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稳定同位素标记的内标总能校正分析物响应吗?关于测定人血浆中卡维地洛对映体的液相色谱/串联质谱法的基质效应研究。

Does a stable isotopically labeled internal standard always correct analyte response? A matrix effect study on a LC/MS/MS method for the determination of carvedilol enantiomers in human plasma.

作者信息

Wang Sherry, Cyronak Matthew, Yang Eric

机构信息

Worldwide Bioanalysis, Drug Metabolism and Pharmacokinetics, GlaxoSmithKline Pharm 709 Swedeland Rd., King of Prussia, PA 19406, USA.

出版信息

J Pharm Biomed Anal. 2007 Jan 17;43(2):701-7. doi: 10.1016/j.jpba.2006.08.010. Epub 2006 Sep 7.

DOI:10.1016/j.jpba.2006.08.010
PMID:16959461
Abstract

A stable isotopically labeled (SIL) analogue is believed to be the most appropriate internal standard in a quantitative bioanalytical liquid chromatography/tandem mass spectrometry (LC/MS/MS) assay. It is assumed that a SIL internal standard always compensates for variability in chemical derivatization, sample extraction and LC/MS/MS analysis due to its nearly identical chemical and physical properties to the unlabeled analyte. Hence, the analyte to internal standard peak area ratio should be constant despite any variations in sample processing or analysis. However, in our laboratories, a deuterium labeled internal standard of carvedilol demonstrated an unexpected behavior-the analyte to internal standard peak area ratio changed with two specific lots of commercially supplied human plasma. Several experiments, including dilution of the extract with LC mobile phase and post-column infusion of the carvedilol solution followed by the injection of extracted blank plasma, have indicated that a high level of matrix suppression affected the ionization of the carvedilol-S enantiomer and its deuterated internal standard differently in these two lots of plasma. For the first time, it was clearly demonstrated that a slight difference in retention time between the analyte and the SIL internal standard, caused by deuterium isotope effect, has resulted in a different degree of ion suppression between these two analogues. This difference was significant enough to change the analyte to internal standard peak area ratio and affect the accuracy of the method.

摘要

稳定同位素标记(SIL)类似物被认为是定量生物分析液相色谱/串联质谱(LC/MS/MS)测定中最合适的内标物。假定SIL内标物因其与未标记分析物几乎相同的化学和物理性质,总能补偿化学衍生化、样品萃取及LC/MS/MS分析过程中的变异性。因此,尽管样品处理或分析存在任何变化,分析物与内标物的峰面积比应保持恒定。然而,在我们实验室中,卡维地洛的氘代内标物表现出意外行为——分析物与内标物的峰面积比随两批市售人血浆而变化。包括用LC流动相稀释提取物以及在柱后注入卡维地洛溶液随后进样提取的空白血浆在内的多项实验表明,在这两批血浆中,高水平的基质抑制对卡维地洛-S对映体及其氘代内标物的电离影响不同。首次清楚地证明,由氘同位素效应导致的分析物与SIL内标物保留时间的细微差异,造成了这两种类似物之间不同程度的离子抑制。这种差异足以改变分析物与内标物的峰面积比并影响方法的准确性。

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