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USRE46130E1 - Method of selectively determining glycated hemoglobin - Google Patents

Method of selectively determining glycated hemoglobin Download PDF

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USRE46130E1
USRE46130E1 US14/329,019 US200114329019A USRE46130E US RE46130 E1 USRE46130 E1 US RE46130E1 US 200114329019 A US200114329019 A US 200114329019A US RE46130 E USRE46130 E US RE46130E
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glycated
whole blood
amino acid
glycated hemoglobin
protease
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Satoshi Yonehara
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Arkray Inc
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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING 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
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/26Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving oxidoreductase
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING 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
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/34Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving hydrolase
    • C12Q1/37Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving hydrolase involving peptidase or proteinase
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/72Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving blood pigments, e.g. haemoglobin, bilirubin or other porphyrins; involving occult blood
    • G01N33/721Haemoglobin
    • G01N33/723Glycosylated haemoglobin
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/72Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving blood pigments, e.g. haemoglobin, bilirubin or other porphyrins; involving occult blood
    • G01N33/721Haemoglobin
    • G01N33/725Haemoglobin using peroxidative activity

Definitions

  • the present invention relates to a method of determining an amount of glycated hemoglobin present in whole blood.
  • Glycated hemoglobin in blood has served as an important index for the diagnosis, treatment, etc. of diabetes because it reflects previous blood glucose levels in vivo.
  • the determination of such glycated hemoglobin has been carried out, for example, by high performance liquid chromatography (HPLC), a minicolumn method, immunoassays, and the like. According to these methods, the amount or ratio of hemoglobin that has been glycated can be determined.
  • HPLC high performance liquid chromatography
  • FOD fructosyl amino acid oxidoreductase
  • the above-mentioned method has a problem as follows. Because the glycated hemoglobin is a component contained in a blood cell, it is absolutely necessary to hemolyze the blood cell to carry out the determination of the glycated hemoglobin. In the case where a sample to be analyzed is whole blood, however, the treatment for causing hemolysis (hereinafter, referred to as “hemolysis treatment”) conducted on the whole blood brings about a state where blood cell components and plasma components are mixed with each other.
  • hemolysis treatment the treatment for causing hemolysis
  • the whole blood sample that has been subjected to the hemolysis treatment contains not only the glycated hemoglobin as a blood cell component but also albumin as a high-content plasma component and glycated albumin as a glycation product thereof, in particular.
  • the glycated albumin is determined together with the glycated hemoglobin because FAOD also acts on the glycated albumin.
  • a complicated process for separating the plasma and blood cells from the whole blood sample is required in order to eliminate the effect of other glycoproteins such as the glycated albumin and the like.
  • a method of determining an amount of glycated hemoglobin includes: degrading glycated hemoglobin in whole blood selectively with a protease to give a glycated hemoglobin degradation product; causing a redox reaction between a glycation site of the glycated hemoglobin degradation product and FAOD; and determining the redox reaction to determine an amount of the glycated hemoglobin.
  • the term “an amount of glycated hemoglobin” as used in the present invention also includes a ratio of glycated hemoglobin.
  • glycated hemoglobin is distinguished from other proteins and peptides and is degraded selectively (i.e., specifically) with a protease as described above, it becomes possible to determine an amount of the glycated hemoglobin while eliminating the effect of other glycoproteins, especially glycated albumin, without separating blood cells from the whole blood because FAOD hardly acts on proteins or long polypeptide chains.
  • a sample to be used in this method may be whole blood that has been subjected to a hemolysis treatment, for example.
  • a protease capable of degrading the glycated hemoglobin selectively in order to degrade glycated hemoglobin selectively, for example, may be used as the protease.
  • a method of degrading glycated hemoglobin selectively is not limited to the use of the protease capable of degrading the glycated hemoglobin selectively.
  • the glycated hemoglobin may be degraded selectively by any other means.
  • the protease capable of degrading glycated hemoglobin selectively may be used in combination with one or more of ordinary proteases.
  • the protease capable of degrading glycated hemoglobin selectively is at least one of bromelains, papains, trypsins derived from porcine pancreas, metalloproteinases, and proteases derived from Bacillus subtilis.
  • the proteases derived from Bacillus subtilis include Protease N (trade name, available from Sigma Aldrich Co.), Protease N “AMANO” (trade name, available from Amano Enzyme Inc.), and the like.
  • the metalloproteinases include a metalloproteinase derived from the genus Bacillus (EC 3. 4. 24. 4) (e.g., available from Toyobo Co., Ltd. under the trade name Toyoteam), and the like. Among these, the metalloproteinases, bromelains, and papains are more preferable, and the metalloproteinases are most preferable.
  • a substrate of the FAOD is at least one glycated amine selected from the group consisting of glycated proteins, glycated peptides, and glycated amino acids, and the FAOD acts on at least one of a glycated ⁇ -amino group and a glyeated side-chain amino group of the glycated amine to catalyze a reaction that causes generation of hydrogen peroxide.
  • the glycation site of the glycated hemoglobin degradation product to be reacted with the FAOD preferably is a glycated amino group in a side chain of an amino acid residue and a glycated ⁇ -amino group, for example, whereas the glycation site to be reacted with the FAOD varies depending on the catalytic reaction caused by the FAOD to be used.
  • the glycation site is the glycated amino group in a side chain of an amino acid residue because FAOD having a catalytic function as described later can act thereon more easily.
  • the glycated amino group include a glycated amino group in a side chain of a lysine residue, a glycated amino group in a side chain of an arginine residue, and the like.
  • the protease is added to the whole blood so that a content of the protease per milliliter of the whole blood is in a range from 1,000 to 10,000,000 U. Further, it is preferable that the FAOD is added to the whole blood so that a content of the FAOD per milliliter of the whole blood is in a range from 500 to 40,000 U.
  • determining the redox reaction is determining an amount of hydrogen peroxide generated by the redox reaction or an amount of oxygen consumed by the redox reaction.
  • the amount of the hydrogen peroxide is determined using a peroxidase (hereinafter, referred to as “POD”) and a substrate that develops color by oxidation.
  • POD peroxidase
  • the substrate that develops color by oxidization is not specifically limited and can be, for example, N-(carboxymethylaminocarbonyl)-4,4′-bis(dimethylamino)diphenylamine sodium, orthophenylenediamine (OPD), and a substrate obtained by combining a Trinder's reagent and 4-aminoantipyrine.
  • the Trinder's reagent include phenols, phenol derivatives, aniline derivatives, naphthols, naphthol derivatives, naphthylamine, naphthylamine derivatives, and the like.
  • aminoantipyrine derivatives vanillin diamine sulfonic acid, methyl benzothiazolinone hydrazone (MBTH), sulfonated methyl benzothiazolinone hydrazone (SMBTH), and the like.
  • MBTH methyl benzothiazolinone hydrazone
  • SMBTH sulfonated methyl benzothiazolinone hydrazone
  • N-(carboxymethylaminocarbonyl)-4,4′-bis (dimethylamino)diphenylamine sodium is most preferable.
  • a method of determining an amount of HbA1c according to the present invention includes: preparing a calibration curve based on a correlation between an amount of glycated hemoglobin determined by the method of determining an amount of glycated hemoglobin according to the present invention and an amount of HbA1c; and substituting the amount of glycated hemoglobin in a whole blood sample determined by the method into the calibration curve to determine an amount of HbA1c in the whole blood sample.
  • HbA 1 c is a glycated hemoglobin in which the N-terminal ⁇ -amino group in the ⁇ -chain of hemoglobin has been glycated.
  • HbA1c has served as a particularly important index for the diagnosis etc. of diabetes.
  • HbA1c As an important index for the diagnosis of diabetes can be determined accurately and easily so that the determination of HbA1c can be made practical in clinical tests etc.
  • the calibration curve is prepared based on a correlation between a known amount of HbA1c in a standard sample and an amount of glycated hemoglobin in the standard sample determined by the method of determining an amount of glycated hemoglobin according to the present invention.
  • a kit used for determining an amount of glycated hemoglobin according to the present invention includes a protease that distinguishes a glycated hemoglobin from other proteins and peptides to degrade the glycated hemoglobin selectively.
  • the protease is at least one protease selected from the group consisting of bromelains, papains, trypsins derived from porcine pancreas, metalloproteinases, and proteases derived from Bacillus subtilis. Further, it is preferable that the kit further includes FAOD.
  • a substrate of the FAOD is at least one glycated amine selected from the group consisting of glycated proteins, glycated peptides, and glycated amino acids, and the FAOD acts on at least one of a glycated ⁇ -amino group and a glycated side-chain amino group of the glycated amine to catalyze a reaction that causes generation of hydrogen peroxide.
  • the kit further includes POD and a substrate that develops color by oxidization.
  • the substrate that develops color by oxidization preferably is N-(carboxymethylaminocarbonyl)-4,4′-bis (dimethylamino)diphenylamine sodium.
  • a reagent used for determining an amount of glycated hemoglobin according to the present invention includes a protease that distinguishes a glycated hemoglobin from other proteins and peptides to degrade the glycated hemoglobin selectively.
  • the protease is at least one protease selected from the group consisting of bromelains, papains, trypsins derived from porcine pancreas, metalloproteinases, and proteases derived from Bacillus subtilis. Further, it is preferable that the reagent further includes FAOD.
  • a substrate of the FAOD is at least one glycated amine selected from the group consisting of glycated proteins, glycated peptides, and glycated amino acids, and the FAOD acts on at least one of a glycated ⁇ -amino group and a glycated side-chain amino group of the glycated amine to catalyze a reaction that causes generation of hydrogen peroxide.
  • the reagent further includes POD and a substrate that develops color by oxidization.
  • the substrate that develops color by oxidization preferably is N-(carboxymethylaminocarbonyl)-4,4′-bis (dimethylamino)diphenylamine sodium.
  • FIG. 1 is a graph showing the correlation between an HbA1c concentration and an absorbance in a method of determining an amount of glycated hemoglobin according to one example of the present invention.
  • FIG. 2 is a graph showing the correlation between HbA1c (%) determined using a calibration curve and HbA1c (%) measured using an automatic measuring apparatus in a method of determining an amount of glycated hemoglobin according to another example of the present invention.
  • FAOD capable of catalyzing a reaction represented by Formula (1) below preferably is used.
  • R 1 —CO—CH 2 —NH—R 2 denotes a glycated protein, glycated peptide, and glycated amino acid, for example.
  • R 1 denotes a hydroxyl group or a residue derided from a sugar that is not yet subjected to the glycation reaction (i.e., sugar moiety).
  • the sugar moiety (R 1 ) is an aldose residue when the unreacted sugar is aldose, and is a ketose residue when the unreacted sugar is ketose.
  • the unreacted sugar is glucose, for example, the sugar in the glycated product takes on the fructose structure after the glycation reaction due to Amadori rearrangement.
  • the sugar moiety (R 1 ) is a glucose residue (aldose residue).
  • This sugar moiety (R 1 ) can be represented, for example, by —[CH(OH)] n —CH 2 OH where n denotes an integer of 0 to 6.
  • R 2 is not specifically limited. However, it is to be noted that R 2 varies depending on which of an ⁇ -amino group and an amino group other than the ⁇ -amino group is glycated.
  • R 2 is an amino acid residue or a peptide residue represented by Formula (2) below. —CHR 3 —CO—R 4 (2)
  • R 3 denotes an amino-acid side chain group.
  • R 4 denotes a hydroxyl group, an amino acid residue, or a peptide residue, and can be represented, for example, by Formula (3) below.
  • n denotes an integer of 0 or more, and R 3 denotes an amino-acid side chain group as described above. —(NH—CR 3 H—CO) n —OH (3)
  • R 2 is represented by Formula (4) below. —R 5 —CH(NH—R 6 )—CO—R 7
  • R 5 denotes a portion other than the glycated amino group in the amino-acid side chain group.
  • R 5 is as follows. —CH 2 —CH 2 —CH 2 —CH 2 —CH 2 —
  • R 5 is as follows. —CH 2 —CH 2 —CH 2 —NH—CH(NH 2 )—
  • R 6 denotes hydrogen, an amino acid residue, or a peptide residue, and can be represented, for example, by Formula (5) below.
  • n denotes an integer of 0 or more
  • R 3 denotes an amino-acid side chain group as described above. —(CO—CR 3 H—NH) n —H (5)
  • R 7 denotes a hydroxyl group, an amino acid residue, or a peptide residue, and can be represented, for example, by Formula (6) below.
  • n denotes an integer of 0 or more
  • R 3 denotes an amino-acid side chain group as described above. —(NH—CHR 3 —CO) n —OH (6)
  • a catalytic reaction caused by FAOD to be used in the method of the present invention is not specifically limited as long as it is a reaction represented by Formula (1).
  • the FAOD acts on the glycation site in which a sugar is bound to an amino group other than an ⁇ -amino group (i.e., R 2 has a structure as represented by Formula (4)).
  • the catalytic function of the FAOD is not limited to such function.
  • the FAOD further may have a catalytic function to act on the glycation site in which a sugar is bound to an ⁇ -amino group (i.e., R 2 has a structure as represented by Formula (2)).
