 | Metagenomi, Inc. | Enzymes with ruvc domains |
SG11202108091YA (en) | 2019-03-18 | 2021-08-30 | Regeneron Pharma | Crispr/cas screening platform to identify genetic modifiers of tau seeding or aggregation |
KR102683424B1 (en) | 2019-03-18 | 2024-07-10 | 리제너론 파마슈티칼스 인코포레이티드 | CRISPR/Cas dropout screening platform to identify genetic vulnerabilities associated with tau aggregation |
KR20210142210A (en) | 2019-03-19 | 2021-11-24 | 더 브로드 인스티튜트, 인코퍼레이티드 | Methods and compositions for editing nucleotide sequences |
US11001831B2 (en) | 2019-03-25 | 2021-05-11 | Inscripta, Inc. | Simultaneous multiplex genome editing in yeast |
CA3134168A1 (en) | 2019-03-25 | 2020-10-01 | Inscripta, Inc. | Simultaneous multiplex genome editing in yeast |
JP2022527766A (en) | 2019-03-27 | 2022-06-06 | パイオニア ハイ-ブレッド インターナショナル, インコーポレイテッド | Transformation of extraplant fragments |
AU2020256225A1 (en) | 2019-04-03 | 2021-09-02 | Regeneron Pharmaceuticals, Inc. | Methods and compositions for insertion of antibody coding sequences into a safe harbor locus |
US11111504B2 (en) | 2019-04-04 | 2021-09-07 | Regeneron Pharmaceuticals, Inc. | Methods for scarless introduction of targeted modifications into targeting vectors |
ES2966625T3 (en) | 2019-04-04 | 2024-04-23 | Regeneron Pharma | Rodents comprising a humanized coagulation factor 12 locus |
KR20210148286A (en) | 2019-04-05 | 2021-12-07 | 고꾸리쯔 다이가꾸 호우징 오사까 다이가꾸 | Method for preparing lysed cells |
MA55598A (en) | 2019-04-12 | 2022-02-16 | Astrazeneca Ab | COMPOSITIONS AND METHODS FOR ENHANCED GENE EDITING |
CN113874510A (en) | 2019-06-04 | 2021-12-31 | 瑞泽恩制药公司 | Non-human animals including humanized TTR loci with beta glide mutations and methods of use |
CN113939593A (en) | 2019-06-06 | 2022-01-14 | 因思科瑞普特公司 | Treatment for recursive nucleic acid-guided cell editing |
EP3796776A1 (en) | 2019-06-07 | 2021-03-31 | Regeneron Pharmaceuticals, Inc. | Non-human animals comprising a humanized albumin locus |
US11845957B2 (en) | 2019-06-14 | 2023-12-19 | Regeneron Pharmaceuticals, Inc. | Models of tauopathy |
US10907125B2 (en) | 2019-06-20 | 2021-02-02 | Inscripta, Inc. | Flow through electroporation modules and instrumentation |
WO2020257395A1 (en) | 2019-06-21 | 2020-12-24 | Inscripta, Inc. | Genome-wide rationally-designed mutations leading to enhanced lysine production in e. coli |
US10927385B2 (en) | 2019-06-25 | 2021-02-23 | Inscripta, Inc. | Increased nucleic-acid guided cell editing in yeast |
CN214973877U (en) | 2019-08-09 | 2021-12-03 | 胡桃钳医疗公司 | Microfluidic device and microfluidic path device for forming therapeutic polynucleotides |
CA3153980A1 (en) | 2019-09-13 | 2021-03-18 | Regeneron Pharmaceuticals, Inc. | Transcription modulation in animals using crispr/cas systems delivered by lipid nanoparticles |
JP2022553573A (en) | 2019-11-08 | 2022-12-23 | リジェネロン・ファーマシューティカルズ・インコーポレイテッド | CRISPR and AAV strategies for X-linked juvenile retinal isolation therapy |
WO2021102059A1 (en) | 2019-11-19 | 2021-05-27 | Inscripta, Inc. | Methods for increasing observed editing in bacteria |
WO2021108363A1 (en) | 2019-11-25 | 2021-06-03 | Regeneron Pharmaceuticals, Inc. | Crispr/cas-mediated upregulation of humanized ttr allele |
WO2021118626A1 (en) | 2019-12-10 | 2021-06-17 | Inscripta, Inc. | Novel mad nucleases |
US10704033B1 (en) | 2019-12-13 | 2020-07-07 | Inscripta, Inc. | Nucleic acid-guided nucleases |
IL292895A (en) | 2019-12-18 | 2022-07-01 | Inscripta Inc | Cascade/dcas3 complementation assays for in vivo detection of nucleic acid-guided nuclease edited cells |
US10689669B1 (en) | 2020-01-11 | 2020-06-23 | Inscripta, Inc. | Automated multi-module cell processing methods, instruments, and systems |
EP4096770A1 (en) | 2020-01-27 | 2022-12-07 | Inscripta, Inc. | Electroporation modules and instrumentation |
WO2021178556A1 (en) | 2020-03-04 | 2021-09-10 | Regeneron Pharmaceuticals, Inc. | Methods and compositions for sensitization of tumor cells to immune therapy |
