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在有和没有苯基丁氮酮的情况下,对人血清白蛋白上的(R)-和(S)-华法林进行蛋白质结合高效前沿分析

Protein-binding high-performance frontal analysis of (R)- and (S)-warfarin on HSA with and without phenylbutazone.

作者信息

He J, Shibukawa A, Tokunaga S, Nakagawa T

机构信息

Faculty of Pharmaceutical Sciences, Kyoto University, Sakyo-ku, Japan.

出版信息

J Pharm Sci. 1997 Jan;86(1):120-5. doi: 10.1021/js9600134.

DOI:10.1021/js9600134
PMID:9002471
Abstract

Applicability of high-performance frontal analysis (HPFA) to the stereoselective study of drug-drug interaction upon plasma protein binding has been investigated. Racemic warfarin and phenylbutazone were used as model drugs. An on-line HPFA/HPLC system consisting of a HPFA column (diol-silica column), an extraction column, and a chiral separation column was developed, and human serum albumin solution containing racemic warfarin and/or phenylbutazone was injected directly to the HPFA column. When the injection volume was large enough, the binding equilibrium in the sample solution was reproduced in the column, and consequently a plateau region appeared on the chromatogram. This plateau region contains unbound drug(s). A given volume of eluent in the plateau part was transferred into the extraction column by column-switching. The concentrated drug(s) was then transferred to the chiral separation column to determine the unbound concentrations of the enantiomers and/or the competitor. The results agreed with those obtained by a conventional ultrafiltration-HPLC method. The influence of phenylbutazone upon the protein binding of warfarin is enantioselective. In warfarin and human serum albumin mixed solution, the unbound concentration of (R)-warfarin was 1.22 times higher than that of the S-isomer. By addition of phenylbutazone, the unbound concentration of (S)-warfarin increased more than that of (R)-warfarin, resulting in the reversed enantioselectivity, i.e., the unbound concentration of (S)-warfarin became 1.19 times larger than that of (R)-warfarin. The present method was also applicable to human plasma samples.

摘要

研究了高效前沿分析(HPFA)在血浆蛋白结合药物相互作用立体选择性研究中的适用性。使用外消旋华法林和保泰松作为模型药物。开发了一种由HPFA柱(二醇硅胶柱)、萃取柱和手性分离柱组成的在线HPFA/HPLC系统,并将含有外消旋华法林和/或保泰松的人血清白蛋白溶液直接注入HPFA柱。当进样体积足够大时,柱内重现了样品溶液中的结合平衡,因此色谱图上出现了一个平台区。该平台区包含未结合的药物。通过柱切换将平台部分给定体积的洗脱液转移到萃取柱中。然后将浓缩的药物转移到手性分离柱中,以测定对映体和/或竞争剂的未结合浓度。结果与传统超滤-HPLC方法得到的结果一致。保泰松对华法林蛋白结合的影响具有对映体选择性。在华法林与人血清白蛋白混合溶液中,(R)-华法林的未结合浓度比S-异构体高1.22倍。加入保泰松后,(S)-华法林的未结合浓度比(R)-华法林增加得更多,导致对映体选择性反转,即(S)-华法林的未结合浓度比(R)-华法林高1.19倍。本方法也适用于人血浆样品。

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