  • FAOD examples include those derived from the genus Fusarium, the genus Gibberella, and the genus Aspergillus. More specifically, commercially available FAODs such as Fructosyl Amino Acid Oxidase (trade name, available from Asahi Chemical Industry Co., Ltd.), Ketoamine Oxidase (trade name, available from Genzyme Corporation), and the like can be used, for example.
  • the whole blood is hemolyzed.
  • the method of hemolyzing the whole blood is not specifically limited, and can be, for example, a method using a surfactant, a method using ultrasonic waves, and a method utilizing the difference in osmotic pressure.
  • the method using a surfactant is preferable on account of the ease of operation.
  • nonionic surfactants such as polyoxyethylene-p-t-octylphenyl ether (Triton-type surfactant etc.), polyoxyethylene sorbitan alkyl ester (Tween-type surfactant etc.), polyoxyethylene alkyl ether (Brij-type surfactant etc.), and the like can be used, for example. More specifically, Triton X-100 (trade name), Tween-20 (trade name), Brij 35 (trade name), and the like can be used, for example.
  • the treatment with the above surfactant can be carried out under the following conditions: in the case where the solution to be treated contains 1 to 10 vol % of blood cells, the surfactant is added to the solution so as to give a concentration of 0.1 to 1 wt % and the resultant mixture is stirred at room temperature for about 5 seconds to 1 minute.
  • the above-mentioned hemolysate sample is treated with the above-mentioned protease, thereby selectively degrading glycated hemoglobin in the sample.
  • this protease treatment is carried out in a buffer.
  • the treatment conditions are decided as appropriate, for example, depending on the type of the protease to be used, the amount of the glycated hemoglobin, and the like.
  • the treatment generally is carried out under the following conditions: the protease concentration in the reaction solution in the range from 100 to 30,000 U/L, the hemoglobin concentration in the reaction solution in the range from 0.1 to 40 g/L, the reaction temperature in the range from 15° C. to 60° C., the reaction time in the range from 10 minutes to 40 hours, and the pH in the range from 5 to 9.
  • the type of the buffer is not specifically limited, and can be, for example, Tris-HCl buffer, EPPS buffer, PIPES buffer, phosphate buffer, ADA buffer, citrate buffer, acetate buffer, and the like.
  • the treatment is carried out, for example, under the following conditions: the protease concentration in the reaction solution in the range from 10 to 10,000 KU/L, the hemoglobin concentration in the reaction solution in the range from 0.02 to 40 g/L, the reaction temperature in the range from 15° C. to 60° C., the reaction time in the range from 2 minutes to 40 hours, and the pH in the range from 6 to 11; preferably, the protease concentration in the reaction solution in the range from 100 to 8,000 KU/L, the hemoglobin concentration in the reaction solution in the range from 0.1 to 10 g/L, the reaction temperature in the range from 15° C. to 60° C., the reaction time in the range from 2 minutes to 1 hour, and the pH in the range from 7 to 10.
  • the buffer the above-mentioned various buffers also can be used. Further, other proteinases also can be used.
  • the glycated hemoglobin degradation product obtained through the above-mentioned protease treatment is treated with FAOD.
  • This FAOD treatment catalyzes the reaction represented by Formula (1) above. More specifically, FAOD acts on a glycated amino group in a side chain of a lysine residue and a side chain of an arginine residue in the glycated hemoglobin degradation product, for example. Further, depending on the type of the FAOD to be used, the FAOD further may act on a glycated ⁇ -amino group according to its catalytic function.
  • this FAOD treatment preferably is carried out in a buffer.
  • the buffer is not specifically limited, and the same buffers as used in the protease treatment also can be used in the FAOD treatment.
  • the FAOD treatment is carried out, for example, under the following conditions: the FAOD concentration in the reaction solution in the range from 200 to 30,000 U/L, the hemoglobin concentration in the reaction solution in the range from 0.02 to 30 g/L, the reaction temperature in the range from 15° C. to 37° C., the reaction time in the range from 1 to 20 minutes, and the pH in the range from 7 to 9; preferably, the FAOD concentration in the range from 1,000 to 20,000 U/L, the hemoglobin concentration in the reaction solution in the range from 0.1 to 5 g/L, the reaction temperature in the range from 15° C. to 37° C., the reaction time in the range from 1 to 5 minutes, and the pH in the range from 7 to 9.
  • the amount of the hydrogen peroxide generated by the FAOD treatment is determined utilizing a redox reaction, by using the POD and a substrate that develops color by oxidization.
  • the redox reaction caused by the POD generally is induced in a buffer under the conditions decided as appropriate, for example, depending on the concentration of the hydrogen peroxide and the like.
  • the redox reaction is induced under the following conditions: the POD concentration in the reaction solution in the range from 1 to 100,000 IU/L, the substrate concentration in the range from 0.0001 to 1 mmol/L, the reaction temperature in the range from 20° C. to 37° C., the reaction time in the range from 1 to 5 minutes, and the pH in the range from 6 to 9; preferably, the POD concentration in the reaction solution in the range from 1,000 to 50,000 IU/L, the substrate concentration in the range from 0.0002 to 0.1 mmol/L, the reaction temperature in the range from 20° C. to 37° C., the reaction time in the range from 1 to 5 minutes, and the pH in the range from 6 to 9.
  • the buffer is not specifically limited, and the same buffers as used in the FAOD treatment also can be used.
  • the amount of the hydrogen peroxide can be determined not only by the above-mentioned enzymic method using the POD etc. but also by an electrical method, for example.
  • the concentration of the hydrogen peroxide can be determined by measuring the color development (i.e., the absorbance of the reaction solution) with a spectrophotometer. From the concentration of the hydrogen peroxide, the concentration of the glycated hemoglobin in the sample can be determined.
  • the respective treatment steps may be performed individually as described above, or some of the treatment steps may be performed simultaneously in the following combinations, for example.
  • the order in which the FAOD, the POD, and the substrate are added is not specifically limited.
  • an amount of glycated hemoglobin in a whole blood sample is determined in the above-mentioned manner.
  • a glycated hemoglobin standard solution in which an amount of HbA1c in glycated hemoglobin is known is provided.
  • an amount of glycated hemoglobin in this standard solution is determined in the above-mentioned manner.
  • a calibration curve is prepared that shows the relation between the amount of glycated hemoglobin thus determined and the known amount of HbA1c in this standard solution.
  • an amount of HbA1c in the whole blood sample can be determined by substituting the amount of glycated hemoglobin in the whole blood sample determined by the method of the present invention into this calibration curve.
  • the determined amount of glycated hemoglobin is not limited to the value finally obtained though the method of the invention, and can be an absorbance of the reaction solution obtained by the POD treatment during the determination process, or an amount of hydrogen peroxide determined based on this absorbance.
  • an amount of HbA1c in whole blood can be determined accurately and easily based on an amount of glycated hemoglobin determined by utilizing the correlation discovered by the inventors of the present invention.
  • Samples containing glycated hemoglobin and glycated albumin were treated with a papain. Then, a redox reaction thereof was caused by FAOD, and the amount of hydrogen peroxide generated was determined.
  • the samples, reagents, and method used in the determination will be described in the following.
  • the above human hemoglobin sample was prepared in the following manner, and the glycation ratio thereof was determined by HPLC using an ion exchange column.
  • Whole blood was collected from a healthy subject using a blood-collecting vessel containing heparin sodium.
  • the whole blood was diluted 8-fold with purified water to hemolyze the blood cells contained therein.
  • the resultant solution was used as whole blood samples.
  • the blood cells obtained though the above-mentioned centrifugation were diluted 16-fold with purified water to cause hemolysis.
  • the resultant solution was used as blood cell samples.
  • a bromelain, papain (available from Hoffmann-La Roche Inc.), elastase (available from Wako Pure Chemical Industries, Ltd.), ⁇ -chymotrypsin (available from Wako Pure Chemical Industries, Ltd.), and proteinase K (available from Wako Pure Chemical Industries, Ltd.) were dissolved in purified water, respectively, to prepare 4g/L solutions of the respective proteases.
  • composition of Redox Solution B POD 20 KU/L DA 64 (trade name) 0.04 mmol/L Potassium phosphate buffer (pH 7.0) 0.1 mol/L
  • Composition of Redox Solution C FAOD 14.3 KU/L Potassium phosphate buffer (pH 7.0) 0.1 mol/L (Determining Method)
  • Example 3 substantially no absorption was observed in the plasma samples.
  • the proteases used in Example 3 can degrade glycated hemoglobin selectively and hardly degrade glycated albumin etc. derived from plasma, for example.
  • Comparative Example 2 absorption was observed in the plasma samples even though the plasma samples contained no glycated hemoglobin. The reason for this is considered to be that, because the proteases used in Comparative Example 2 degrade glycated proteins without distinguishing glycated hemoglobin from other glycated proteins, glycated albumin and the like also are degraded in the plasma samples, for example, thereby allowing the absorption to be observed in the plasma samples.
  • HbA1c standard reagents (available from SRL, Inc.) were dissolved in purified water to prepare glycated hemoglobin standard solutions containing HbA1c at concentrations 4.3%, 7.8%, 11.2%, and 14.7%, respectively, while containing 10 g/L hemoglobin. Further, HbA1c standard reagents (available from International Regents Corporation) were dissolved in purified water to prepare glycated hemoglobin standard solutions containing HbA1c at concentrations 5.5% and 10.8%, respectively, while containing 10 g/L hemoglobin.
  • a 2 g/L solution of a bromelain F (available from Amano Enzyme Inc.) and a 1 g/L solution of a papain (available from Hoffmann-La Roche Inc.) were prepared by dissolving the respective proteases in purified water.
  • FIG. 1 is a graph showing the correlation between an HbA1c concentration and an absorbance in the glycated hemoglobin standard solution.
  • Hemolysate samples were treated with a metalloproteinase, a papain, and a protease derived from Bacillus subtilis, and the amounts of glycated hemoglobin in the respective samples were determined according to the method of the present invention. Further, the amounts of HbA1c in the respective samples were determined based on the amounts of glycated hemoglobin thus determined.
  • the samples, reagents, and method used in the determination will be described in the following.
  • HbA1c standard reagents (available from International Regents Corporation) were dissolved in 0.05 wt % Triron X-100 aqueous solutions to prepare glycated hemoglobin standard solutions containing HbA1c at concentrations 5.5% and 10.5%, respectively, while containing 200 g/L hemoglobin.
  • a metalloproteinase (available from Toyobo Co., Ltd.), Protease N “AMANO” (trade name, available from Amano Enzyme Inc.), and a papain (available from Hoffmann-La Roche Inc.) were dissolved in purified water to prepare 1 g/L solutions of the respective proteases.
  • composition of Redox Solution D POD 20 KU/L DA-64 (trade name) 0.04 mmol/L Phosphate buffer (pH 8.0) 0.8 mol/L
  • Composition of Redox Solution E FAOD 14.3 KU/L Potassium phosphate buffer (pH 8.0) 0.1 mmol/L (Method of Determining Amount of glycated hemoglobin)
  • the absorbance of the respective reaction solutions was measured at the main wavelength of 751 nm and the sub-wavelength of 884 nm. The absorbance thus measured corresponds to the amount of glycated hemoglobin.
  • Hemoglobin concentrations in the respective samples were determined according to the cyanmethemoglobin method using Hemoglobin Test Wako (trade name, available from Wako Pure Chemical Industries, Ltd.).
  • HbA1c concentrations (%) of the above-mentioned respective standard solutions were measured using an automatic measuring apparatus (the trade name HA-8150: available from ARKRAY, INC.).
  • the absorbances corresponding to the amounts of glycated hemoglobin were measured by the method of determining an amount of glycated hemoglobin according to the present invention and hemoglobin concentrations were determined by the above-mentioned method of determining a hemoglobin concentration.
  • the absorbances corresponding to the amounts of glycated hemoglobin were measured by the above-mentioned method of determining the amount of glycated hemoglobin, and hemoglobin concentrations were determined by the above-mentioned method of determining a hemoglobin concentration. Then, the percentages obtained by dividing the absorbances corresponding to the amounts of glycated hemoglobin by the hemoglobin concentrations were regarded as the ratios of the glycated hemoglobin, and the amounts of HbA1c in the respective hemolysate samples were determined by substituting the thus-obtained ratios into the above-mentioned respective calibration curves.
  • FIG. 2 is a graph showing the correlations between the amounts of HbA1c determined using the calibration curves according to the method of the present invention and the amounts of HbA1c measured using the automatic measuring apparatus.
  • Hemolysate samples to which plasma samples have been added were treated with a metalloproteinase. Amounts of glycated hemoglobin in the respective samples were determined to examine the change in the amounts of glycated hemoglobin caused by the addition of the plasma samples.
  • Whole blood collected from a healthy subject (1 subject) and diabetic subjects was centrifuged (1000 G, about 15 min), and blood cell fractions and plasma fractions of the respective subjects were collected. Thereafter, predetermined amounts (0 mL, 0.005 mL, 0.010 mL, 0.015 mL, and 0.020 mL) of the plasma fractions of the respective subjects were added to 0.01 mL of the blood cell fractions of the corresponding subjects. Then, to the respective mixtures was added 0.3 mL of the following hemolysis reagent. The resultant solutions were used as hemolysate samples.
  • a ratio of glycated hemoglobin in a whole blood sample can be determined easily and accurately without separating plasma and blood cells in the whole blood sample. Further, since there is a strong correlation between an amount of glycated hemoglobin determined by the method of the present invention and an amount of HbA1c, by preparing a calibration curve based on this correlation in advance, it becomes possible to determine an amount of HbA1c in a whole blood sample accurately and easily by merely determining the amount of glycated hemoglobin in the whole blood sample.

