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. 2005 Oct 1;19(19):2301–2306. doi: 10.1101/gad.344205

RNA Pol II subunit Rpb7 promotes centromeric transcription and RNAi-directed chromatin silencing

Ingela Djupedal 1,4, Manuela Portoso 2,4, Henrik Spåhr 3, Carolina Bonilla 1, Claes M Gustafsson 3, Robin C Allshire 2, Karl Ekwall 1,5
PMCID: PMC1240039  PMID: 16204182

Abstract

Fission yeast centromeric repeats are transcribed into small interfering RNA (siRNA) precursors (pre-siRNAs), which are processed by Dicer to direct heterochromatin formation. Recently, Rpb1 and Rpb2 subunits of RNA polymerase II (RNA Pol II) were shown to mediate RNA interference (RNAi)-directed chromatin modification but did not affect pre-siRNA levels. Here we show that another Pol II subunit, Rpb7 has a specific role in pre-siRNA transcription. We define a centromeric pre-siRNA promoter from which initiation is exquisitely sensitive to the rpb7-G150D mutation. In contrast to other Pol II subunits, Rpb7 promotes pre-siRNA transcription required for RNAi-directed chromatin silencing.

Keywords: RNAi, heterochromatin, centromeres, RNA polymerase II, Rpb7


In RNA interference (RNAi), Dicer processes double-stranded RNA to produce short small interfering RNAs (siRNAs) that act to silence gene expression post-transcriptionally (Fire et al. 1998; Zamore et al. 2000; Bernstein et al. 2001). RNAi also mediates transcriptional silencing via formation of heterochromatin. Centromeres in many organisms are composed of repetitive DNAs, which act as a substrate for the formation of kinetochores, flanked by domains of centromeric heterochromatin (Cleveland et al. 2003). In fission yeast (Schizosaccharomyces pombe) genes inserted within this heterochromatin are transcriptionally silenced (Allshire et al. 1995). Paradoxically, the centromeric repeats themselves are transcribed to form long siRNA precursors (pre-siRNAs), which are required for the RNAi-mediated chromatin modifications resulting in transcriptional silencing (Provost et al. 2002; Volpe et al. 2002). Defective RNAi leads to loss of silencing and defective heterochromatin formation in several organisms (Mochizuki et al. 2002; Pal-Bhadra et al. 2002; Zilberman et al. 2003) and transcripts homologous to centromere repeats have been detected in chicken cells as well as mice (Fukagawa et al. 2004; Kanellopoulou et al. 2005). Interestingly, in plants, specialized RNA polymerase IV (RNA Pol IV) subunits have been implicated in RNAi-directed silencing (Herr et al. 2005; Onodera et al. 2005). Animal and fungal genomes lack such Pol IV subunits. Very recently, however, two subunits of RNA pol II (Rpb1 and Rpb2) were shown to have specific roles in chromatin modification and siRNA production, respectively, but did not affect pre-siRNA levels (Kato et al. 2005; Schramke et al. 2005).

Here, we have characterized the temperature sensitive csp3 (centromere: suppressor of position effect) mutant isolated in a screen for trans-acting mutants that are required for centromeric silencing (Ekwall et al. 1999). csp3 is a G150D missense mutation in the rpb7 gene, a subunit of Pol II. We show that Rpb7 has a specific defect in centromeric pre-siRNA transcription. We define a centromeric pre-siRNA promoter from which initiation is exquisitely sensitive to rpb7-G150D. Thus, in contrast to the previously characterized silencing defective Pol II subunits, which affect siRNA production and/or down-stream events, Rpb7 has a distinct role in generating centromeric pre-siRNAs needed for RNAi-directed chromatin silencing.