US20230096378A1 (en) | 2020-03-12 | 2023-03-30 | Institute For Basic Science | Composition for inducing apoptosis of cells having genomic sequence variation and method for inducing apoptosis of cells by using composition |
WO2021195079A1 (en) | 2020-03-23 | 2021-09-30 | Regeneron Pharmaceuticals, Inc. | Non-human animals comprising a humanized ttr locus comprising a v30m mutation and methods of use |
MX2022012110A (en) | 2020-03-31 | 2022-10-18 | Metagenomi Inc | Class ii, type ii crispr systems. |
US12057197B2 (en) | 2020-04-03 | 2024-08-06 | Creyon Bio, Inc. | Oligonucleotide-based machine learning |
US20210332388A1 (en) | 2020-04-24 | 2021-10-28 | Inscripta, Inc. | Compositions, methods, modules and instruments for automated nucleic acid-guided nuclease editing in mammalian cells |
US20230193212A1 (en) | 2020-05-06 | 2023-06-22 | Orchard Therapeutics (Europe) Limited | Treatment for neurodegenerative diseases |
GB2614813A (en) | 2020-05-08 | 2023-07-19 | Harvard College | Methods and compositions for simultaneous editing of both strands of a target double-stranded nucleotide sequence |
US11787841B2 (en) | 2020-05-19 | 2023-10-17 | Inscripta, Inc. | Rationally-designed mutations to the thrA gene for enhanced lysine production in E. coli |
US11299731B1 (en) | 2020-09-15 | 2022-04-12 | Inscripta, Inc. | CRISPR editing to embed nucleic acid landing pads into genomes of live cells |
JP2023543602A (en) | 2020-10-06 | 2023-10-17 | キージーン ナムローゼ フェンノートシャップ | Targeted sequence addition |
US20230416709A1 (en) | 2020-11-06 | 2023-12-28 | Editforce, Inc. | Foki nuclease domain mutant |
US11512297B2 (en) | 2020-11-09 | 2022-11-29 | Inscripta, Inc. | Affinity tag for recombination protein recruitment |
WO2022103799A1 (en) | 2020-11-10 | 2022-05-19 | Industrial Microbes, Inc. | Microorganisms capable of producing poly(hiba) from feedstock |
US20240002904A1 (en) | 2020-11-24 | 2024-01-04 | Keygene N.V. | Targeted enrichment using nanopore selective sequencing |
US20240002839A1 (en) | 2020-12-02 | 2024-01-04 | Decibel Therapeutics, Inc. | Crispr sam biosensor cell lines and methods of use thereof |
US11306298B1 (en) | 2021-01-04 | 2022-04-19 | Inscripta, Inc. | Mad nucleases |
US11332742B1 (en) | 2021-01-07 | 2022-05-17 | Inscripta, Inc. | Mad nucleases |
US11884924B2 (en) | 2021-02-16 | 2024-01-30 | Inscripta, Inc. | Dual strand nucleic acid-guided nickase editing |
WO2022219175A1 (en) | 2021-04-15 | 2022-10-20 | Keygene N.V. | Mobile endonucleases for heritable mutations |
CN117136003A (en) | 2021-04-15 | 2023-11-28 | 主基因有限公司 | Co-regenerated recalcitrant plants |
WO2022240846A1 (en) | 2021-05-10 | 2022-11-17 | Sqz Biotechnologies Company | Methods for delivering genome editing molecules to the nucleus or cytosol of a cell and uses thereof |
JP2024518793A (en) | 2021-05-27 | 2024-05-02 | アストラゼネカ・アクチエボラーグ | CAS9 Effector Proteins with Enhanced Stability |
WO2022251644A1 (en) | 2021-05-28 | 2022-12-01 | Lyell Immunopharma, Inc. | Nr4a3-deficient immune cells and uses thereof |
US20230052243A1 (en) | 2021-06-02 | 2023-02-16 | Lyell Immunopharma, Inc. | Nr4a-deficient cells expressing c-jun and uses thereof |
US11814689B2 (en) | 2021-07-21 | 2023-11-14 | Montana State University | Nucleic acid detection using type III CRISPR complex |
AU2022343300A1 (en) | 2021-09-10 | 2024-04-18 | Agilent Technologies, Inc. | Guide rnas with chemical modification for prime editing |
CN118119707A (en) | 2021-09-30 | 2024-05-31 | 阿斯利康(瑞典)有限公司 | Use of inhibitors to increase CRISPR/Cas insertion efficiency |
IL311962A (en) | 2021-10-14 | 2024-06-01 | Lonza Sales Ag | Modified producer cells for extracellular vesicle production |
CN118251491A (en) | 2021-10-28 | 2024-06-25 | 瑞泽恩制药公司 | CRISPR/Cas related methods and compositions for knockout of C5 |
KR20240110597A (en) * | 2021-11-24 | 2024-07-15 | 메타지노미, 인크. | endonuclease system |
KR20240117571A (en) | 2021-12-08 | 2024-08-01 | 리제너론 파마슈티칼스 인코포레이티드 | Mutant myocilin disease model and uses thereof |