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Abstract

A method of determining glycated hemoglobin is provided, by which a ratio of the glycated hemoglobin in a sample can be determined accurately and easily. The ratio of glycated hemoglobin can be determined by degrading a glycated hemoglobin in a whole blood sample selectively with a protease to give a glycated hemoglobin degradation product; causing a redox reaction between a glycation site of the glycated hemoglobin degradation product and a fructosyl amino acid oxidoreductase; and determining this redox reaction. Further, as shown in FIG. 1, in a whole blood sample, there is a correlation between the ratio of the glycated hemoglobin determined by this method and an HbA1c concentration. Thus, without determining the glycated α-amino group as a characteristic structure of HbA1c, an amount of HbA1c can be determined accurately and easily from the determined ratio of the glycated hemoglobin.

Description

Notice: More than one reissue application has been filed for the reissue of U.S. Pat. No. 7,235,378. The reissue applications are application Ser. Nos. 14/329,019 (the present application) filed Jul. 11, 2014; 14/521,525 filed Oct. 23, 2014; 14/521,528 filed Oct. 23, 2014; and 14/521,534 filed Oct. 23, 2014, the last three of which are continuation reissues of application Ser. No. 14/329,019.
TECHNICAL FIELD
The present invention relates to a method of determining an amount of glycated hemoglobin present in whole blood.
BACKGROUND ART
Glycated hemoglobin in blood has served as an important index for the diagnosis, treatment, etc. of diabetes because it reflects previous blood glucose levels in vivo.
The determination of such glycated hemoglobin has been carried out, for example, by high performance liquid chromatography (HPLC), a minicolumn method, immunoassays, and the like. According to these methods, the amount or ratio of hemoglobin that has been glycated can be determined. Recently, an enzymic method that enables the determination of glycated proteins by means of a fructosyl amino acid oxidoreductase (FAOD) has been developed, and attempts have been made to determine an amount of hemoglobin that has been glycated (i.e., glycated hemoglobin) by this enzymic method.
DISCLOSURE OF INVENTION
However, the above-mentioned method has a problem as follows. Because the glycated hemoglobin is a component contained in a blood cell, it is absolutely necessary to hemolyze the blood cell to carry out the determination of the glycated hemoglobin. In the case where a sample to be analyzed is whole blood, however, the treatment for causing hemolysis (hereinafter, referred to as “hemolysis treatment”) conducted on the whole blood brings about a state where blood cell components and plasma components are mixed with each other. Thus, the whole blood sample that has been subjected to the hemolysis treatment contains not only the glycated hemoglobin as a blood cell component but also albumin as a high-content plasma component and glycated albumin as a glycation product thereof, in particular. The glycated albumin is determined together with the glycated hemoglobin because FAOD also acts on the glycated albumin. On this account, a complicated process for separating the plasma and blood cells from the whole blood sample is required in order to eliminate the effect of other glycoproteins such as the glycated albumin and the like.
Therefore, it is an object of the present invention to provide a method of determining an amount of glycated hemoglobin, which allows the effect of other glycoproteins to be eliminated without separating plasma and blood cells in a whole blood sample so that an amount of glycated hemoglobin in the whole blood sample is determined accurately and easily.
In order to achieve the above object, a method of determining an amount of glycated hemoglobin according to the present invention includes: degrading glycated hemoglobin in whole blood selectively with a protease to give a glycated hemoglobin degradation product; causing a redox reaction between a glycation site of the glycated hemoglobin degradation product and FAOD; and determining the redox reaction to determine an amount of the glycated hemoglobin. The term “an amount of glycated hemoglobin” as used in the present invention also includes a ratio of glycated hemoglobin.
If the glycated hemoglobin is distinguished from other proteins and peptides and is degraded selectively (i.e., specifically) with a protease as described above, it becomes possible to determine an amount of the glycated hemoglobin while eliminating the effect of other glycoproteins, especially glycated albumin, without separating blood cells from the whole blood because FAOD hardly acts on proteins or long polypeptide chains. Thus, a sample to be used in this method may be whole blood that has been subjected to a hemolysis treatment, for example.
In the method of the present invention, in order to degrade glycated hemoglobin selectively, a protease capable of degrading the glycated hemoglobin selectively, for example, may be used as the protease. Further, in the present invention, a method of degrading glycated hemoglobin selectively is not limited to the use of the protease capable of degrading the glycated hemoglobin selectively. The glycated hemoglobin may be degraded selectively by any other means. Also, the protease capable of degrading glycated hemoglobin selectively may be used in combination with one or more of ordinary proteases.
It is preferable that the protease capable of degrading glycated hemoglobin selectively is at least one of bromelains, papains, trypsins derived from porcine pancreas, metalloproteinases, and proteases derived from Bacillus subtilis. Examples of the proteases derived from Bacillus subtilis include Protease N (trade name, available from Sigma Aldrich Co.), Protease N “AMANO” (trade name, available from Amano Enzyme Inc.), and the like. Examples of the metalloproteinases include a metalloproteinase derived from the genus Bacillus (EC 3. 4. 24. 4) (e.g., available from Toyobo Co., Ltd. under the trade name Toyoteam), and the like. Among these, the metalloproteinases, bromelains, and papains are more preferable, and the metalloproteinases are most preferable.
In the method of the present invention, it is preferable that a substrate of the FAOD is at least one glycated amine selected from the group consisting of glycated proteins, glycated peptides, and glycated amino acids, and the FAOD acts on at least one of a glycated α-amino group and a glyeated side-chain amino group of the glycated amine to catalyze a reaction that causes generation of hydrogen peroxide.
In the method of the present invention, the glycation site of the glycated hemoglobin degradation product to be reacted with the FAOD preferably is a glycated amino group in a side chain of an amino acid residue and a glycated α-amino group, for example, whereas the glycation site to be reacted with the FAOD varies depending on the catalytic reaction caused by the FAOD to be used. Preferably, the glycation site is the glycated amino group in a side chain of an amino acid residue because FAOD having a catalytic function as described later can act thereon more easily. Examples of the glycated amino group include a glycated amino group in a side chain of a lysine residue, a glycated amino group in a side chain of an arginine residue, and the like.
In the method of the present invention, it is preferable that the protease is added to the whole blood so that a content of the protease per milliliter of the whole blood is in a range from 1,000 to 10,000,000 U. Further, it is preferable that the FAOD is added to the whole blood so that a content of the FAOD per milliliter of the whole blood is in a range from 500 to 40,000 U.
In the method of the present invention, it is preferable that determining the redox reaction is determining an amount of hydrogen peroxide generated by the redox reaction or an amount of oxygen consumed by the redox reaction. In the method of the present invention, it is preferable that the amount of the hydrogen peroxide is determined using a peroxidase (hereinafter, referred to as “POD”) and a substrate that develops color by oxidation.
In the method of the present invention, the substrate that develops color by oxidization is not specifically limited and can be, for example, N-(carboxymethylaminocarbonyl)-4,4′-bis(dimethylamino)diphenylamine sodium, orthophenylenediamine (OPD), and a substrate obtained by combining a Trinder's reagent and 4-aminoantipyrine. Examples of the Trinder's reagent include phenols, phenol derivatives, aniline derivatives, naphthols, naphthol derivatives, naphthylamine, naphthylamine derivatives, and the like. Further, in place of the above-mentioned 4-aminoantipyrine, it is possible to use aminoantipyrine derivatives, vanillin diamine sulfonic acid, methyl benzothiazolinone hydrazone (MBTH), sulfonated methyl benzothiazolinone hydrazone (SMBTH), and the like. Among these chromogenic substrates, N-(carboxymethylaminocarbonyl)-4,4′-bis (dimethylamino)diphenylamine sodium is most preferable.
Next, a method of determining an amount of HbA1c according to the present invention includes: preparing a calibration curve based on a correlation between an amount of glycated hemoglobin determined by the method of determining an amount of glycated hemoglobin according to the present invention and an amount of HbA1c; and substituting the amount of glycated hemoglobin in a whole blood sample determined by the method into the calibration curve to determine an amount of HbA1c in the whole blood sample.
Through a further intensive study, the inventors of the present invention have found that there is a strong correlation between an amount of glycated hemoglobin in a whole blood sample determined according to the method of the present invention and an amount of HbA1c in the whole blood sample. HbA1c is a glycated hemoglobin in which the N-terminal α-amino group in the β-chain of hemoglobin has been glycated. Among various glyeated hemoglobins, HbA1c has served as a particularly important index for the diagnosis etc. of diabetes. According to conventional methods of determining HbA1c, it is necessary that FAOD specifically acts on the glycated N-terminal α-amino group in the β-chain, which is the characteristic structure of HbA1c, among its glycation site and thereafter, the redox reaction caused by the FAOD is determined. In this case, special techniques are required because it is necessary that FAOD to be used has high substrate specificity to the glycated α-amino group and that the FAOD acts on the glycated α-amino group sufficiently, for example. In contrast, according to the method of determining HbA1c of the present invention, HbA1c as an important index for the diagnosis of diabetes can be determined accurately and easily so that the determination of HbA1c can be made practical in clinical tests etc.
In the method of determining HbA1c of the present invention, it is preferable that the calibration curve is prepared based on a correlation between a known amount of HbA1c in a standard sample and an amount of glycated hemoglobin in the standard sample determined by the method of determining an amount of glycated hemoglobin according to the present invention.
Next, a kit used for determining an amount of glycated hemoglobin according to the present invention includes a protease that distinguishes a glycated hemoglobin from other proteins and peptides to degrade the glycated hemoglobin selectively. By using this kit, the method of the present invention can be carried out easily.
In the kit of the present invention, the protease is at least one protease selected from the group consisting of bromelains, papains, trypsins derived from porcine pancreas, metalloproteinases, and proteases derived from Bacillus subtilis. Further, it is preferable that the kit further includes FAOD. Furthermore, it is preferable that a substrate of the FAOD is at least one glycated amine selected from the group consisting of glycated proteins, glycated peptides, and glycated amino acids, and the FAOD acts on at least one of a glycated α-amino group and a glycated side-chain amino group of the glycated amine to catalyze a reaction that causes generation of hydrogen peroxide. Still further, it is preferable that the kit further includes POD and a substrate that develops color by oxidization. The substrate that develops color by oxidization preferably is N-(carboxymethylaminocarbonyl)-4,4′-bis (dimethylamino)diphenylamine sodium.
Next, a reagent used for determining an amount of glycated hemoglobin according to the present invention includes a protease that distinguishes a glycated hemoglobin from other proteins and peptides to degrade the glycated hemoglobin selectively. By using this reagent, the method of the present invention can be carried out easily.
In the reagent of the present invention, the protease is at least one protease selected from the group consisting of bromelains, papains, trypsins derived from porcine pancreas, metalloproteinases, and proteases derived from Bacillus subtilis. Further, it is preferable that the reagent further includes FAOD. Furthermore, it is preferable that a substrate of the FAOD is at least one glycated amine selected from the group consisting of glycated proteins, glycated peptides, and glycated amino acids, and the FAOD acts on at least one of a glycated α-amino group and a glycated side-chain amino group of the glycated amine to catalyze a reaction that causes generation of hydrogen peroxide. Still further, it is preferable that the reagent further includes POD and a substrate that develops color by oxidization. The substrate that develops color by oxidization preferably is N-(carboxymethylaminocarbonyl)-4,4′-bis (dimethylamino)diphenylamine sodium.
BRIEF DESCRIPTION OF DRAWINGS
FIG. 1 is a graph showing the correlation between an HbA1c concentration and an absorbance in a method of determining an amount of glycated hemoglobin according to one example of the present invention.
FIG. 2 is a graph showing the correlation between HbA1c (%) determined using a calibration curve and HbA1c (%) measured using an automatic measuring apparatus in a method of determining an amount of glycated hemoglobin according to another example of the present invention.