Results and Discussion

The csp3 gene was isolated by complementation of its temperature sensitivity. Complementing plasmids contained the rpb7 gene, and the corresponding open reading frame bears a missense mutation (rpb7-G150D) in csp3 mutant cells. The rpb7 gene was previously reported to encode an essential component of Pol II in S. pombe (Sakurai and Ishihama 1997; Mitsuzawa et al. 2003). The rpb7-G150D mutation lies within an RNA-binding motif (Fig. 1A). To biochemically characterize the rpb7-G150D mutation, we purified Pol II from wild-type and rpb7-G150D cells (Spahr et al. 2003). The subunit composition of wild-type and mutant Pol II was identical, as demonstrated by SDS-PAGE analysis, Coomassie Brilliant Blue staining, and protein identification by mass spectroscopy (Fig. 1B). Western blotting showed that Rpb7 remained associated with the rpb7-G150D mutant polymerase (Fig. 1C). The phenotype associated with the rpb7-G150D mutation was therefore not due to gross alterations in the Pol II subunit composition. We analyzed mutant Pol II isolated from the rpb7-G150D strain in a reconstituted in vitro system (Spahr et al. 2003). At the permissive temperature (23°C), basal transcription with mutant Pol II was functional, albeit reduced, as compared with wild type Pol II. At 36°C, however, the activity of the wild type Pol II was unaffected, whereas the activity of Pol II from the rpb7-G150D strain was almost completely abolished (Fig. 1D). Interestingly, Pol II from the rpb7-G150D strain had higher affinity for binding single-stranded RNA (ssRNA) than wild type Pol II at 23°C-25°C and 36°C (Supplementary Fig. S1). The basic biochemical properties of Pol II, however, seem to be unaffected in rpb7-G150D at 23°C-25°C.

Figure 1.

Figure 1.

Characterization of the rpb7-G150D mutation. (A) Alignment of the amino acid sequence of Rpb7 from Saccharomyces cerevisiae, S. pombe, and Homo sapiens. The arrows indicate secondary structure motifs discovered in the crystal structure of Rpb7 from archaebacterium Methanococcus jannaschii (Todone et al. 2001). The rpb7-G150D point mutation substitutes a glycine with an aspartic acid at position 150. (B) Purification of Pol II from wild-type and rpb7-G150D strains. Proteins were separated on a 10% gel (upper panel) and on a 10%-20% gel (lower panel) and revealed by Coomassie Brilliant Blue staining. Rpb7 (19.1 kDa), Rpb4 (15.3 kDa), and eight other subunits were present in both wild-type and rpb7-G150D preparations as confirmed by MALDI-TOF mass fingerprinting of the indicated bands. The asterisks (*) denote major protein contaminants not related to Pol II. (C) The presence of Rpb7 in both wild type and rpb7-G150D was confirmed with immunoblotting. (D) Transcription was reconstituted in vitro with a reporter construct containing the S. pombe adh1+ promoter followed by a G-less cassette as previously described (Spahr et al. 2003). Either wild-type Pol II or rpb7-G150D mutant were used at the permissive or restrictive temperature.

In order to assay the general effects on transcription of the rpb7-G150D mutation, cDNA expression profiling microarray analyses were performed (Xue et al. 2004). To compare the drastic reduction at the restrictive temperature (36°C) with 25°C, the data were normalized using luciferase RNA spiking controls. At 25°C, only 106 genes were more than twofold down-regulated in rpb7-G150D as compared with wild type, and expression of genes with known functions in centromeric silencing were not significantly altered (Supplementary Table S2). In contrast, only after 1 h at the growth restrictive temperature (36°C) a substantial part of the genome (>1803 genes) were down-regulated in rpb7-G150D as compared with wild type (Supplementary Fig. S2). Thus, the rpb7-G150D strain is generally defective for transcription at the restrictive temperature but displays a specific defect in centromeric silencing at 25°C.