GB202118058D0 (en) | 2021-12-14 | 2022-01-26 | Univ Warwick | Methods to increase yields in crops |
US20230279442A1 (en) | 2021-12-15 | 2023-09-07 | Versitech Limited | Engineered cas9-nucleases and method of use thereof |
EP4447649A1 (en) | 2021-12-17 | 2024-10-23 | Keygene N.V. | Double decapitation of plants |
KR20240128067A (en) | 2021-12-29 | 2024-08-23 | 브리스톨-마이어스 스큅 컴퍼니 | Generation of landing pad cell lines |
WO2023150181A1 (en) | 2022-02-01 | 2023-08-10 | President And Fellows Of Harvard College | Methods and compositions for treating cancer |
KR20240135629A (en) | 2022-02-02 | 2024-09-11 | 리제너론 파마슈티칼스 인코포레이티드 | Anti-TfR:GAA and anti-CD63:GAA insertions for the treatment of Pompe disease |
WO2023212677A2 (en) | 2022-04-29 | 2023-11-02 | Regeneron Pharmaceuticals, Inc. | Identification of tissue-specific extragenic safe harbors for gene therapy approaches |
WO2023220603A1 (en) | 2022-05-09 | 2023-11-16 | Regeneron Pharmaceuticals, Inc. | Vectors and methods for in vivo antibody production |
WO2023225665A1 (en) | 2022-05-19 | 2023-11-23 | Lyell Immunopharma, Inc. | Polynucleotides targeting nr4a3 and uses thereof |
WO2023235725A2 (en) | 2022-05-31 | 2023-12-07 | Regeneron Pharmaceuticals, Inc. | Crispr-based therapeutics for c9orf72 repeat expansion disease |
WO2023235726A2 (en) | 2022-05-31 | 2023-12-07 | Regeneron Pharmaceuticals, Inc. | Crispr interference therapeutics for c9orf72 repeat expansion disease |
GB202209518D0 (en) | 2022-06-29 | 2022-08-10 | Snipr Biome Aps | Treating & preventing E coli infections |
GB2621813A (en) | 2022-06-30 | 2024-02-28 | Univ Newcastle | Preventing disease recurrence in Mitochondrial replacement therapy |
WO2024026474A1 (en) | 2022-07-29 | 2024-02-01 | Regeneron Pharmaceuticals, Inc. | Compositions and methods for transferrin receptor (tfr)-mediated delivery to the brain and muscle |
WO2024031053A1 (en) | 2022-08-05 | 2024-02-08 | Regeneron Pharmaceuticals, Inc. | Aggregation-resistant variants of tdp-43 |
WO2024064958A1 (en) | 2022-09-23 | 2024-03-28 | Lyell Immunopharma, Inc. | Methods for culturing nr4a-deficient cells |
WO2024064952A1 (en) | 2022-09-23 | 2024-03-28 | Lyell Immunopharma, Inc. | Methods for culturing nr4a-deficient cells overexpressing c-jun |
WO2024073606A1 (en) | 2022-09-28 | 2024-04-04 | Regeneron Pharmaceuticals, Inc. | Antibody resistant modified receptors to enhance cell-based therapies |
WO2024077174A1 (en) | 2022-10-05 | 2024-04-11 | Lyell Immunopharma, Inc. | Methods for culturing nr4a-deficient cells |
WO2024098002A1 (en) | 2022-11-04 | 2024-05-10 | Regeneron Pharmaceuticals, Inc. | Calcium voltage-gated channel auxiliary subunit gamma 1 (cacng1) binding proteins and cacng1-mediated delivery to skeletal muscle |
US20240173426A1 (en) | 2022-11-14 | 2024-05-30 | Regeneron Pharmaceuticals, Inc. | Compositions and methods for fibroblast growth factor receptor 3-mediated delivery to astrocytes |
WO2024133851A1 (en) | 2022-12-22 | 2024-06-27 | Keygene N.V. | Regeneration by protoplast callus grafting |
WO2024159071A1 (en) | 2023-01-27 | 2024-08-02 | Regeneron Pharmaceuticals, Inc. | Modified rhabdovirus glycoproteins and uses thereof |
WO2024201368A1 (en) | 2023-03-29 | 2024-10-03 | Astrazeneca Ab | Use of inhibitors to increase efficiency of crispr/cas insertions |
CN116617414B (en) * | 2023-03-31 | 2024-04-05 | 中国农业大学 | Liposome and preparation method and application thereof |
Family Cites Families (27)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
US3862002A (en) * | 1962-05-08 | 1975-01-21 | Sanfar Lab Inc | Production of physiologically active placental substances |
CA2961849C (en) | 2005-08-26 | 2022-08-02 | Dupont Nutrition Biosciences Aps | Use of crispr associated genes (cas) |
PL2126130T3 (en) | 2007-03-02 | 2015-10-30 | Dupont Nutrition Biosci Aps | Cultures with improved phage resistance |
