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液相色谱-串联质谱法用于定量分析包括烯醚类在内的溶血磷脂的改良方法。

Improved method for the quantification of lysophospholipids including enol ether species by liquid chromatography-tandem mass spectrometry.

机构信息

Department of Chemistry, University of Washington, Seattle, WA, USA.

出版信息

J Lipid Res. 2010 Feb;51(2):440-7. doi: 10.1194/jlr.D000885. Epub 2009 Aug 29.

Abstract

LC/ESI-MS/MS has been previously demonstrated to be a powerful method to detect and quantify molecular species of glycerophospholipids including lysophospholipids. In this study, we provide an improved pre-mass spectrometry lipid extraction procedure that avoids the acid-catalyzed decomposition of plasmenyl phospholipids that is problematic with previously reported methods. We show that the use of lysophospholipid internal standards with perdeuterated fatty acyl chains avoids isobar problems associated with the use of internal standards containing odd carbon number fatty acyl chains. We also show that LC prior to MS is required to avoid numerous problems associated with isobars and with MS in-source decomposition of lysophosphatidylserine. The reported method of using normal phase chromatography/ESI-MS is used to quantify lysophospholipids in serum and to quantify lysophospholipids produced in mammalian cells by human group X secreted phospholipase A(2). The latter shows that group X phospholipase A(2) added exogenously to cells generates a different set of lysophospholipids compared with enzyme produced endogenously in cells, which supports earlier studies showing that this phospholipase A(2) can act on cell membranes prior to externalization from cells.

摘要

LC/ESI-MS/MS 先前已被证明是一种强大的方法,可用于检测和定量甘油磷脂的分子种类,包括溶血磷脂。在这项研究中,我们提供了一种改进的质谱前脂质提取程序,避免了先前报道的方法中存在的酸催化分解溶血磷脂的问题。我们表明,使用具有全氘化脂肪酸链的溶血磷脂内标可以避免与使用含奇数碳数脂肪酸链的内标相关的同量异位问题。我们还表明,在 MS 之前进行 LC 是必需的,以避免与同量异位和 MS 源内分解溶血磷脂丝氨酸相关的许多问题。报告的使用正相色谱/ESI-MS 的方法用于定量血清中的溶血磷脂,并定量人组 X 分泌型磷脂酶 A2(secreted phospholipase A2)产生的哺乳动物细胞中的溶血磷脂。后者表明,与细胞内产生的内源性酶相比,外加至细胞的组 X 磷脂酶 A2 产生了一组不同的溶血磷脂,这支持了早期的研究,表明该磷脂酶 A2 可以在细胞外化之前作用于细胞膜。

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