Next, we tested whether rpb7-G150D had any defects in the RNAi pathway that directs heterochromatin formation and transcriptional silencing over the centromeric dg-dh repeats. RT-PCR was used to investigate silencing of a cen1R:ade6+ marker (Fig. 2A). At 25°C cen1R:ade6+ expression was undetectable in wild-type cells, but detectable in rpb7-G150D, dcr1Δ, and dcr1Δrpb7-G150D double-mutant cells. Dicer and RITS mutants show reduced dimethylation of histone H3 at Lys 9 (H3K9me2) and reduced binding of Swi6 and cohesin (Volpe et al. 2002, 2003; Verdel et al. 2004). We therefore tested if this was also defective in rpb7-G150D at the permissive temperature (25°C). Chromatin immunoprecipitation (ChIP) analyses with rpb7-G150D strains showed strongly reduced levels of H3K9me2, Swi6, and Rad21 cohesin associated with a ura4 marker gene inserted in the centromere repeats and at endogenous dg-dh sequences (Fig. 2B-D; Supplementary Table S4). Loss of centromeric cohesin causes a typical lagging chromosome defect in anaphase cells (Pidoux et al. 2000; Bernard et al. 2001). Dicer and RITS mutant cells show this phenotype (Provost et al. 2002; Hall et al. 2003; Volpe et al. 2003). We found that <0.1% of wild-type control and 16% of rpb7-G150D anaphase cells displayed lagging chromosomes at 25°C. Thus, rpb7-G150D cells show defects in transcriptional silencing, heterochromatin assembly at centromeres, and chromosome segregation.

Figure 2.

Figure 2.

Centromeric heterochromatin defects in rpb7-G150D and dcr1Δrpb7-G150D double-mutant cells. (A) RT-PCR analysis of centromeric silencing. Schematic representation of the ade6+ marker gene within centromeric dg-dh repeats and the truncated ade6N/N allele at the endogenous locus. Arrows, B11 and B12, mark the location of primers. RT-PCR analysis performed on total RNA from wild-type, dcr1Δ, dcr1Δrpb7-G150D double-mutant, and rpb7-G150D strains. Expression of the centromeric marker gene was undetectable in wild type, as compared with all three mutant strains where a distinct band was visible. Control reactions, without reverse transcriptase, were run to check for DNA contamination. (B-D, left panels) ChIP analysis of cen1R:ura4+ marker gene at the centromeric dg-dh repeat and the truncated ura4-DS/E allele at the endogenous locus. Competitive PCR was used in which one set of primers amplify two products: cen1R:ura4+ and ura4-DS/E. The relative fold enrichment was calculated by comparing the cen1R:ura4+ and ura4-DS/E ratio in DNA from the immunoprecipitated chromatin (IP) with input material (T). The ChIP method involves shearing of DNA that will cause shorter genes, such as ura4-DS/E, to give rise to stronger signals. (Right panels) ChIP analysis of dg-dh chromatin in wild type, rpb7-1, and swi6Δ at 25°C. Duplex PCR was used to amplify two products: dg and fbp1. The relative fold enrichment was calculated by comparing the dg and fbp1 ratio in DNA from the immunoprecipitated chromatin (IP) with input material (T). (B) ChIP with H3K9me2 antibodies at 25°C on wild type, rpb7-G150D, and clr4Δ.(C) ChIP with Rad21-HA antibodies at 25°C on wild type, rpb7-G150D, and swi6Δ. (D) ChIP with Swi6 antibodies at 25°C on wild type, rpb7-G150D, and swi6Δ. The numbers indicate the mean and standard deviations of three experiments.