US20100076057A1 (en) | 2008-09-23 | 2010-03-25 | Northwestern University | TARGET DNA INTERFERENCE WITH crRNA |
US8586526B2 (en) * | 2010-05-17 | 2013-11-19 | Sangamo Biosciences, Inc. | DNA-binding proteins and uses thereof |
EP2580331A4 (en) * | 2010-06-14 | 2013-11-27 | Univ Iowa State Res Found Inc | Nuclease activity of tal effector and foki fusion protein |
CA2805442C (en) * | 2010-07-21 | 2020-05-12 | Sangamo Biosciences, Inc. | Methods and compositions for modification of an hla locus |
WO2013141680A1 (en) | 2012-03-20 | 2013-09-26 | Vilnius University | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX |
US9637739B2 (en) | 2012-03-20 | 2017-05-02 | Vilnius University | RNA-directed DNA cleavage by the Cas9-crRNA complex |
MA37663B1 (en) | 2012-05-25 | 2019-12-31 | Univ California | Methods and compositions for modifying rna-directed target DNA and modulating rna-directed transcription |
KR102052286B1 (en) * | 2012-10-23 | 2019-12-06 | 주식회사 툴젠 | Composition for cleaving a target DNA comprising a guideRNA specific for the target DNA and Cas protein-encoding nucleicacid or Cas protein, and use thereof |
DK3138910T3 (en) | 2012-12-06 | 2017-10-16 | Sigma Aldrich Co Llc | CRISPR-BASED RE-MODIFICATION AND REGULATION |
RU2721275C2 (en) | 2012-12-12 | 2020-05-18 | Те Брод Инститьют, Инк. | Delivery, construction and optimization of systems, methods and compositions for sequence manipulation and use in therapy |
US8697359B1 (en) | 2012-12-12 | 2014-04-15 | The Broad Institute, Inc. | CRISPR-Cas systems and methods for altering expression of gene products |
ES2536353T3 (en) * | 2012-12-12 | 2015-05-22 | The Broad Institute, Inc. | Systems engineering, methods and guide compositions optimized for sequence manipulation |
BR112015013786B1 (en) | 2012-12-12 | 2022-03-15 | President And Fellows Of Harvard College | crispr-cas component systems, methods and compositions for sequence manipulation |
WO2014093701A1 (en) * | 2012-12-12 | 2014-06-19 | The Broad Institute, Inc. | Functional genomics using crispr-cas systems, compositions, methods, knock out libraries and applications thereof |
CA2895155C (en) * | 2012-12-17 | 2021-07-06 | President And Fellows Of Harvard College | Rna-guided human genome engineering |
CA3176690A1 (en) * | 2013-06-04 | 2014-12-11 | President And Fellows Of Harvard College | Rna-guided transcriptional regulation |
US20150275231A1 (en) * | 2014-03-31 | 2015-10-01 | Mice With Horns, Llc | Method of Preventing or Reducing Virus Transmission in Animals |
EP4400597A3 (en) * | 2015-10-09 | 2024-10-16 | Monsanto Technology LLC | Novel rna-guided nucleases and uses thereof |
CN110312792B (en) * | 2016-12-14 | 2024-04-09 | 瓦赫宁根大学 | Thermostable Cas9 nucleases |
CN111448313A (en) * | 2017-11-16 | 2020-07-24 | 阿斯利康(瑞典)有限公司 | Compositions and methods for improving the effectiveness of Cas 9-based knock-in strategies |
WO2019217336A2 (en) * | 2018-05-06 | 2019-11-14 | Massachusetts Institute Of Technology | APPLICATIONS OF STREPTOCOCCUS-DERIVED Cas9 NUCLEASSES ON MINIMAL ADENINE-RICH PAM TARGETS |
US11756194B2 (en) * | 2018-07-11 | 2023-09-12 | Vilniaus Universitetas; | Computer-implemented process on an image of a biological sample |
WO2022261115A1 (en) * | 2021-06-07 | 2022-12-15 | Yale University | Peptide nucleic acids for spatiotemporal control of crispr-cas binding |
WO2023025767A1 (en) * | 2021-08-23 | 2023-03-02 | Max-Delbrück-Centrum Für Molekulare Medizin In Der Helmholtz-Gemeinschaft | Method for cas9 nickase-mediated gene editing |
-
2013
- 2013-03-15 US US14/385,241 patent/US9637739B2/en active Active
- 2013-03-20 CN CN201380023255.3A patent/CN104520429B/en active Active
- 2013-03-20 BR BR112014023353A patent/BR112014023353A2/en not_active Application Discontinuation
- 2013-03-20 ES ES13715080T patent/ES2749108T3/en active Active
- 2013-03-20 EA EA201491728A patent/EA029544B1/en not_active IP Right Cessation
- 2013-03-20 CA CA2867849A patent/CA2867849C/en active Active
