Heterologous expression of human cytochrome P450 (CYP) 2C19 in Escherichia coli and establishment of RP‐HPLC method to serve as activity marker

化学 色谱法 高效液相色谱法 大肠杆菌 异源表达 重组DNA 吸光度 检出限 生物化学 基因
作者
Yan Pan,Joon Wah Mak,Chin Eng Ong
出处
期刊:Biomedical Chromatography [Wiley]
卷期号:27 (7): 859-865 被引量:9
标识
DOI:10.1002/bmc.2872
摘要

ABSTRACT In this study, a simple and reliable reverse‐phase high‐performance liquid chromatography (RP‐HPLC) method was established and validated to analyze S ‐mephenytoin 4‐hydroxylase activity of a recombinant CYP2C19 system. This system was obtained by co‐expressing CYP2C19 and NADPH‐CYP oxidoreductase (OxR) proteins in Escherichia coli ( E . coli ) cells. In addition to RP‐HPLC, the expressed proteins were evaluated by immunoblotting and reduced CO difference spectral scanning. The RP‐HPLC assay showed good linearity ( r 2 = 1.00) with 4‐hydroxymephenytoin concentration from 0.100 to 50.0 μ m and the limit of detection was 5.00 × 10 −2 μ m . Intraday and interday precisions determined were from 1.90 to 8.19% and from 2.20 to 14.9%, respectively. Recovery and accuracy of the assay were from 83.5 to 85.8% and from 95.0 to 105%. Enzyme kinetic parameters ( K m , V max and K i ) were comparable to reported values. The presence of CYP2C19 in bacterial membranes was confirmed by immunoblotting and the characteristic absorbance peak at 450 nm was determined in the reduced CO difference spectral assay. Moreover, the activity level of co‐expressed OxR was found to be comparable to that of the literature. As a conclusion, the procedures described here have generated catalytically active CYP2C19 and the RP‐HPLC assay developed is able to serve as CYP2C19 activity marker for pharmacokinetic drug interaction study in vitro . Copyright © 2013 John Wiley & Sons, Ltd.
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