BEST MODE FOR CARRYING OUT THE INVENTION
In a method of determining an amount of glycated hemoglobin according to the present invention, FAOD capable of catalyzing a reaction represented by Formula (1) below preferably is used.
R1—CO—CH2—NH—R2+H2O+O2→R 1—CO—CHO+NH2—R2+H2O2   (1)
In Formula (1), R1—CO—CH2—NH—R2 denotes a glycated protein, glycated peptide, and glycated amino acid, for example. In Formula (1), R1 denotes a hydroxyl group or a residue derided from a sugar that is not yet subjected to the glycation reaction (i.e., sugar moiety). The sugar moiety (R1) is an aldose residue when the unreacted sugar is aldose, and is a ketose residue when the unreacted sugar is ketose. When the unreacted sugar is glucose, for example, the sugar in the glycated product takes on the fructose structure after the glycation reaction due to Amadori rearrangement. In this case, the sugar moiety (R1) is a glucose residue (aldose residue). This sugar moiety (R1) can be represented, for example, by
—[CH(OH)]n—CH2OH
where n denotes an integer of 0 to 6.
In Formula (1), R2 is not specifically limited. However, it is to be noted that R2 varies depending on which of an α-amino group and an amino group other than the α-amino group is glycated.
In Formula (1), in the case where an α-amino group is glycated, R2 is an amino acid residue or a peptide residue represented by Formula (2) below.
—CHR3—CO—R4   (2)
In Formula (2), R3 denotes an amino-acid side chain group. R4 denotes a hydroxyl group, an amino acid residue, or a peptide residue, and can be represented, for example, by Formula (3) below. In Formula (3), n denotes an integer of 0 or more, and R3 denotes an amino-acid side chain group as described above.
—(NH—CR3H—CO)n—OH   (3)
In Formula (1), in the case where an amino group other than the α-amino group is glycated (i.e., an amino-acid side chain group is glycated), R2 is represented by Formula (4) below.
—R5—CH(NH—R6)—CO—R7
In Formula (4), R5 denotes a portion other than the glycated amino group in the amino-acid side chain group. For example, in the case where the glycated amino acid is lysine, R5 is as follows.
—CH2—CH2—CH2—CH2
On the other hand, in the case where the glycated amino acid is arginine, for example, R5 is as follows.
—CH2—CH2—CH2—NH—CH(NH2)—
In Formula (4), R6 denotes hydrogen, an amino acid residue, or a peptide residue, and can be represented, for example, by Formula (5) below. In Formula (5), n denotes an integer of 0 or more, and R3 denotes an amino-acid side chain group as described above.
—(CO—CR3H—NH)n—H   (5)
In Formula (4), R7 denotes a hydroxyl group, an amino acid residue, or a peptide residue, and can be represented, for example, by Formula (6) below. In Formula (6), n denotes an integer of 0 or more, and R3 denotes an amino-acid side chain group as described above.
—(NH—CHR3—CO)n—OH   (6)
A catalytic reaction caused by FAOD to be used in the method of the present invention is not specifically limited as long as it is a reaction represented by Formula (1). However, in Formula (1), it is preferable that the FAOD acts on the glycation site in which a sugar is bound to an amino group other than an α-amino group (i.e., R2 has a structure as represented by Formula (4)). Further, the catalytic function of the FAOD is not limited to such function. In addition to the above catalytic function, the FAOD further may have a catalytic function to act on the glycation site in which a sugar is bound to an α-amino group (i.e., R2 has a structure as represented by Formula (2)).
Examples of such FAOD include those derived from the genus Fusarium, the genus Gibberella, and the genus Aspergillus. More specifically, commercially available FAODs such as Fructosyl Amino Acid Oxidase (trade name, available from Asahi Chemical Industry Co., Ltd.), Ketoamine Oxidase (trade name, available from Genzyme Corporation), and the like can be used, for example.
Hereinafter, an example of a method of determining an amount of glycated hemoglobin according to the present invention will be described.
First, the whole blood is hemolyzed. The method of hemolyzing the whole blood is not specifically limited, and can be, for example, a method using a surfactant, a method using ultrasonic waves, and a method utilizing the difference in osmotic pressure. Among these, the method using a surfactant is preferable on account of the ease of operation.
As the surfactant, nonionic surfactants such as polyoxyethylene-p-t-octylphenyl ether (Triton-type surfactant etc.), polyoxyethylene sorbitan alkyl ester (Tween-type surfactant etc.), polyoxyethylene alkyl ether (Brij-type surfactant etc.), and the like can be used, for example. More specifically, Triton X-100 (trade name), Tween-20 (trade name), Brij 35 (trade name), and the like can be used, for example. Generally, the treatment with the above surfactant can be carried out under the following conditions: in the case where the solution to be treated contains 1 to 10 vol % of blood cells, the surfactant is added to the solution so as to give a concentration of 0.1 to 1 wt % and the resultant mixture is stirred at room temperature for about 5 seconds to 1 minute.
Further, when utilizing the difference in osmotic pressure, to the whole blood was added 2 to 100 times its volume of purified water to cause hemolysis, for example.
Subsequently, the above-mentioned hemolysate sample is treated with the above-mentioned protease, thereby selectively degrading glycated hemoglobin in the sample. Generally, this protease treatment is carried out in a buffer. The treatment conditions are decided as appropriate, for example, depending on the type of the protease to be used, the amount of the glycated hemoglobin, and the like.
In the case where the hemolysate sample is treated using a papain as the protease, the treatment generally is carried out under the following conditions: the protease concentration in the reaction solution in the range from 100 to 30,000 U/L, the hemoglobin concentration in the reaction solution in the range from 0.1 to 40 g/L, the reaction temperature in the range from 15° C. to 60° C., the reaction time in the range from 10 minutes to 40 hours, and the pH in the range from 5 to 9. Further, the type of the buffer is not specifically limited, and can be, for example, Tris-HCl buffer, EPPS buffer, PIPES buffer, phosphate buffer, ADA buffer, citrate buffer, acetate buffer, and the like.
In the case where the hemolysate sample is treated using a metalloproteinase as the protease, the treatment is carried out, for example, under the following conditions: the protease concentration in the reaction solution in the range from 10 to 10,000 KU/L, the hemoglobin concentration in the reaction solution in the range from 0.02 to 40 g/L, the reaction temperature in the range from 15° C. to 60° C., the reaction time in the range from 2 minutes to 40 hours, and the pH in the range from 6 to 11; preferably, the protease concentration in the reaction solution in the range from 100 to 8,000 KU/L, the hemoglobin concentration in the reaction solution in the range from 0.1 to 10 g/L, the reaction temperature in the range from 15° C. to 60° C., the reaction time in the range from 2 minutes to 1 hour, and the pH in the range from 7 to 10. As the buffer, the above-mentioned various buffers also can be used. Further, other proteinases also can be used.
Next, the glycated hemoglobin degradation product obtained through the above-mentioned protease treatment is treated with FAOD. This FAOD treatment catalyzes the reaction represented by Formula (1) above. More specifically, FAOD acts on a glycated amino group in a side chain of a lysine residue and a side chain of an arginine residue in the glycated hemoglobin degradation product, for example. Further, depending on the type of the FAOD to be used, the FAOD further may act on a glycated α-amino group according to its catalytic function.
Similarly to the above-mentioned protease treatment, this FAOD treatment preferably is carried out in a buffer. The buffer is not specifically limited, and the same buffers as used in the protease treatment also can be used in the FAOD treatment.
The FAOD treatment is carried out, for example, under the following conditions: the FAOD concentration in the reaction solution in the range from 200 to 30,000 U/L, the hemoglobin concentration in the reaction solution in the range from 0.02 to 30 g/L, the reaction temperature in the range from 15° C. to 37° C., the reaction time in the range from 1 to 20 minutes, and the pH in the range from 7 to 9; preferably, the FAOD concentration in the range from 1,000 to 20,000 U/L, the hemoglobin concentration in the reaction solution in the range from 0.1 to 5 g/L, the reaction temperature in the range from 15° C. to 37° C., the reaction time in the range from 1 to 5 minutes, and the pH in the range from 7 to 9.
Next, the amount of the hydrogen peroxide generated by the FAOD treatment is determined utilizing a redox reaction, by using the POD and a substrate that develops color by oxidization.
The redox reaction caused by the POD generally is induced in a buffer under the conditions decided as appropriate, for example, depending on the concentration of the hydrogen peroxide and the like. Generally, the redox reaction is induced under the following conditions: the POD concentration in the reaction solution in the range from 1 to 100,000 IU/L, the substrate concentration in the range from 0.0001 to 1 mmol/L, the reaction temperature in the range from 20° C. to 37° C., the reaction time in the range from 1 to 5 minutes, and the pH in the range from 6 to 9; preferably, the POD concentration in the reaction solution in the range from 1,000 to 50,000 IU/L, the substrate concentration in the range from 0.0002 to 0.1 mmol/L, the reaction temperature in the range from 20° C. to 37° C., the reaction time in the range from 1 to 5 minutes, and the pH in the range from 6 to 9. Further, the buffer is not specifically limited, and the same buffers as used in the FAOD treatment also can be used.
It is to be noted here that the amount of the hydrogen peroxide can be determined not only by the above-mentioned enzymic method using the POD etc. but also by an electrical method, for example.
In the case where the substrate that develops color by the above oxidization is used, the concentration of the hydrogen peroxide can be determined by measuring the color development (i.e., the absorbance of the reaction solution) with a spectrophotometer. From the concentration of the hydrogen peroxide, the concentration of the glycated hemoglobin in the sample can be determined.
In the process of determining an amount of glycated hemoglobin as described above, the respective treatment steps may be performed individually as described above, or some of the treatment steps may be performed simultaneously in the following combinations, for example.
1: hemolysis treatment+protease treatment
2: protease treatment+FAOD treatment
3: FAOD treatment+POD treatment
Also, the order in which the FAOD, the POD, and the substrate are added is not specifically limited.
Hereinafter, an example of a method of determining HbA1c according to the present invention will be described.
First, an amount of glycated hemoglobin in a whole blood sample is determined in the above-mentioned manner. On the other hand, a glycated hemoglobin standard solution in which an amount of HbA1c in glycated hemoglobin is known is provided. Then, an amount of glycated hemoglobin in this standard solution is determined in the above-mentioned manner. After that, a calibration curve is prepared that shows the relation between the amount of glycated hemoglobin thus determined and the known amount of HbA1c in this standard solution. Since there is a correlation between the determined amount of glycated hemoglobin and the known amount of HbA1c as described above, an amount of HbA1c in the whole blood sample can be determined by substituting the amount of glycated hemoglobin in the whole blood sample determined by the method of the present invention into this calibration curve. In the preparation of the calibration curve, the determined amount of glycated hemoglobin is not limited to the value finally obtained though the method of the invention, and can be an absorbance of the reaction solution obtained by the POD treatment during the determination process, or an amount of hydrogen peroxide determined based on this absorbance. As described above, according to the method of determining an amount of HbA1c of the present invention, an amount of HbA1c in whole blood can be determined accurately and easily based on an amount of glycated hemoglobin determined by utilizing the correlation discovered by the inventors of the present invention.
EXAMPLES Example 1
Samples containing glycated hemoglobin and glycated albumin were treated with a papain. Then, a redox reaction thereof was caused by FAOD, and the amount of hydrogen peroxide generated was determined. The samples, reagents, and method used in the determination will be described in the following.
(Samples)
    • Human serum albumin with glycation ratio of 22.5% (Sigma Chemical Co.)
    • Human hemoglobin with glycation ratio of 14%
The above human hemoglobin sample was prepared in the following manner, and the glycation ratio thereof was determined by HPLC using an ion exchange column.
(Preparation of Human Hemoglobin)
Whole blood of a healthy subject was centrifuged (1500 G, 10 min) and blood cells were collected. After washing the blood cells with a physiological salt solution several times, a substantially equivalent amount of purified water was added to the blood cells to cause hemolysis. The hemolysate was then centrifuged to remove cell membranes. The solution thus obtained was supplied to GLYCO•GEL II (trade name, available from Pierce Chemical Company). A fraction containing a glycated protein was separated and collected according to the usual method, and the solution thus obtained was used as the human hemoglobin sample.
(Composition of Redox Solution A)
FAOD (Asahi Chemical Industry Co., Ltd., 2.09 KU/L
hereinafter the same)
POD (Type III: Toyobo Co., Ltd., hereinafter the same) 730 U/L
N-(carboxymethylaminocarbonyl)-4,4′-bis(di- 1.46 mmol/L
methylamino)diphenylamine sodium (Trade name
DA 64: Wako Pure Chemical Industries, Ltd.,
hereinafter the same)
Tris-HCl buffer (pH 8.0) 73 mmol/L

