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使用毛细管电泳分析血管紧张素转换酶抑制剂中脯氨酸肽键的异构体组成。

Analysis of the isomeric composition of the proline peptide bond in an angiotensin-converting enzyme inhibitor using capillary electrophoresis.

作者信息

Stellwagen Earle, Ledger Robin

机构信息

Department of Biochemistry, University of Iowa, Iowa City, IA 52242, USA.

出版信息

Anal Biochem. 2003 Oct 15;321(2):167-73. doi: 10.1016/s0003-2697(03)00437-8.

DOI:10.1016/s0003-2697(03)00437-8
PMID:14511680
Abstract

The cis and trans isomeric composition of a proline peptide bond can be determined by routine free-solution capillary electrophoresis measurements provided that one isomeric form is preferentially stabilized by a dissociable ionic group. This capability is illustrated using the angiotensin converting enzyme (ACE) inhibitor (S)-1-N-[1-(ethoxycarbonyl)-3-phenylpropyl]-L-ala-L-pro, which has the trade name enalapril. Electropherograms indicate that the two isomeric forms of enalapril can be separated with baseline resolution at 15 degrees C using capillary buffers having pH values in the dissociation ranges of the enalapril carboxyl group, pK(cis) and pK(trans) of 2.6 and 3.1, and of the enalapril amine group, pK(cis) and pK(trans) of 5.9 and 5.6. Such baseline resolution indicates that the isomeric composition does not change during analysis, facilitating measurement of the isomer composition of a sample prior to its injection into the capillary. Thus the effect of pH, ionic strength, or an aprotic solvent on the isomeric composition of enalapril can be measured under uniform analytical conditions. The trans isomer composition changes from 68% in the cationic form, pH <2, to 50% in the isoelectric form, pH approximately 4.5, to 60% in the anionic form, pH >7. Addition of salt to the isoelectric form or addition of an aprotic solvent to any form prior to analysis increases the trans isomer composition. Similar analyses can be made using the alternative ACE inhibitors captopril and enalaprilat.

摘要

只要一种异构体形式能被可解离的离子基团优先稳定,脯氨酸肽键的顺式和反式异构体组成就可以通过常规的自由溶液毛细管电泳测量来确定。使用商品名为依那普利的血管紧张素转换酶(ACE)抑制剂(S)-1-N-[1-(乙氧羰基)-3-苯基丙基]-L-丙氨酰-L-脯氨酸,说明了这种能力。电泳图表明,在15℃下,使用pH值处于依那普利羧基解离范围(顺式pK为2.6,反式pK为3.1)以及依那普利胺基解离范围(顺式pK为5.9,反式pK为5.6)的毛细管缓冲液,依那普利的两种异构体形式可以实现基线分离。这种基线分离表明异构体组成在分析过程中不会改变,便于在将样品注入毛细管之前测量其异构体组成。因此,可以在统一的分析条件下测量pH、离子强度或非质子溶剂对依那普利异构体组成的影响。反式异构体组成从阳离子形式(pH <2)下的68%,变为等电形式(pH约4.5)下的50%,再变为阴离子形式(pH >7)下的60%。在等电形式中加入盐或在分析前向任何形式中加入非质子溶剂会增加反式异构体组成。使用替代的ACE抑制剂卡托普利和依那普利拉可以进行类似的分析。

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