- 2013-03-20 MX MX2014011279A patent/MX370435B/en active IP Right Grant
- 2013-03-20 US US14/385,857 patent/US20150050699A1/en not_active Abandoned
- 2013-03-20 EP EP19179124.3A patent/EP3594341A1/en active Pending
- 2013-03-20 PT PT137150801T patent/PT2828386T/en unknown
- 2013-03-20 CA CA3124374A patent/CA3124374C/en active Active
- 2013-03-20 WO PCT/US2013/033106 patent/WO2013142578A1/en active Application Filing
- 2013-03-20 HU HUE13715080A patent/HUE046295T2/en unknown
- 2013-03-20 EP EP13715080.1A patent/EP2828386B1/en active Active
- 2013-03-20 CN CN202111462778.0A patent/CN114410625B/en active Active
- 2013-03-20 IN IN7846DEN2014 patent/IN2014DN07846A/en unknown
- 2013-03-20 PL PL13715080T patent/PL2828386T3/en unknown
- 2013-03-20 JP JP2015501880A patent/JP6423338B2/en active Active
- 2013-03-20 DK DK13715080.1T patent/DK2828386T3/en active
-
2014
- 2014-09-19 MX MX2019009736A patent/MX2019009736A/en unknown
-
2015
- 2015-04-10 US US14/683,443 patent/US20150240261A1/en not_active Abandoned
- 2015-06-18 US US14/743,764 patent/US20150291961A1/en not_active Abandoned
- 2015-07-27 HK HK15107124.7A patent/HK1206392A1/en unknown
-
2017
- 2017-12-07 US US15/834,578 patent/US11555187B2/en active Active
-
2018
- 2018-10-01 US US16/148,783 patent/US10844378B2/en active Active
- 2018-10-18 JP JP2018196574A patent/JP7186574B2/en active Active
-
2020
- 2020-10-16 JP JP2020174803A patent/JP7113877B2/en active Active
-
2022
- 2022-07-05 US US17/857,480 patent/US20230123754A1/en active Pending
- 2022-12-13 US US18/065,006 patent/US20230272394A1/en active Pending
Non-Patent Citations (1)
Title |
---|
Gaberc-Porekar et al., Chem. Eng. Technol. 2005, 28(1)1306-1324 * |
Cited By (109)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
US10844378B2 (en) | 2012-03-20 | 2020-11-24 | Vilnius University | RNA-directed DNA cleavage by the Cas9-crRNA complex |
US11555187B2 (en) | 2012-03-20 | 2023-01-17 | Vilnius University | RNA-directed DNA cleavage by the Cas9-crRNA complex |
US11001863B2 (en) | 2012-05-25 | 2021-05-11 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10640791B2 (en) | 2012-05-25 | 2020-05-05 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US12123015B2 (en) | 2012-05-25 | 2024-10-22 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11186849B2 (en) | 2012-05-25 | 2021-11-30 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11274318B2 (en) | 2012-05-25 | 2022-03-15 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10227611B2 (en) | 2012-05-25 | 2019-03-12 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10266850B2 (en) | 2012-05-25 | 2019-04-23 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11293034B2 (en) | 2012-05-25 | 2022-04-05 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10301651B2 (en) | 2012-05-25 | 2019-05-28 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10308961B2 (en) | 2012-05-25 | 2019-06-04 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10337029B2 (en) | 2012-05-25 | 2019-07-02 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10351878B2 (en) | 2012-05-25 | 2019-07-16 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10358658B2 (en) | 2012-05-25 | 2019-07-23 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10358659B2 (en) | 2012-05-25 | 2019-07-23 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10385360B2 (en) | 2012-05-25 | 2019-08-20 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10400253B2 (en) | 2012-05-25 | 2019-09-03 | The Regents Of The University Of California | Methods and compositions or RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11970711B2 (en) | 2012-05-25 | 2024-04-30 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10407697B2 (en) | 2012-05-25 | 2019-09-10 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10415061B2 (en) | 2012-05-25 | 2019-09-17 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10421980B2 (en) | 2012-05-25 | 2019-09-24 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10428352B2 (en) | 2012-05-25 | 2019-10-01 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11332761B2 (en) | 2012-05-25 | 2022-05-17 | The Regenis of Wie University of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10443076B2 (en) | 2012-05-25 | 2019-10-15 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10487341B2 (en) | 2012-05-25 | 2019-11-26 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10513712B2 (en) | 2012-05-25 | 2019-12-24 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10519467B2 (en) | 2012-05-25 | 2019-12-31 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10526619B2 (en) | 2012-05-25 | 2020-01-07 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10533190B2 (en) | 2012-05-25 | 2020-01-14 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10550407B2 (en) | 2012-05-25 | 2020-02-04 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10563227B2 (en) | 2012-05-25 | 2020-02-18 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10570419B2 (en) | 2012-05-25 | 2020-02-25 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10577631B2 (en) | 2012-05-25 | 2020-03-03 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10597680B2 (en) | 2012-05-25 | 2020-03-24 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10612045B2 (en) | 2012-05-25 | 2020-04-07 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10626419B2 (en) | 2012-05-25 | 2020-04-21 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11401532B2 (en) | 2012-05-25 | 2022-08-02 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11242543B2 (en) | 2012-05-25 | 2022-02-08 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10669560B2 (en) | 2012-05-25 | 2020-06-02 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10676759B2 (en) | 2012-05-25 | 2020-06-09 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11473108B2 (en) | 2012-05-25 | 2022-10-18 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11479794B2 (en) | 2012-05-25 | 2022-10-25 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10752920B2 (en) | 2012-05-25 | 2020-08-25 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10774344B1 (en) | 2012-05-25 | 2020-09-15 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10793878B1 (en) | 2012-05-25 | 2020-10-06 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10113167B2 (en) | 2012-05-25 | 2018-10-30 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11549127B2 (en) | 2012-05-25 | 2023-01-10 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10900054B2 (en) | 2012-05-25 | 2021-01-26 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11814645B2 (en) | 2012-05-25 | 2023-11-14 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10982231B2 (en) | 2012-05-25 | 2021-04-20 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10982230B2 (en) | 2012-05-25 | 2021-04-20 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10988780B2 (en) | 2012-05-25 | 2021-04-27 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10988782B2 (en) | 2012-05-25 | 2021-04-27 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10000772B2 (en) | 2012-05-25 | 2018-06-19 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11674159B2 (en) | 2012-05-25 | 2023-06-13 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11634730B2 (en) | 2012-05-25 | 2023-04-25 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11008590B2 (en) | 2012-05-25 | 2021-05-18 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11028412B2 (en) | 2012-05-25 | 2021-06-08 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US11008589B2 (en) | 2012-05-25 | 2021-05-18 | The Regents Of The University Of California | Methods and compositions for RNA-directed target DNA modification and for RNA-directed modulation of transcription |
US10851380B2 (en) | 2012-10-23 | 2020-12-01 | Toolgen Incorporated | Methods for cleaving a target DNA using a guide RNA specific for the target DNA and Cas protein-encoding nucleic acid or Cas protein |