siRNAs homologous to dg-dh repeats have been detected in wild-type cells (Reinhart and Bartel 2002) and transcripts from the reverse strand of dg-dh are produced (Volpe et al. 2002). These transcripts are rapidly processed in wild-type cells and their levels are very low but they accumulate to high levels in dcr1Δ cells. To determine if the production of forward and reverse strand transcripts from the dg-dh repeats is defective in rpb7-G150D cells, a dcr1Δrpb7-G150D double mutant was created, because such transcripts were expected to be undetectable in a Dicer context. The double mutant was similar to both dcr1Δ and rpb7-G150D regarding centromeric silencing defects (Fig. 2A). Accumulation of transcripts originating from centromeric repeats was assayed with strand specific RT-PCR, real-time PCR, and Northern analysis (Fig. 3B,C). Both reverse (real-time PCR; 276 times wild-type levels) and forward (596 times wild-type levels) dg-dh transcripts were readily detectable in dcr1Δ cells (Fig. 3B,C). In rpb7-G150D cells, forward dg-dh transcripts were increased (real-time PCR; 16 times wild-type levels) and reverse transcripts were found by real-time PCR to be 25% reduced as compared with wild-type cells. It is known that forward strand dg-dh transcripts are repressed by Swi6. Therefore, the increase of forward transcript levels in rpb7-G150D is likely to be a secondary effect, caused by the compromised heterochromatin, which allows more transcription. Importantly, transcript levels, particularly that of the reverse, remained low even in a dcr1Δrpb7-G150D double mutant at 25°C, whereas both transcripts accumulated to high levels in dcr1Δ (Fig. 3B,C). The fact that reverse transcript levels remained low in the dcr1Δrpb7-G150D double mutant indicated that Rpb7 functions upstream of Dcr1 in the RNAi pathway and may be required for the generation of centromeric pre-siRNAs. Recently, two other Pol II subunits, Rpb1 and Rpb2, were implicated in centromeric silencing (Kato et al. 2005; Schramke et al. 2005). Importantly dcr1Δrpb1-11 and dcr1Δrpb2-m203 mutants show no reduction of reverse dg-dh transcripts as compared with dcr1Δ controls.

Figure 3.

Figure 3.

Pol II transcribes centromeric siRNA precursors. (A) Schematic representation of the centromeric otr1 repeat region of centromere 1. Arrows shows the primer locations. (B) Strand-specific RT-PCR analysis of dg-dh repeat transcripts. RNA was harvested from cells grown at 25°C and after a 1-h shift to 36°C. Forward and reverse dg-dh transcripts were analysed, as indicated. Centromeric transcripts were not detected in wild-type cells. Actin serves as loading control. (C) Northern analysis of noncoding centromeric dg-dh transcripts. Centromeric transcripts were detected with a probe specific for the dg-dh repeat. The loading control was actin/rDNA (nonspecific hybridization). (D)3′-RACE mapping demonstrated that reverse dg-dh transcripts were polyadenylated. DNA from dg-dh repeat (1) aligned to 3′ end of 3′-RACE sequence. (E) TRO analysis of dg-dh transcripts at 25°C. rRNA sense (s) and antisense (as) probes were used as controls. The numbers indicate the rRNA sense normalized dg-dh RNA synthesis rate. Quantification is an average of two independent experiments.

3′-RACE mapping of centromeric dg-dh transcripts was performed and the resulting sequences were aligned with genomic DNA sequences revealing that the reverse transcripts are polyadenylated (Fig. 3D) supporting the idea that transcripts originating from centromeres indeed are transcribed by Pol II. We were also able to ChIP the dg-dh region in wild-type and rpb7-G150D cells with antibody against Pol II (Supplementary Fig. S1). Thus, Pol II is associated with dg-dh and Rpb7 is not required for Pol II recruitment to these centromere repeats.

To test if the altered dg-dh transcript levels in rpb7-G150D were due to changes in the rate of RNA synthesis, we carried out transcriptional run-on (TRO) analysis at 25°C of forward and reverse dg-dh transcripts using Pol I transcribed rRNA probes as controls (Fig. 3E). These analyses show a reproducible twofold reduction of reverse synthesis and a 1.5-fold increase in forward synthesis in rpb7-G150D versus wild type. This finding is consistent with RT-PCR/Northern data (Fig. 3B,C) and indicates that initiation or elongation rates of reverse dg-dh transcription are reduced in rpb7-G150D cells.

Previous studies have indicated a role for Rpb7 in initiation of transcription. Together with Rpb4, Rpb7 forms a dissociable substructure of Pol II (Choder 2004) and it was found that Pol II lacking Rpb4/7 was inactive in promoter-directed initiation of transcription whereas addition of Rpb4/7 restored activity (Edwards et al. 1991). To test if Rpb4 has a role together with Rpb7 in RNAi-directed centromeric functions, we expressed rpb4+ with a high copy expression vector (pREP3x-rpb4+) and, interestingly, we were able to partially suppress both the microtubule-poison (TBZ) sensitivity and cen1R:ade6 silencing defects of rpb7-G150D by overexpression of Rpb4 (Supplementary Fig. S3). This suggested that Rpb4 and Rpb7 share a special role at fission yeast centromeres.