(Method) First, 1 mL of a 1 KU/L papain (available from Sigma Aldrich Co.) was added to 1 mL of the above-mentioned respective samples (human serum albumin, human hemoglobin), and the mixtures were reacted at 40° C. for 24 hours. To 0.018 mL of the thus-obtained solutions was added 0.15 mL of the above redox solution A to cause a redox reaction. Then, 5 minutes after the start of the reaction, the absorbance of these reaction solutions was measured at the main wavelength of 694 nm and the sub-wavelength of 884 nm using a biochemical automatic analysis apparatus (the trade name JCA-BM 8: available from Japan Electron Optics Laboratory Co. Ltd., hereinafter the same). The results are shown in Table 1 below.
Example 2
The above-mentioned respective samples (human serum albumin, human hemoglobin) were treated in the same manner as in Example 1 except that 1 mL of a 1 g/L bromelain (available from Amano Enzyme Inc., hereinafter the same) was used in place of the papain, and the absorbance thereof was measured in the same manner as in Example 1. The results are shown in Table 1 below.
Comparative Example 1
The above-mentioned respective samples (human serum albumin, human hemoglobin) were treated in the same manner as in Example 1 except that 1 mL of a 1 g/L α-chymotrypsin was used in place of the papain, and the absorbance thereof was measured in the same manner as in Example 1. The results are shown in Table 1 below.
TABLE 1
Human serum Human
albumin hemoglobin
Protease (Abs.) (Abs.)
Example 1: Papain 0.014 0.090
Example 2: Bromelain 0.0008 0.037
Comparative Example 1: α-chymotrypsin 0.063 0.042
As shown in Table 1, in the case where the papain and bromelain were used as in Examples 1 and 2, the human hemoglobin sample exhibited a high absorbance while the human serum albumin sample exhibited a very low absorbance. These results demonstrate that the papain and bromelain can degrade glycated hemoglobin selectively and hardly degrade glycated albumin. In contrast, in the case where the w-chymotrypsin was used as in Comparative Example 1, both the samples exhibited a high absorbance. These results demonstrate that the w-chymotrypsin acts not only on glycated hemoglobin but also on glycated albumin and thus does not degrade glycated hemoglobin selectively.
Example 3 and Comparative Example 2
Whole blood, plasma, and blood cells were used as samples, and the amount of glycated hemoglobin in the respective samples were determined after treating the respective samples with various proteases.
(Preparation of Whole Blood Samples)
Whole blood was collected from a healthy subject using a blood-collecting vessel containing heparin sodium. The whole blood was diluted 8-fold with purified water to hemolyze the blood cells contained therein. The resultant solution was used as whole blood samples.
(Preparation of Plasma Samples)
Whole blood collected from the above-mentioned healthy subject was centrifuged (1500 G, 10 min) to remove blood cells, and the supernatant obtained was diluted 8-fold with purified water. The resultant solution was used as plasma samples.
(Preparation of Blood Cell Samples)
The blood cells obtained though the above-mentioned centrifugation were diluted 16-fold with purified water to cause hemolysis. The resultant solution was used as blood cell samples.
(Proteases)
A bromelain, papain (available from Hoffmann-La Roche Inc.), elastase (available from Wako Pure Chemical Industries, Ltd.), α-chymotrypsin (available from Wako Pure Chemical Industries, Ltd.), and proteinase K (available from Wako Pure Chemical Industries, Ltd.) were dissolved in purified water, respectively, to prepare 4g/L solutions of the respective proteases.
(Composition of Redox Solution B)
POD 20 KU/L
DA 64 (trade name) 0.04 mmol/L
Potassium phosphate buffer (pH 7.0) 0.1 mol/L
(Composition of Redox Solution C)
FAOD 14.3 KU/L
Potassium phosphate buffer (pH 7.0) 0.1 mol/L

(Determining Method)
First, 0.1 mL of each of the protease solutions and 0.7 mL of potassium phosphate buffer (pH 7.0) were mixed with 0.2 mL of the above-mentioned respective samples, and the resultant mixtures were reacted at 37° C. for 24 hours. Thereafter, the reaction solutions were supplied to Ultra Free 4 Unit 5K (trade name, available from Millipore Corporation) so that the reaction solutions were centrifuged and the supernatants were collected. Subsequently, 45 μL of the redox solution B was added to 25 μL of the respective supernatants, and 20 μl of the redox solution C was further added after 5 minutes to cause a redox reaction. Then, 5 minutes after the start of the reaction, the absorbance of the respective reaction solutions was measured at the main wavelength of 694 nm and the sub-wavelength of 884 nm using the above-mentioned biochemical automatic analysis apparatus. The results are shown in Table 2 below. The bromelain and papain were used in Example 3, and the elastase, α-chymotrypsin, and proteinase K were used in Comparative Example 2.
TABLE 2
Plasma Blood cells Whole blood
Sample Protease (Abs.) (Abs.) (Abs.)
Example 3 Bromelain 0.0 0.009 0.002
Papain 0.001 0.021 0.015
Comparative Elastase 0.012 0.019 0.015
Example 2 α-chymotrypsin 0.015 0.016 0.013
Proteinase K 0.036 0.027 0.034
As can be seen from Table 2, in Example 3, substantially no absorption was observed in the plasma samples. These results demonstrate that the proteases used in Example 3 can degrade glycated hemoglobin selectively and hardly degrade glycated albumin etc. derived from plasma, for example. In contrast, in Comparative Example 2, absorption was observed in the plasma samples even though the plasma samples contained no glycated hemoglobin. The reason for this is considered to be that, because the proteases used in Comparative Example 2 degrade glycated proteins without distinguishing glycated hemoglobin from other glycated proteins, glycated albumin and the like also are degraded in the plasma samples, for example, thereby allowing the absorption to be observed in the plasma samples.
Example 4
(Preparation of Glycated hemoglobin Standard Solutions)
HbA1c standard reagents (available from SRL, Inc.) were dissolved in purified water to prepare glycated hemoglobin standard solutions containing HbA1c at concentrations 4.3%, 7.8%, 11.2%, and 14.7%, respectively, while containing 10 g/L hemoglobin. Further, HbA1c standard reagents (available from International Regents Corporation) were dissolved in purified water to prepare glycated hemoglobin standard solutions containing HbA1c at concentrations 5.5% and 10.8%, respectively, while containing 10 g/L hemoglobin.
(Preparation of Various Protease Solutions)
A 2 g/L solution of a bromelain F (available from Amano Enzyme Inc.) and a 1 g/L solution of a papain (available from Hoffmann-La Roche Inc.) were prepared by dissolving the respective proteases in purified water.
(Determining Method)
First, 0.4 mL of each of the protease solutions and 0.1 mL of a 1.0 mol/L potassium phosphate buffer (pH 8.0) were mixed with 0.5 mL of the above-mentioned respective glycated hemoglobin standard solutions with different hemoglobin concentrations. The mixtures were reacted at 37° C. for 24 hours. Thereafter, the reaction solutions were supplied to Ultrafree-MC 5000 MW (trade name, available from Millipore Corporation, hereinafter the same) so that the reaction solutions were centrifuged and the supernatants were collected. Then, 25 μL of the supernatants were diluted 2-fold with purified water. Subsequently, 45 μL of the redox solution B was added to the respective diluted solutions, and 20 μl of the redox solution C was further added after 5 minutes to cause a redox reaction. Then, 5 minutes after the start of the reaction, the absorbance of the respective reaction solutions was measured at the main wavelength of 694 nm and the sub-wavelength of 884 nm using the above-mentioned biochemical automatic analysis apparatus. The results are shown in Table 3 below and in the graph shown in FIG. 1.
TABLE 3
HbA1c (%)
Protease 4.3 5.5 7.8 10.8 11.2 14.7
Papain 0.010 0.016 0.026 0.043 0.041 0.059
Bromelain 0.002 0.004 0.005 0.014 0.008 0.010
FIG. 1 is a graph showing the correlation between an HbA1c concentration and an absorbance in the glycated hemoglobin standard solution. In the case where the papain was used, the correlation equation was y=210x+2.2 and the correlation coefficient was r=0.998. On the other hand, in the case where the bromelain was used, the correlation equation was y=1321x+1.0 and the correlation coefficient was r=0.968.
As shown in Table 3 and FIG. 1, the absorbance increases linearly with an increase in the HbA1c concentration in the glycated hemoglobin standard solution. These results demonstrate that there is a strong correlation between an HbA1c concentration and an absorbance (which corresponds to an amount of glycated hemoglobin determined by the method of the present invention). Therefore, by preparing the calibration curve showing the correlation between the HbA1c concentration and the absorbance in advance, it becomes possible to determine an amount of HbA1c in a whole blood sample indirectly using the calibration curve and the amount of glycated hemoglobin in the whole blood sample determined in the above-mentioned manner.
Example 5
Hemolysate samples were treated with a metalloproteinase, a papain, and a protease derived from Bacillus subtilis, and the amounts of glycated hemoglobin in the respective samples were determined according to the method of the present invention. Further, the amounts of HbA1c in the respective samples were determined based on the amounts of glycated hemoglobin thus determined. The samples, reagents, and method used in the determination will be described in the following.
(Preparation of Samples)
Whole blood was collected from healthy subjects and diabetic subjects (12 subjects in total), and allowed to stand for about 6 hours so that red blood cells contained therein were settled. Then, to 0.1 mL of the blood cell fractions were added 1.4 mL of 0.05 wt % Triton X-100 aqueous solutions, respectively, to cause hemolysis. The resultant solutions were used as hemolysate samples.
(Preparation of Standard Solutions)
HbA1c standard reagents (available from International Regents Corporation) were dissolved in 0.05 wt % Triron X-100 aqueous solutions to prepare glycated hemoglobin standard solutions containing HbA1c at concentrations 5.5% and 10.5%, respectively, while containing 200 g/L hemoglobin.
(Preparation of Protease Solutions)
A metalloproteinase (available from Toyobo Co., Ltd.), Protease N “AMANO” (trade name, available from Amano Enzyme Inc.), and a papain (available from Hoffmann-La Roche Inc.) were dissolved in purified water to prepare 1 g/L solutions of the respective proteases.
(Composition of Redox Solution D)
POD 20 KU/L
DA-64 (trade name) 0.04 mmol/L
Phosphate buffer (pH 8.0) 0.8 mol/L
(Composition of Redox Solution E)
FAOD 14.3 KU/L
Potassium phosphate buffer (pH 8.0) 0.1 mmol/L

(Method of Determining Amount of glycated hemoglobin)
First, 0.16 mL of each of the protease solutions and 0.04 mL of a 1.0 mol/L potassium phosphate buffer (pH 8.0) were mixed with 0.2 mL of the above-mentioned respective samples. The mixtures were reacted at 37° C. for 36 hours. Thereafter, the reaction solutions were supplied to the Ultrafree-MC 5000 MW (trade name) so that the reaction solutions were centrifuged and the supernatants were collected. Then, 25 μL of the supernatants were diluted 2-fold with purified water. Subsequently, 45 μL of the redox solution D was added to the respective diluted solutions, and 20 μl of the redox solution E was further added after 5 minutes to cause a redox reaction. Then, 2 minutes after the start of the reaction, the absorbance of the respective reaction solutions was measured at the main wavelength of 751 nm and the sub-wavelength of 884 nm. The absorbance thus measured corresponds to the amount of glycated hemoglobin.
(Method of Determining Hemoglobin Concentration)
Hemoglobin concentrations in the respective samples were determined according to the cyanmethemoglobin method using Hemoglobin Test Wako (trade name, available from Wako Pure Chemical Industries, Ltd.).
(Preparation of Calibration Curve) HbA1c concentrations (%) of the above-mentioned respective standard solutions were measured using an automatic measuring apparatus (the trade name HA-8150: available from ARKRAY, INC.). On the other hand, with regard to the above-mentioned respective standard solutions, the absorbances corresponding to the amounts of glycated hemoglobin were measured by the method of determining an amount of glycated hemoglobin according to the present invention and hemoglobin concentrations were determined by the above-mentioned method of determining a hemoglobin concentration. Then, primary regression equations were prepared for the respective standard solutions based on the percentages (%) obtained by dividing the absorbances corresponding to the amounts of glycated hemoglobin by the hemoglobin concentrations and the measured values (%) given by the automatic measuring apparatus. The primary regression equations thus obtained were used as calibration curves. It is to be noted that the above-mentioned percentages are proportional to the ratios (%) of the glycated hemoglobin. The primary regression equations used as calibration curves in the case where the above-mentioned respective proteases were used are shown in the following.
(Calibration Curve)
Protease Primary Regression Equation
Metalloproteinase y = 15846x + 3.2
Protease N “AMANO” y = 16659x + 3.3
Papain y = 17258x + 3.4