US10745716B2 (en) | 2012-12-06 | 2020-08-18 | Sigma-Aldrich Co. Llc | CRISPR-based genome modification and regulation |
US10731181B2 (en) | 2012-12-06 | 2020-08-04 | Sigma, Aldrich Co. LLC | CRISPR-based genome modification and regulation |
US10640788B2 (en) | 2013-11-07 | 2020-05-05 | Editas Medicine, Inc. | CRISPR-related methods and compositions with governing gRNAs |
US11390887B2 (en) | 2013-11-07 | 2022-07-19 | Editas Medicine, Inc. | CRISPR-related methods and compositions with governing gRNAS |
US10190137B2 (en) | 2013-11-07 | 2019-01-29 | Editas Medicine, Inc. | CRISPR-related methods and compositions with governing gRNAS |
US11680268B2 (en) | 2014-11-07 | 2023-06-20 | Editas Medicine, Inc. | Methods for improving CRISPR/Cas-mediated genome-editing |
US9888673B2 (en) | 2014-12-10 | 2018-02-13 | Regents Of The University Of Minnesota | Genetically modified cells, tissues, and organs for treating disease |
US10278372B2 (en) | 2014-12-10 | 2019-05-07 | Regents Of The University Of Minnesota | Genetically modified cells, tissues, and organs for treating disease |
US10993419B2 (en) | 2014-12-10 | 2021-05-04 | Regents Of The University Of Minnesota | Genetically modified cells, tissues, and organs for treating disease |
US11234418B2 (en) | 2014-12-10 | 2022-02-01 | Regents Of The University Of Minnesota | Genetically modified cells, tissues, and organs for treating disease |
US11390884B2 (en) | 2015-05-11 | 2022-07-19 | Editas Medicine, Inc. | Optimized CRISPR/cas9 systems and methods for gene editing in stem cells |
US11911415B2 (en) | 2015-06-09 | 2024-02-27 | Editas Medicine, Inc. | CRISPR/Cas-related methods and compositions for improving transplantation |
US11414657B2 (en) | 2015-06-29 | 2022-08-16 | Ionis Pharmaceuticals, Inc. | Modified CRISPR RNA and modified single CRISPR RNA and uses thereof |
US11642375B2 (en) | 2015-07-31 | 2023-05-09 | Intima Bioscience, Inc. | Intracellular genomic transplant and methods of therapy |
US10166255B2 (en) | 2015-07-31 | 2019-01-01 | Regents Of The University Of Minnesota | Intracellular genomic transplant and methods of therapy |
US11147837B2 (en) | 2015-07-31 | 2021-10-19 | Regents Of The University Of Minnesota | Modified cells and methods of therapy |
US11903966B2 (en) | 2015-07-31 | 2024-02-20 | Regents Of The University Of Minnesota | Intracellular genomic transplant and methods of therapy |
US11642374B2 (en) | 2015-07-31 | 2023-05-09 | Intima Bioscience, Inc. | Intracellular genomic transplant and methods of therapy |
US11583556B2 (en) | 2015-07-31 | 2023-02-21 | Regents Of The University Of Minnesota | Modified cells and methods of therapy |
US11266692B2 (en) | 2015-07-31 | 2022-03-08 | Regents Of The University Of Minnesota | Intracellular genomic transplant and methods of therapy |
US11925664B2 (en) | 2015-07-31 | 2024-03-12 | Intima Bioscience, Inc. | Intracellular genomic transplant and methods of therapy |
US10406177B2 (en) | 2015-07-31 | 2019-09-10 | Regents Of The University Of Minnesota | Modified cells and methods of therapy |
US11667911B2 (en) | 2015-09-24 | 2023-06-06 | Editas Medicine, Inc. | Use of exonucleases to improve CRISPR/CAS-mediated genome editing |
US11597924B2 (en) | 2016-03-25 | 2023-03-07 | Editas Medicine, Inc. | Genome editing systems comprising repair-modulating enzyme molecules and methods of their use |
US12049651B2 (en) | 2016-04-13 | 2024-07-30 | Editas Medicine, Inc. | Cas9 fusion molecules, gene editing systems, and methods of use thereof |
US11236313B2 (en) | 2016-04-13 | 2022-02-01 | Editas Medicine, Inc. | Cas9 fusion molecules, gene editing systems, and methods of use thereof |
US11078481B1 (en) | 2016-08-03 | 2021-08-03 | KSQ Therapeutics, Inc. | Methods for screening for cancer targets |
US11912987B2 (en) | 2016-08-03 | 2024-02-27 | KSQ Therapeutics, Inc. | Methods for screening for cancer targets |