Rpb7 has been previously shown to affect transcriptional initiation of some genes in budding yeast (Choder 2004). Rpb7 interacts strongly in protein-DNA photo-cross-linking experiments with promoter DNA (Chen et al. 2004). Therefore to test if transcriptional initiation was defective in rpb7-G150D cells, we first mapped the 5′ end of the dg-dh transcripts by 5′-RACE. The putative forward (For) and reverse (Rev) transcript promoters in the dg-dh region were then cloned into a lacZ reporter plasmid (Forsburg 1993). Truncated versions of the Rev promoter were also constructed (Fig. 4A). The plasmids were introduced into wild-type, rpb7-G150D, and rpb1-11 cells, and β-galactosidase assays were performed (Fig. 4B). Importantly, elongation, processing, and stability of the lacZ transcript were not affected since expression of β-galactosidase from the positive control nmt1-promoter-lacZ construct was not reduced in any of the mutants. It was clear from these data that the Rev promoter activity is strongly reduced at 25°C in rpb7-G150D but relatively unaffected in rpb1-11 as compared with wild type. In expression profiling microarray analysis rpb1-11 reduced transcription of 26 genes genome wide as compared with wild type (Schramke et al. 2005). Using the same microarray platform, normalizations, and cut-off value, we found that rpb7-G150D reduces expression of 51 genes as compared with wild type at 25°C (Supplementary Table S3). Therefore the two mutant Pol II enzymes are both only mildly compromised for transcription. Thus, the two mutant enzymes have a similar degree of genome-wide transcriptional defects, but only rpb7-G150D shows a defect in initiation of transcription from the Rev promoter.

Figure 4.

Figure 4.

Rpb7 is specifically required to promote initiation of centromere repeat transcription and siRNA production at 25°C. The transcription start site was revealed with 5′ RACE analysis of pre-siRNAs originating in the outer centromeric repeats of a dcr1Δ strain. (A) Centromeric dg-dh promoter fragments were cloned upstream of the lacZ reporter gene. RevL, RevM, and RevS are different truncated versions of the reverse (Rev) promoter starting at the carat () and ending at the transcription start site (green). The position of the putative TATA box is indicated in red. (B) Analysis of dg-dh promoter gene expression using forward (For) and reverse (Rev) lacZ fusions in wild-type, rpb7-G150D, and rpb1-11 cells. β-Galactosidase activity (Miller Units) was assayed in cells grown at 25°C. The nmt1 promoter (pREP41X-lacZ) was used as a positive control. The mean activity of five independent transformed colonies is shown as a percentage of wild type. The error bars represent the standard deviation. (C) Analysis of centromeric siRNA. (Top) Phosphorimages showing Northern blots of PEG precipitated small RNA extracted at 25°C from wild-type, rpb7-G150D, and dcr1Δ cells. The Northern blots were probed with a centromeric (dg-dh) probe. (Bottom) Gel image (loading) control representing the amount of PEG precipitated small RNA.

As a consequence of reducing siRNA precursor synthesis, centromeric siRNA levels are expected to be reduced in the rpb7-G150D strain compared with wild type. In order to test this, centromeric siRNA levels were probed by Northern analysis (Fig. 4C) and, although readily detected in wild-type cells, they were undetectable in rpb7-G150D and dcr1Δ cells.