(Method of Determining HbA1c)
With regard to the above-mentioned respective hemolysate samples, the absorbances corresponding to the amounts of glycated hemoglobin were measured by the above-mentioned method of determining the amount of glycated hemoglobin, and hemoglobin concentrations were determined by the above-mentioned method of determining a hemoglobin concentration. Then, the percentages obtained by dividing the absorbances corresponding to the amounts of glycated hemoglobin by the hemoglobin concentrations were regarded as the ratios of the glycated hemoglobin, and the amounts of HbA1c in the respective hemolysate samples were determined by substituting the thus-obtained ratios into the above-mentioned respective calibration curves. Further, as controls, the amounts of HbA1c in the respective hemolysate samples were measured using the above-mentioned automatic analysis apparatus. The results are shown in FIG. 2. FIG. 2 is a graph showing the correlations between the amounts of HbA1c determined using the calibration curves according to the method of the present invention and the amounts of HbA1c measured using the automatic measuring apparatus.
As can be seen from FIG. 2, correlation coefficients between HbA1c (%) determined using the calibration curves according to the method of the present invention and HbA1c (%) measured using the automatic measuring apparatus were very high. More specifically, a correlation coefficient in the case where the metalloproteinase was used was 0.9937; a correlation coefficient in the case where the Protease N was used was 0.993; and a correlation coefficient in the case where the papain was used was 0.9941. These results demonstrate that the method of determining an amount of HbA1c according to the present invention can determine the amount of HbA1c with an accuracy comparable to that of the automatic analysis apparatus.
Example 6
Hemolysate samples to which plasma samples have been added were treated with a metalloproteinase. Amounts of glycated hemoglobin in the respective samples were determined to examine the change in the amounts of glycated hemoglobin caused by the addition of the plasma samples.
(Preparation of Samples)
Whole blood collected from a healthy subject (1 subject) and diabetic subjects (diabetic subject 1 and diabetic subject 2) was centrifuged (1000 G, about 15 min), and blood cell fractions and plasma fractions of the respective subjects were collected. Thereafter, predetermined amounts (0 mL, 0.005 mL, 0.010 mL, 0.015 mL, and 0.020 mL) of the plasma fractions of the respective subjects were added to 0.01 mL of the blood cell fractions of the corresponding subjects. Then, to the respective mixtures was added 0.3 mL of the following hemolysis reagent. The resultant solutions were used as hemolysate samples.
Subsequently, 0.065 mL of the following metalloproteinase reagent was added to 0.01 mL of the respective hemolysate samples. The mixtures were incubated at 37° C. for 5 minutes. Then, 0.045 mL of the following redox solution F was further added, and the resultant mixtures were incubated at 37° C. for 2 minutes. Thereafter, the absorbance of the respective reaction solutions was measured at the main wavelength of 751 nm and the sub-wavelength of 805 nm. The absorbance thus measured corresponds to the amount of glycated hemoglobin. Because the amount of the reaction solutions varies depending on the amount of the plasma fractions added thereto, the absorbances shown in Table 4 are the values that have been corrected to show the absorbances per equivalent amounts of the respective reaction solutions.
(Hemolysis Reagent)
Polyoxyethylene lauryl ether 9 g/L
CHES buffer (pH 9.4) 100 mmol/L
(Metalloproteinase Reagent: pH 5.5)
Metalloproteinase (Toyobo Co., Ltd.) 4000 KU/L
WST-3 (Dojindo Laboratories) 2 mmol/L
MES
5 mmol/L
CaCl2
5 mmol/L
NaCl 50 mmol/L
*WST-3: 2-(4-iodophenyl)-3-(2,4-dinitropheny1)-5-(2,4-disulfopheny1)-2H-tetrazolium monosodium salt
(Redox Solution F)
FAOD 30 KU/L
POD 90 KU/L
DA-64 0.06 mmol/L
Phosphate buffer (pH 7.0) 200 mmol/L
TABLE 4
Added Amount of Plasma fraction Healthy Diabetic Diabetic
(mL) subject subject 1 subject 2
0 0.0215 0.0283 0.0348
0.005 0.0216 0.0278 0.343
0.010 0.0196 0.0283 0.350
0.015 0.0204 0.0289 0.354
0.020 0.0212 0.0288 0.359
As can be seen from Table 4, even when the plasma fractions were added to the blood cell fractions to give different concentrations, the resultant absorbances differed only slightly. These results demonstrate that, according to the method of the present invention, the amount of glycated hemoglobin can be determined without being affected by the glycated proteins present in plasma.
INDUSTRIAL APPLICABILITY
As specifically described above, according to the method of present invention, a ratio of glycated hemoglobin in a whole blood sample can be determined easily and accurately without separating plasma and blood cells in the whole blood sample. Further, since there is a strong correlation between an amount of glycated hemoglobin determined by the method of the present invention and an amount of HbA1c, by preparing a calibration curve based on this correlation in advance, it becomes possible to determine an amount of HbA1c in a whole blood sample accurately and easily by merely determining the amount of glycated hemoglobin in the whole blood sample. Therefore, by applying the method of the present invention in the field of clinical tests etc., for example, it becomes possible to evaluate a large number of subjects easily, which further increases the reliability and the importance of glycated hemoglobin, especially HbA1c, as an index for the diagnosis and the like of diabetes.

Claims (25)

The invention claimed is:
1. A method of determining an amount of glycated hemoglobin in a sample comprising glycated hemoglobin and glycated albumin from whole blood, comprising:
selectively degrading the glycated hemoglobin in the sample with a proteasetreating the sample with a protease that selectively degrades the glycated hemoglobin over the glycated albumin to give a glycated hemoglobin degradation product, wherein the protease is a metalloproteinase;
reacting a glycation site of the glycated hemoglobin degradation product and a fructosyl amino acid oxidoreductase in a redox reaction;
determining a product produced by the redox reaction; and
correlating the amount of the product produced with the amount of glycated hemoglobin in the sample,
wherein the sample to be used in the method is whole blood that has been subjected to a hemolysis treatment.
2. The method according to claim 1, wherein the protease is at least one protease selected from the group consisting of bromelains, papains, trypsins derived from porcine pancreas, metalloproteinases, and proteases derived from Bacillus subtilis.
3. The method according to claim 1, wherein the glycation site of the glycated hemoglobin degradation product that reacts with the fructosyl amino acid oxidoreductase is a glycated amino group in a side chain of an amino acid residue.
4. The method according to claim 3, wherein the glycated amino group in the side chain of the amino acid residue is a glycated amino group in a side chain of at least one of a lysine residue and an arginine residue,
5. The method according to claim 1, wherein determining the redox reaction is determining an amount of hydrogen peroxide generated by the redox reaction or an amount of oxygen consumed by the redox reaction.
6. The method according to claim 5, wherein the amount of the hydrogen peroxide is determined using a peroxidase and a substrate that develops color by oxidization.
7. The method according to claim 6, wherein the substrate that develops color by oxidization is N-(carboxymethylaminocarbonyl)-4,4′-bis(dimethylamino)diphenylamine sodium.
8. The method according to claim 1, wherein the protease is added to the whole blood so that a concentration of the protease per milliliter of the whole blood is in a range from 1,000 to 10,000,000 U.
9. The method according to claim 1, wherein a substrate of the fructosyl amino acid oxidoreductase is at least one glycated amine selected from the group consisting of glycated proteins, glycated peptides, and glycated amino acids, and the fructosyl amino acid oxidoreductase acts on at least one of a glycated α-amino group and a glycated side-chain amino group of the glycated amine to catalyze a reaction that causes generation of hydrogen peroxide.
10. The method according to claim 1, wherein the fructosyl amino acid oxidoreductase is added to the whole blood so that a concentration of the fructosyl amino acid oxidoreductase per milliliter of the whole blood is in a range from 500 to 40,000 U.
11. The method according to claim 1, wherein a sample to be used in the method is whole blood that has been subjected to a hemolysis treatment.
12. The method according to claim 1, wherein the glycation site of the glycated hemoglobin degradation product that reacts with the fructosyl amino acid oxidoreductase is a glycated amino group in a side chain of an amino acid residue.
13. The method according to claim 12, wherein the glycated amino group in the side chain of the amino acid residue is a glycated amino group in a side chain of at least one of a lysine residue and an arginine residue.
14. The method according to claim 1, wherein determining the redox reaction is determining an amount of hydrogen peroxide generated by the redox reaction or an amount of oxygen consumed by the redox reaction.
15. The method according to claim 14, wherein the amount of the hydrogen peroxide is determined using a peroxidase and a substrate that develops color by oxidization.
16. The method according to claim 15, wherein the substrate that develops color by oxidization is N-(carboxymethylaminocarbonyl)-4,4′-bis(dimethylamino)diphenylamine sodium.
17. The method according to claim 1, wherein the protease is added to the whole blood so that a concentration of the protease per milliliter of the whole blood is in a range from 1,000 to 10,000,000 U.
18. The method according to claim 1, wherein a substrate of the fructosyl amino acid oxidoreductase is at least one glycated amine selected from the group consisting of glycated proteins, glycated peptides, and glycated amino acids, and the fructosyl amino acid oxidoreductase acts on at least one of a glycated α-amino group and a glycated side-chain amino group of the glycated amine to catalyze a reaction that causes generation of hydrogen peroxide.
19. The method according to claim 1, wherein the fructosyl amino acid oxidoreductase is added to the whole blood so that a concentration of the fructosyl amino acid oxidoreductase per milliliter of the whole blood is in a range from 500 to 40,000 U.
20. The method according to claim 1, wherein the fructosyl amino acid oxidoreductase is selected from the group consisting of Fusarium, Gibberella and Aspergillus.
21. The method according to claim 1, wherein the hemolysis treatment is selected from the method consisting of using ultrasonic waves and utilizing differences in osmotic pressure.
22. The method according to claim 1, wherein the treatment of the sample with the protease is carried out in a buffer.
23. The method according to claim 22, where the buffer is selected from the group consisting of Tris-HCl buffer, EPPS buffer, PIPES buffer, phosphate buffer, ADA buffer, citrate buffer and acetate buffer.
24. The method according to claim 1, wherein the treatment of the sample with the protease is carried out at a pH in a range from 6 to 11.
25. The method according to claim 1, wherein the whole blood sample to be used in the method has been centrifuged.
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Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US10006923B2 (en) 2013-07-09 2018-06-26 Kyowa Medex Co., Ltd. Method for measuring glycated hemoglobin

