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一种快速定量的 LC-MS/MS 方法来分析神经酰胺。

A rapid and quantitative LC-MS/MS method to profile sphingolipids.

机构信息

Institute for Clinical Chemistry and Laboratory Medicine, University of Regensburg, Regensburg, Germany.

出版信息

J Lipid Res. 2010 Jul;51(7):2001-11. doi: 10.1194/jlr.D005322. Epub 2010 Mar 12.

Abstract

Sphingolipids comprise a highly diverse and complex class of molecules that serve not only as structural components of membranes but also as signaling molecules. To understand the differential role of sphingolipids in a regulatory network, it is important to use specific and quantitative methods. We developed a novel LC-MS/MS method for the rapid, simultaneous quantification of sphingolipid metabolites, including sphingosine, sphinganine, phyto-sphingosine, di- and trimethyl-sphingosine, sphingosylphosphorylcholine, hexosylceramide, lactosylceramide, ceramide-1-phosphate, and dihydroceramide-1-phosphate. Appropriate internal standards (ISs) were added prior to lipid extraction. In contrast to most published methods based on reversed phase chromatography, we used hydrophilic interaction liquid chromatography and achieved good peak shapes, a short analysis time of 4.5 min, and, most importantly, coelution of analytes and their respective ISs. To avoid an overestimation of species concentrations, peak areas were corrected regarding isotopic overlap where necessary. Quantification was achieved by standard addition of naturally occurring sphingolipid species to the sample matrix. The method showed excellent precision, accuracy, detection limits, and robustness. As an example, sphingolipid species were quantified in fibroblasts treated with myriocin or sphingosine-kinase inhibitor. In summary, this method represents a valuable tool to evaluate the role of sphingolipids in the regulation of cell functions.

摘要

鞘脂类化合物包括高度多样化和复杂的分子类别,它们不仅作为膜的结构成分,而且还作为信号分子发挥作用。为了了解鞘脂类在调控网络中的差异作用,使用特定和定量的方法非常重要。我们开发了一种新的 LC-MS/MS 方法,用于快速、同时定量鞘脂代谢物,包括神经鞘氨醇、鞘氨醇、植物鞘氨醇、二甲基和三甲基神经鞘氨醇、神经鞘氨醇磷酸胆碱、己糖神经酰胺、乳糖神经酰胺、神经酰胺-1-磷酸和二氢神经酰胺-1-磷酸。在进行脂质提取之前,添加适当的内标(IS)。与大多数基于反相色谱的已发表方法不同,我们使用亲水相互作用液相色谱,实现了良好的峰形,分析时间短至 4.5 分钟,最重要的是,分析物及其各自的 IS 共洗脱。为了避免对物种浓度的高估,必要时根据同位素重叠校正峰面积。通过向样品基质中添加天然存在的鞘脂类物质进行标准添加来实现定量。该方法显示出出色的精密度、准确性、检测限和稳健性。例如,对经霉菌酸或鞘氨醇激酶抑制剂处理的成纤维细胞中的鞘脂类物质进行了定量。总之,该方法是评估鞘脂类在调节细胞功能中的作用的有价值工具。

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