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Enzymes used for the determination of HbA1C
Authors:Hirokawa Kozo  Nakamura Kazuo  Kajiyama Naoki
Affiliation:Research and Development Division, Kikkoman Corporation, 399 Noda, Noda-city, Chiba Pref. 278-0037, Japan. khirokawa@mail.kikkoman.co.jp
Abstract:To develop an enzymatic measurement of HbA(1C), two key enzymes, i.e., fructosyl peptide oxidase and Aspergillus protease were characterized. Fructosyl peptide oxidase from Eupenicillium terrenum was a flavoenzyme that could catalyze the oxidation of N-(1-deoxyfructosyl)-Val-His. The enzyme showed high specificity toward alpha-glycated molecules, therefore it seemed suitable for the HbA(1C) assay. Since high levels of FPOX expression seemed toxic to host cells, we applied a gene expression system using a bacteriophage vector and achieved high levels of expression in Escherichia coli. Next, we found that Aspergillus protease was able to digest N-(1-deoxyfructosyl)-hexapeptide, a glycated peptide that was released from the beta-chain of HbA(1C) by Glu-C endoproteinase. We showed that the N-(1-deoxyfructosyl)-Val-His released from N-(1-deoxyfructosyl)-hexapeptide by Aspergillus protease could be assayed enzymatically using fructosyl peptide oxidase, therefore these enzymes could be applied to the enzymatic measurement of HbA(1C).
Keywords:Hemoglobin A1C    Fructosyl peptide oxidase    Fructosyl amino acid oxidase    Amadoriase    Fructosyl-hexapeptide    Enzymatic measurement of HbA1C    Eupenicillium terrenum
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