Families Citing this family (91)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US6391005B1 (en) 1998-03-30 2002-05-21 Agilent Technologies, Inc. Apparatus and method for penetration with shaft having a sensor for sensing penetration depth
JP4803696B2 (en) * 2000-09-28 2011-10-26 アークレイ株式会社 Method for measuring hemoglobin and method for measuring glycation rate of hemoglobin
US8641644B2 (en) 2000-11-21 2014-02-04 Sanofi-Aventis Deutschland Gmbh Blood testing apparatus having a rotatable cartridge with multiple lancing elements and testing means
US9427532B2 (en) 2001-06-12 2016-08-30 Sanofi-Aventis Deutschland Gmbh Tissue penetration device
US9795747B2 (en) 2010-06-02 2017-10-24 Sanofi-Aventis Deutschland Gmbh Methods and apparatus for lancet actuation
WO2002100254A2 (en) 2001-06-12 2002-12-19 Pelikan Technologies, Inc. Method and apparatus for lancet launching device integrated onto a blood-sampling cartridge
US7981056B2 (en) 2002-04-19 2011-07-19 Pelikan Technologies, Inc. Methods and apparatus for lancet actuation
JP4149911B2 (en) 2001-06-12 2008-09-17 ペリカン テクノロジーズ インコーポレイテッド Electric lancet actuator
ATE450210T1 (en) 2001-06-12 2009-12-15 Pelikan Technologies Inc SELF-OPTIMIZING LANCET DEVICE WITH ADAPTATION AGENT FOR TIME Fluctuations in SKIN PROPERTIES
US9226699B2 (en) 2002-04-19 2016-01-05 Sanofi-Aventis Deutschland Gmbh Body fluid sampling module with a continuous compression tissue interface surface
US8337419B2 (en) 2002-04-19 2012-12-25 Sanofi-Aventis Deutschland Gmbh Tissue penetration device
US7041068B2 (en) 2001-06-12 2006-05-09 Pelikan Technologies, Inc. Sampling module device and method
CN1257942C (en) * 2001-10-11 2006-05-31 爱科来株式会社 Method of stabilizing oxidation color former
ATE367583T1 (en) * 2002-01-31 2007-08-15 Arkray Inc METHOD FOR QUANTIFYING GLYCOSYLATED PROTEIN USING A REDOX REACTION AND A QUANTIFICATION KIT
US7976476B2 (en) 2002-04-19 2011-07-12 Pelikan Technologies, Inc. Device and method for variable speed lancet
US7547287B2 (en) 2002-04-19 2009-06-16 Pelikan Technologies, Inc. Method and apparatus for penetrating tissue
US7232451B2 (en) 2002-04-19 2007-06-19 Pelikan Technologies, Inc. Method and apparatus for penetrating tissue
US7892185B2 (en) 2002-04-19 2011-02-22 Pelikan Technologies, Inc. Method and apparatus for body fluid sampling and analyte sensing
US8702624B2 (en) 2006-09-29 2014-04-22 Sanofi-Aventis Deutschland Gmbh Analyte measurement device with a single shot actuator
US9314194B2 (en) 2002-04-19 2016-04-19 Sanofi-Aventis Deutschland Gmbh Tissue penetration device
US7491178B2 (en) 2002-04-19 2009-02-17 Pelikan Technologies, Inc. Method and apparatus for penetrating tissue
US7229458B2 (en) 2002-04-19 2007-06-12 Pelikan Technologies, Inc. Method and apparatus for penetrating tissue
US8784335B2 (en) 2002-04-19 2014-07-22 Sanofi-Aventis Deutschland Gmbh Body fluid sampling device with a capacitive sensor
US7331931B2 (en) 2002-04-19 2008-02-19 Pelikan Technologies, Inc. Method and apparatus for penetrating tissue
US7909778B2 (en) 2002-04-19 2011-03-22 Pelikan Technologies, Inc. Method and apparatus for penetrating tissue
US7713214B2 (en) 2002-04-19 2010-05-11 Pelikan Technologies, Inc. Method and apparatus for a multi-use body fluid sampling device with optical analyte sensing
US8360992B2 (en) 2002-04-19 2013-01-29 Sanofi-Aventis Deutschland Gmbh Method and apparatus for penetrating tissue
US7892183B2 (en) 2002-04-19 2011-02-22 Pelikan Technologies, Inc. Method and apparatus for body fluid sampling and analyte sensing
US7901362B2 (en) 2002-04-19 2011-03-08 Pelikan Technologies, Inc. Method and apparatus for penetrating tissue
US9795334B2 (en) 2002-04-19 2017-10-24 Sanofi-Aventis Deutschland Gmbh Method and apparatus for penetrating tissue
US8579831B2 (en) 2002-04-19 2013-11-12 Sanofi-Aventis Deutschland Gmbh Method and apparatus for penetrating tissue
US7297122B2 (en) 2002-04-19 2007-11-20 Pelikan Technologies, Inc. Method and apparatus for penetrating tissue
US7674232B2 (en) 2002-04-19 2010-03-09 Pelikan Technologies, Inc. Method and apparatus for penetrating tissue
US7175642B2 (en) 2002-04-19 2007-02-13 Pelikan Technologies, Inc. Methods and apparatus for lancet actuation
US8221334B2 (en) 2002-04-19 2012-07-17 Sanofi-Aventis Deutschland Gmbh Method and apparatus for penetrating tissue
US8267870B2 (en) 2002-04-19 2012-09-18 Sanofi-Aventis Deutschland Gmbh Method and apparatus for body fluid sampling with hybrid actuation
US9248267B2 (en) 2002-04-19 2016-02-02 Sanofi-Aventis Deustchland Gmbh Tissue penetration device
AU2003235974A1 (en) 2002-06-14 2003-12-31 Arkray, Inc. Method of assay with sulfonic acid compound and nitro compound
US8021855B2 (en) 2002-07-17 2011-09-20 Arkray Inc. Method of decomposing protein with sulfonic acid compound
US7393549B2 (en) 2002-10-23 2008-07-01 Daiichi Pure Chemicals Co., Ltd. Defructosylation method
US8574895B2 (en) 2002-12-30 2013-11-05 Sanofi-Aventis Deutschland Gmbh Method and apparatus using optical techniques to measure analyte levels
EP2096173B1 (en) 2003-05-21 2019-01-30 Asahi Kasei Pharma Corporation Method of measuring glycolated hemoglobin A1C, enzyme to be used therefor and process for producing the same
EP1628567B1 (en) 2003-05-30 2010-08-04 Pelikan Technologies Inc. Method and apparatus for fluid injection
US7850621B2 (en) 2003-06-06 2010-12-14 Pelikan Technologies, Inc. Method and apparatus for body fluid sampling and analyte sensing
WO2006001797A1 (en) 2004-06-14 2006-01-05 Pelikan Technologies, Inc. Low pain penetrating
WO2005033659A2 (en) 2003-09-29 2005-04-14 Pelikan Technologies, Inc. Method and apparatus for an improved sample capture device
EP1680014A4 (en) 2003-10-14 2009-01-21 Pelikan Technologies Inc Method and apparatus for a variable user interface
CN1875115B (en) * 2003-11-19 2012-04-18 积水医疗株式会社 Method for assaying glycosylated protein
KR20060123751A (en) * 2003-11-19 2006-12-04 다이이치 가가쿠 야쿠힝 가부시키가이샤 Method of determining substrate contained in hemoglobin-containing sample
JPWO2005056823A1 (en) 2003-12-12 2007-07-05 アークレイ株式会社 Method for measuring saccharified amines
US7822454B1 (en) 2005-01-03 2010-10-26 Pelikan Technologies, Inc. Fluid sampling device with improved analyte detecting member configuration
EP1706026B1 (en) 2003-12-31 2017-03-01 Sanofi-Aventis Deutschland GmbH Method and apparatus for improving fluidic flow and sample capture
WO2006011062A2 (en) 2004-05-20 2006-02-02 Albatros Technologies Gmbh & Co. Kg Printable hydrogel for biosensors
EP1765194A4 (en) 2004-06-03 2010-09-29 Pelikan Technologies Inc Method and apparatus for a fluid sampling device
US9775553B2 (en) 2004-06-03 2017-10-03 Sanofi-Aventis Deutschland Gmbh Method and apparatus for a fluid sampling device
JP5131955B2 (en) 2004-08-05 2013-01-30 旭化成ファーマ株式会社 Reagent containing protease reaction accelerator and / or dye stabilizer
US8652831B2 (en) 2004-12-30 2014-02-18 Sanofi-Aventis Deutschland Gmbh Method and apparatus for analyte measurement test time
US7361513B2 (en) * 2005-04-08 2008-04-22 Streck, Inc. Cellular controls for glycated hemoglobin Hb A1c
CN101171342B (en) * 2005-05-06 2011-11-16 爱科来株式会社 Protein cleavage method and use thereof
JP5204483B2 (en) * 2005-07-19 2013-06-05 キッコーマン株式会社 Method and kit for measuring glycated protein
CN101297044B (en) * 2005-10-27 2012-12-12 爱科来株式会社 Albumin-denaturing agent
CN101484809B (en) 2006-07-25 2013-12-04 通用原子公司 Methods for assaying percentage of glycated hemoglobin
US7943385B2 (en) 2006-07-25 2011-05-17 General Atomics Methods for assaying percentage of glycated hemoglobin
JP5261180B2 (en) * 2006-08-11 2013-08-14 アークレイ株式会社 Postprandial hyperglycemia marker, measuring method thereof and use thereof
JP4437216B2 (en) 2007-01-30 2010-03-24 アークレイ株式会社 Method for detecting phenothiazine-derivative dye and color former used therefor
EP2116611B1 (en) * 2007-01-30 2013-08-14 ARKRAY, Inc. Measurement method for hba1c
JP4697809B2 (en) 2007-02-22 2011-06-08 旭化成ファーマ株式会社 Method for stabilizing leuco dyes
EP2210113B1 (en) * 2007-11-20 2015-05-27 Siemens Healthcare Diagnostics Inc. Methods for the detection of glycated hemoglobin
JPWO2009116575A1 (en) 2008-03-19 2011-07-21 アークレイ株式会社 Color former stabilizer and use thereof
WO2009126900A1 (en) 2008-04-11 2009-10-15 Pelikan Technologies, Inc. Method and apparatus for analyte detecting device
US8673646B2 (en) * 2008-05-13 2014-03-18 General Atomics Electrochemical biosensor for direct determination of percentage of glycated hemoglobin
JP5438020B2 (en) 2008-10-10 2014-03-12 東洋紡株式会社 Novel fructosyl valyl histidine oxidase activity protein, its modification, and use thereof
US9375169B2 (en) 2009-01-30 2016-06-28 Sanofi-Aventis Deutschland Gmbh Cam drive for managing disposable penetrating member actions with a single motor and motor and control system
US8128545B2 (en) * 2009-05-07 2012-03-06 Cmd Corporation Machine for securing a closure system onto a discrete pouch
EP2281900A1 (en) 2009-08-03 2011-02-09 Roche Diagnostics GmbH Fructosyl peptidyl oxidase and sensor for assaying a glycated protein
US8965476B2 (en) 2010-04-16 2015-02-24 Sanofi-Aventis Deutschland Gmbh Tissue penetration device
EP2604699B1 (en) * 2010-08-11 2017-10-04 Kyowa Medex CO., LTD. Method for measuring glycated hemoglobin
JP2012108062A (en) * 2010-11-19 2012-06-07 Hitachi High-Technologies Corp Autoanalyzer
WO2013096856A1 (en) 2011-12-22 2013-06-27 Massachusetts Institute Of Technology Raman spectroscopy for detection of glycated analytes
JP5858945B2 (en) * 2012-03-15 2016-02-10 アークレイ株式会社 Measuring method using enzyme
JP5938713B2 (en) * 2013-03-11 2016-06-22 彰 三池 High-sensitivity measurement method and reagent for hemoglobin
EP3760717A1 (en) 2013-08-09 2021-01-06 Kikkoman Corporation Amadoriase and method for producing the same, agent for improving surfactant resistance of amadoriase and composition for measuring hba1c using the same
EP3216865B1 (en) 2014-11-07 2020-09-30 Kikkoman Corporation Amadoriase having enhanced anionic-surfactant tolerance
CN106596209B (en) * 2015-10-14 2020-05-12 杭州量康科技有限公司 Dry blood sample pretreatment and detection method
CN109073646A (en) * 2016-05-13 2018-12-21 荣研化学株式会社 Seek the determinand method of proportion, program, storage medium and device in comparison
CN110520728B (en) 2017-03-03 2022-12-06 聚合物技术系统公司 Systems and methods for enzymatic A1C detection and quantification
US11703513B2 (en) 2017-08-07 2023-07-18 Polymer Technology Systems, Inc. Systems and methods for enzymatic A1C detection and quantification
CN109680036A (en) 2017-10-02 2019-04-26 爱科来株式会社 The measurement of glycated proteins
WO2019143637A1 (en) * 2018-01-18 2019-07-25 Cellics Therapeutics, Inc. Methods and compositions for quantifying hemoglobin
CN113009021B (en) * 2018-12-29 2023-04-14 江山德瑞医疗科技有限公司 Application method of additive in measurement of glycosylated hemoglobin
WO2021016380A1 (en) * 2019-07-22 2021-01-28 Ortho-Clinical Diagnostics, Inc. Glycated hemoglobin measurement