Taken together, the data presented represents the first direct evidence that pre-siRNA's are transcribed by Pol II. Pol II has previously been reported to transcribe microRNAs (Lee et al. 2004). However, microRNAs, which work in post-transcriptional gene silencing, are very different from centromeric pre-siRNAs, which are transcribed from heterochromatin and act in transcriptional gene silencing. Furthermore, our data suggest that a particular subunit of Pol II, Rpb7, is required for initiation of centromeric siRNA precursor transcription and that this reverse dg-dh transcript is required to drive centromeric silencing. We speculate that the increased ssRNA-binding property of rpb7-G150D may inhibit initiation of transcription by stalling the transition from Pol II initiation to elongation complex. The effect is specific to rpb7-G150D, since two other fission yeast Pol II mutants do not have the same phenotype (Kato et al. 2005; Schramke et al. 2005). The CTD deleted mutant rpb1-11 has normal synthesis of pre-siRNAs, as well as siRNAs corresponding to centromeres (Schramke et al. 2005). A point mutation in the second largest Pol II subunit rpb2-m203 produces normal levels of pre-siRNAs but no centromeric siRNAs (Kato et al. 2005). Hence, both mutants are different than rpb7-G150D, which has reduced levels of pre-siRNA and no centromeric siRNAs. Thus, remarkably, the three different subunits Rpb7, Rpb2, and Rpb1 affect distinct steps of the same pathway (pre-siRNA synthesis, generation of siRNA, and chromatin modifications). This may reflect an adaption of the RNAi machinery to the multisubunit structure of RNA pol II, to coordinate different mechanistic steps of the RNAi-directed chromatin silencing pathway.

Materials and methods

Strains and media

Cells were grown in yeast extract supplemented with adenine (YES). Standard genetic techniques were used for crossing of strains. S. pombe strains used are listed in Supplementary Table S1.

Expression profiling DNA microarrays

Microarrays were purchased from Eurogentec and experiments were carried out as described (Xue et al. 2004). The microarray covers up to 99.5% of the annotated fission yeast genes. RNA was extracted from log phase cells using a standardized acid phenol method. cDNA was generated with a combination of S. pombe-specific primers and random hexamers and labeled with Cy3 and Cy5, respectively. Dye-swaps were done for all experiments. Hybridized slides were scanned using a Bio-Rad scanner and spots were quantified using ImageQuant version 4.2 (Imagene). The gene expression analysis was done with Genespring (Silicon Genetics). Normalization: To directly compare the rpb7-G150D 25°C and 36°C data sets, each gene's measured intensity was divided by the median of a list of positive control genes (luciferase spiking controls). To compare rpb7-G150D 25°C with rpb1-11 expresion profiles (Schramke et al. 2005) the Lowess normalization was used (Xue et al. 2004).

RT-PCR

Log phase cells were subjected to RNA extraction by standard acid phenol extraction or with RNeasy Mini kit for Preparation (QIAGEN). Before RT-PCR, all RNA samples were DNase treated (DNaseI, Invitrogen). Superscript first-strand synthesis system (Invitrogen) or OneStep RT-PCR Kit (QIAGEN) was used for RT-PCR. In strand-specific RT-PCR reactions only one primer, forward or reverse, was added to the RT reaction. Control reactions lacking RT were run for all RNA samples. Real-time PCR for cen forward, reverse and actin controls was carried out using a MyIQ (Bio-Rad) single-color apparatus.

ChIP

ChIP was performed as previously described except for the following modification: Cells were spheroplasted at 108 cells/mL in PEMS (100 mM Pipes at pH 7, 1 mM EDTA, 1 mM MgCl2, 1.2 M sorbitol) with 0.4 mg/mL Zymolyase-100T for 25 min at 36°C. Cells were washed twice in PEMS, and cell pellets were frozen at -20°C. Thereafter the standard ChIP procedure was followed. Quantitation of bands was performed using the Eastman Kodak Co. EDAS 290 system and 1D Image Analysis software.

Immunofluorescence microscopy

Cell growth, fixation in 3.8% paraformaldehyde, staining, detection of α-tubulin, collection of images, and spindle length measurements have been described (Mitsuzawa et al. 2003).

Northern blots

Ten micrograms of total RNA, prepared as described above, was resolved on 6.3% formaldehyde gels containing 1% agarose and blotted overnight to a Hybond-XL membrane (Amersham Biosciences). DNA probes, complementary to centromeric dg-dh repeats and actin, were generated with Random Primed DNA Labeling Kit (Roche). The probes were hybridized to the membranes overnight at 65°C in a rotating oven and washed according to the protocol provided by the manufacturer of the membrane.