US11946163B2 (en) | 2016-09-02 | 2024-04-02 | KSQ Therapeutics, Inc. | Methods for measuring and improving CRISPR reagent function |
US11078483B1 (en) | 2016-09-02 | 2021-08-03 | KSQ Therapeutics, Inc. | Methods for measuring and improving CRISPR reagent function |
US11154574B2 (en) | 2016-10-18 | 2021-10-26 | Regents Of The University Of Minnesota | Tumor infiltrating lymphocytes and methods of therapy |
US10912797B2 (en) | 2016-10-18 | 2021-02-09 | Intima Bioscience, Inc. | Tumor infiltrating lymphocytes and methods of therapy |
US12110545B2 (en) | 2017-01-06 | 2024-10-08 | Editas Medicine, Inc. | Methods of assessing nuclease cleavage |
US11499151B2 (en) | 2017-04-28 | 2022-11-15 | Editas Medicine, Inc. | Methods and systems for analyzing guide RNA molecules |
US11371030B2 (en) | 2017-05-31 | 2022-06-28 | The University Of Tokyo | Modified Cas9 protein and use thereof |
US11702645B2 (en) | 2017-05-31 | 2023-07-18 | The University Of Tokyo | Polynucleotide encoding modified CAS9 protein |
EP3878961A1 (en) | 2017-06-06 | 2021-09-15 | Zymergen, Inc. | A htp genomic engineering platform for improving escherichia coli |
WO2018226880A1 (en) | 2017-06-06 | 2018-12-13 | Zymergen Inc. | A htp genomic engineering platform for improving escherichia coli |
WO2018226900A2 (en) | 2017-06-06 | 2018-12-13 | Zymergen Inc. | A htp genomic engineering platform for improving fungal strains |
US11098297B2 (en) | 2017-06-09 | 2021-08-24 | Editas Medicine, Inc. | Engineered Cas9 nucleases |
US10428319B2 (en) | 2017-06-09 | 2019-10-01 | Editas Medicine, Inc. | Engineered Cas9 nucleases |
US11098325B2 (en) | 2017-06-30 | 2021-08-24 | Intima Bioscience, Inc. | Adeno-associated viral vectors for gene therapy |
US11866726B2 (en) | 2017-07-14 | 2024-01-09 | Editas Medicine, Inc. | Systems and methods for targeted integration and genome editing and detection thereof using integrated priming sites |
US11530396B2 (en) | 2017-09-05 | 2022-12-20 | The University Of Tokyo | Modified CAS9 protein, and use thereof |
US11066663B2 (en) | 2018-10-31 | 2021-07-20 | Zymergen Inc. | Multiplexed deterministic assembly of DNA libraries |
US11053515B2 (en) | 2019-03-08 | 2021-07-06 | Zymergen Inc. | Pooled genome editing in microbes |
US11053506B2 (en) | 2019-03-08 | 2021-07-06 | Zymergen Inc. | Iterative genome editing in microbes |
US11279940B2 (en) | 2019-03-08 | 2022-03-22 | Zymergen Inc. | Iterative genome editing in microbes |
Also Published As
Similar Documents
Publication | Publication Date | Title |
---|---|---|
US20230123754A1 (en) | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX | |
WO2013141680A1 (en) | RNA-DIRECTED DNA CLEAVAGE BY THE Cas9-crRNA COMPLEX | |
US20230132569A1 (en) | DNase H Activity of Neisseria Meningitidis Cas9 | |
AU2016319110B2 (en) | Full interrogation of nuclease DSBs and sequencing (FIND-seq) | |
IL288263B (en) | Crispr hybrid dna/rna polynucleotides and methods of use | |
Johnson et al. | Plasmid RK2 ParB protein: purification and nuclease properties | |
US20050084938A1 (en) | Method for plasmid preparation by conversion of open circular plasmid to supercoiled plasmid | |
JP7125727B1 (en) | Compositions for modifying nucleic acid sequences and methods for modifying target sites in nucleic acid sequences | |
US20220380738A1 (en) | Programmable Cleavage of Double-Stranded DNA | |
JP4143070B2 (en) | NOVEL ENZYME, METHOD FOR PRODUCING THE SAME AND METHOD FOR PRODUCING MOLECULAR WEIGHT ADJUSTED DOUBLE-STRAIN DNA USING THE SAME | |
Gasiūnas | DNA interference mechanism in Type II CRISPR/Cas systems |
Legal Events
Date | Code | Title | Description |
---|---|---|---|
AS | Assignment |
Owner name: VILNIUS UNIVERSITY, LITHUANIA Free format text: ASSIGNMENT OF ASSIGNORS INTEREST;ASSIGNORS:SIKSNYS, VIRGINIJUS;GASIUNAS, GIEDRIUS;KARVELIS, TAUTVYDAS;REEL/FRAME:035410/0733 Effective date: 20141219 |
|
STCB | Information on status: application discontinuation |
Free format text: ABANDONED -- FAILURE TO RESPOND TO AN OFFICE ACTION |