Citations (22)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US3914436A (en) * 1972-12-11 1975-10-21 Noda Inst For Scientific Res Process for manufacturing soy sauce using enzymatic preparation(s)
JPH0288568A (en) 1988-09-27 1990-03-28 Idemitsu Kosan Co Ltd Fluorine-containing epoxide and production thereof
JPH02195900A (en) 1989-01-25 1990-08-02 Sanyo Chem Ind Ltd Determination of glycoprotein and determination reagent
EP0526150A1 (en) 1991-07-29 1993-02-03 GENZYME LIMITED (formerly known as Genzyme (UK) Ltd) Assay
EP0576838A2 (en) 1992-06-05 1994-01-05 Nakano Vinegar Co., Ltd. Fructosylamine deglycase, method of producing it, and method of quantitative determination of amadori compounds using the enzyme
EP0598329A2 (en) 1992-11-17 1994-05-25 Boehringer Mannheim Gmbh Simultaneous determination of HbA1c and haemoglobin variants with a HbA1c analog glycation
EP0678576A2 (en) 1994-03-03 1995-10-25 Kyoto Daiichi Kagaku Co., Ltd. Fructosyl amino acid oxidase and process for producing the same
EP0693559A1 (en) 1994-07-18 1996-01-24 Roche Diagnostics GmbH Method for quantitative determination of glycated proteins
JPH08208492A (en) 1994-01-11 1996-08-13 Nagase & Co Ltd Separation of blood cell
WO1997013872A1 (en) 1995-10-12 1997-04-17 Kyoto Daiichi Kagaku Co., Ltd. Method and assaying amodori compounds
US5712138A (en) * 1994-10-05 1998-01-27 Kyoto Daiichi Kagaku Co., Ltd. Fructosyl amino acid oxidase
EP0864647A1 (en) 1995-11-30 1998-09-16 Kabushiki Kaisha Kyoto Daiichi Kagaku Fructosyl amino acid oxidase, process for producing the same, and method of assaying amadori compounds using the enzyme
WO1998048043A1 (en) 1997-04-24 1998-10-29 Kyoto Daiichi Kagaku Co., Ltd. Method for enzymatically assaying saccharification protein
EP0919632A2 (en) 1997-11-26 1999-06-02 Kyoto Daiichi Kagaku Co., Ltd. Method for the determination of glycosylated proteins
EP1002874A2 (en) 1998-11-17 2000-05-24 Kyoto Daiichi Kagaku Co., Ltd. Redox reactions for analyte determination using tetrazolium compounds
JP2000300294A (en) 1999-04-16 2000-10-31 Dai Ichi Pure Chem Co Ltd DETERMINATION OF HEMOGLOBIN Alc
CN1280241A (en) 1999-07-07 2001-01-17 韩国科学技术研究院 Method and device for controlling noise of exhaust gas
JP2001054398A (en) 1999-08-18 2001-02-27 Asahi Chem Ind Co Ltd Selective fragmentation of protein
JP2001095598A (en) 1999-10-01 2001-04-10 Kikkoman Corp Method for measuring glucosylated protein
JP2001204495A (en) 2000-01-28 2001-07-31 Asahi Kasei Corp Method for assaying proportion of saccharified protein
US6790665B2 (en) * 2000-09-28 2004-09-14 Arkray, Inc. Method of quantifying hemoglobin and method of measuring glycation ratio of hemoglobin
US6825016B1 (en) * 1999-04-12 2004-11-30 Arkray, Inc. α-glycated amino acid releasing enzyme

Family Cites Families (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US4465774A (en) * 1981-07-16 1984-08-14 Sherwood Medical Company Standard or control material for glysocylated or total hemoglobin determination
CA2591834C (en) * 1992-03-04 2009-04-28 Abbott Laboratories Determination of glycated hemoglobin by fluorescence quenching

Patent Citations (33)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US3914436A (en) * 1972-12-11 1975-10-21 Noda Inst For Scientific Res Process for manufacturing soy sauce using enzymatic preparation(s)
JPH0288568A (en) 1988-09-27 1990-03-28 Idemitsu Kosan Co Ltd Fluorine-containing epoxide and production thereof
JPH02195900A (en) 1989-01-25 1990-08-02 Sanyo Chem Ind Ltd Determination of glycoprotein and determination reagent
EP0526150A1 (en) 1991-07-29 1993-02-03 GENZYME LIMITED (formerly known as Genzyme (UK) Ltd) Assay
US5370990A (en) * 1991-07-29 1994-12-06 Genzyme Corporation Diagnostic assay for fructosamines
EP0576838A2 (en) 1992-06-05 1994-01-05 Nakano Vinegar Co., Ltd. Fructosylamine deglycase, method of producing it, and method of quantitative determination of amadori compounds using the enzyme
US5387109A (en) * 1992-06-05 1995-02-07 Nakano Vinegar Co., Ltd. Fructosylamine deglycase and a method of producing it
EP0598329A2 (en) 1992-11-17 1994-05-25 Boehringer Mannheim Gmbh Simultaneous determination of HbA1c and haemoglobin variants with a HbA1c analog glycation
JPH08208492A (en) 1994-01-11 1996-08-13 Nagase & Co Ltd Separation of blood cell
EP0678576A2 (en) 1994-03-03 1995-10-25 Kyoto Daiichi Kagaku Co., Ltd. Fructosyl amino acid oxidase and process for producing the same
EP0693559A1 (en) 1994-07-18 1996-01-24 Roche Diagnostics GmbH Method for quantitative determination of glycated proteins
US5631140A (en) * 1994-07-18 1997-05-20 Boehringer Mannheim Gmbh Method for the quantitative determination of glycated proteins
US5712138A (en) * 1994-10-05 1998-01-27 Kyoto Daiichi Kagaku Co., Ltd. Fructosyl amino acid oxidase
WO1997013872A1 (en) 1995-10-12 1997-04-17 Kyoto Daiichi Kagaku Co., Ltd. Method and assaying amodori compounds
EP0864647A1 (en) 1995-11-30 1998-09-16 Kabushiki Kaisha Kyoto Daiichi Kagaku Fructosyl amino acid oxidase, process for producing the same, and method of assaying amadori compounds using the enzyme
US6033867A (en) * 1995-11-30 2000-03-07 Kyoto Daiichi Kagaku Co., Ltd. Fructosyl amino acid oxidase, process for producing the same, and method of assaying amadori compounds using the enzyme
WO1998048043A1 (en) 1997-04-24 1998-10-29 Kyoto Daiichi Kagaku Co., Ltd. Method for enzymatically assaying saccharification protein
EP0921198A1 (en) 1997-04-24 1999-06-09 Kyoto Daiichi Kagaku Co., Ltd. Method for enzymatically assaying saccharification protein
EP0919632A2 (en) 1997-11-26 1999-06-02 Kyoto Daiichi Kagaku Co., Ltd. Method for the determination of glycosylated proteins
US6352835B1 (en) * 1998-11-17 2002-03-05 Kyoto Daiichi Kagaku Co. Ltd. Method of measuring substance in sample using a redox reaction
EP1002874A2 (en) 1998-11-17 2000-05-24 Kyoto Daiichi Kagaku Co., Ltd. Redox reactions for analyte determination using tetrazolium compounds
US20020025546A1 (en) * 1998-11-17 2002-02-28 Kyoto Daiichi Kagaku Co., Ltd. Method of measuring substance in sample using a redox reaction
US20040247587A1 (en) * 1999-04-12 2004-12-09 Arkray, Inc. Alpha-glycated amino acid releasing enzyme
US6825016B1 (en) * 1999-04-12 2004-11-30 Arkray, Inc. α-glycated amino acid releasing enzyme
JP2000300294A (en) 1999-04-16 2000-10-31 Dai Ichi Pure Chem Co Ltd DETERMINATION OF HEMOGLOBIN Alc
CN1280241A (en) 1999-07-07 2001-01-17 韩国科学技术研究院 Method and device for controlling noise of exhaust gas
JP2001054398A (en) 1999-08-18 2001-02-27 Asahi Chem Ind Co Ltd Selective fragmentation of protein
EP1223224A1 (en) 1999-10-01 2002-07-17 Kikkoman Corporation Method of assaying glycoprotein
WO2001025475A1 (en) 1999-10-01 2001-04-12 Kikkoman Corporation Method of assaying glycoprotein
JP2001095598A (en) 1999-10-01 2001-04-10 Kikkoman Corp Method for measuring glucosylated protein
US7070948B1 (en) * 1999-10-01 2006-07-04 Kikkoman Corporation Method for assaying glycated protein
JP2001204495A (en) 2000-01-28 2001-07-31 Asahi Kasei Corp Method for assaying proportion of saccharified protein
US6790665B2 (en) * 2000-09-28 2004-09-14 Arkray, Inc. Method of quantifying hemoglobin and method of measuring glycation ratio of hemoglobin

Non-Patent Citations (31)

* Cited by examiner, † Cited by third party
Title
Ajabnoor et al. "Bacillus subtilis aminopeptidase: Specificity toward amino acid amides, dipeptides and oligopeptides" Arch Biochem Biophys 202(2) 540-545 (1980). *
Barrett et al., "Nomenclature: protease, proteinase and peptidase", Biochemical Journal 231, 935 (1986).
Barrett et al., "Nomenclature: protease, proteinase and peptidase", Biochemical Journal Letters; 237:935 (1986).
Biozym http://www.biozym.de/datasheets/bromelain.php [accessed Apr. 13, 2015]. *
Collins Dictionary of Biology, Second Edition (W.G. Hale, J.P. Margham & V.A. Saunders) 474, 512 et al. (1995).
Dorland's Illustrated Medical Dictionary, 29th Edition, W.B. Saunders Company, 595, 1095, 1348 et al. (2000).
EPO Search Report for PCT/JP01/06064 provided by Applicant.
European Search Opinion issued in European Patent Application No. 10010191.4 dated Apr. 2, 2014.
European Search Report issued in European Patent Application No. 10010191 dated Aug. 2, 2011.
European Search Report issued in related European Patent Application No. 01947995 dated Mar. 26, 2006.
Experimental Data Certificate submitted in corresponding European Patent Application No. 01947995.5 dated Jun. 16, 2008.
Extended European Search Report issued in corresponding European Patent Application No. 15174619.5 dated Sep. 24, 2015.
Filing of Opposition Proceedings in European Patent No. 1304385 dated Sep. 28, 2011.
Gil H, Mata-Segreda J, Schowen R. Acta Cient. Venez. (1997) 42, 16-23 Effect of non-enzymqatic glycosylation on reactivity in proteolysis. Article in Spanish. *
Iberg et al. "Nonenzymatic Glycosylation of Albumin in Vivo Identification of Multiple Glycosylated Sites" J. Biol Chem. 261: 13542-13545 (1986). *
International Preliminary Examination Report issued in PCT/JP01/06064 dated Apr. 12, 2002.
International Search Report issued in related PCT/JP2001/06064 dated Sep. 18, 2001.
Japanese Office Action issued in related Japanese Patent Application No. 2002-512410 mailed May 29, 2006.
Letter declaration withdrawal of opposition in European Patent No. 1304385 dated Nov. 17, 2011.
Office Action issued in related Japanese Patent Application No. 2002-512410 dated Jan. 9, 2007.
Patentee's Reply to Notice of Opposition Proceedings in European Patent No. 1304385 dated May 18, 2012.
Rice et al. "The papain digestion of native, denatured and 'stabilized' human serum albumin" J. Biol Chem. 158: 609-617 (1945). *
Rivett et al., "Proteolytic Enzymes and Inhibitors", "Protease Nomenclature, classification, structure and specificity", Essays in Biochemistry, 25:60-61 (1990).
Rufo et al., "Isolation and Characterization of a Novel Extracellular Metalloprotease from Bacillus subtilis"Journal of Bacteriology, Feb. 1990, vol. 172, No. 2, pp. 1019-1023. *
Sakurabayashi, et al., "New Enzymatic Assay for Glycohemoglobin", Clinical Chemistry, American Association for Clinical Chemistry, Washington. DC 49:2, 269-274 (2003).
Shapiro et al. "Sites of Nonenzymatic Glycosylation of Human Hemoglobin A" J Biol Chem 255(7): 3120-3127 (1980). *
Submission of publications to Commissioner of Patents in Japanese Patent Application No. 2007-038171 dated Jan. 16, 2009 (translation only).
Submission of publications to Commissioner of Patents in Japanese Patent Application No. 2007-038171 dated Jul. 31, 2008 (translation only).
Submission of publications to Commissioner of Patents in Japanese Patent Application No. 2007-038171 dated Jun. 4, 2008 (translation only).
Termination of opposition proceedings of European Patent No. 1304385 dated Jan. 18, 2013.
Yoshida et al., "Primary structures of fungal fructosyl amino acid oxidases and their application to the measurement of glycated proteins" Eur. J. Biochem. 242, 499-505 (1996). *

Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US10006923B2 (en) 2013-07-09 2018-06-26 Kyowa Medex Co., Ltd. Method for measuring glycated hemoglobin

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