3′- and 5′-RACE

3′- and 5′-RACE mapping of RNA transcripts from strain 978 was done according to protocol from the manufacturer, RACE System for Rapid Amplification of cDNA Ends version 2.0 (Invitrogen). Sequencing was done with ABI Prism BigDye Terminator Cycle Sequencing Ready Reactions Kits, Original and version 2.0 (AB Applied Biosystems).

TRO assay

TRO assays were carried out as described (Alen et al. 2002). Seven-hundred-nucleotide single-stranded MAXIscript probes for rRNA and dg-dh region were used.

Small RNA preparations and detection

Log phase cells were subjected to RNA extraction by standard acid phenol extraction followed by PEG precipitation. Samples were resuspended in 50% formamide and separated on a 17.5% Urea-denaturating polyacrylamide gel. A 32P-DNA probe, complementary to centromeric dg-dh repeats, was generated with Random Primed DNA Labeling Kit (Roche). The probe was hybridized to the membranes overnight at 42°C in a rotating oven and washed twice with 2× SSC 2% SDS at 50°C. Phosphorscreen or films were exposed for a minimum of 3 h up to 3 d. DNA Oligonucleotides 22 nucleotides (nt) in length were used as a marker.

RNA filter assay

Centromeric dg-dh repeats PCR-fragments were generated with T7 promoters at both ends. Radioactively labeled RNA was produced from these templates with the MAXIscript in vitro transcription Kit from Ambion. Pol II was purified from strains 303 and 801 and subjected to transcription assays as described previously (Spahr et al. 2003). Pol II binding to RNA was assayed by nitrocellulose filter binding in a 25 μL reaction volume. Proteins were incubated with in vitro transcribed RNA (40,000 counts per minute) in RNA-binding buffer (5 mM magnesium acetate, 2.5 mM magnesium sulfate, 3.7 mM EDTA, 37 mM Hepes-KOH at pH 7.6, 100 mM potassium acetate, 1.25 mM dithiothreitol, and RNase inhibitors) for 30 min at 36°C. The mix was transferred to a nitrocellulose membrane (Schleicher and Schuell, Protran 0.45 μM), washed twice with 1 mL RNA-binding buffer without RNase inhibitor, and measured in a liquid scintillation counter (Wallac 1410).

Purification of RNA Pol II

Purification of RNA Pol II was carried out according to Spahr et al. (2003). Western blotting with Rpb7-specific (Santa Cruz) and Rpb1-specific (Neoclone) antibodies was performed according to the manufacturers instructions.

β-Galactosidase activity assay

Cells containing the pREP-lacZ constructs (Fig. 4B) were grown in PMG medium lacking leucine and thiamine to mid-logarithmic phase at 25° C. Units were defined as equal to (1000 × OD414) × (min × mL × OD595)-1. The nmt1 promoter (pREP41X-lacZ) was used as a positive control (Forsburg 1993).

Acknowledgments

We thank Thomas Jenuwein for contributing with α-H3K9Me2 and Susan Forsburg for providing plasmids. K.E. is a Royal Swedish Academy of Sciences Research Fellow supported by a grant from the Knut and Alice Wallenberg Foundation. K.E is funded by Cancerfonden 4284-B02-04XBB and VR-M 31X-12562, VR-NT 621-2002-4311 grants. C.M.G. is funded by grants from Swedish Cancer Society and the Swedish Foundation for Strategic Research. R.C.A. is a Wellcome Trust Principal Research Fellow (065061), and M.P. is funded by a Wellcome Trust Prize Studentship (067844). R.C.A and K.E. are members of the EC FP6 Network “The Epigenome” LSHG-CT-2004-503433.

Supplemental material is available at http://www.genesdev.org.

Article and publication are at http://www.genesdev.org/cgi/doi/10.1101/gad.344205.

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