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采用气相离子化学对脑苷脂和神经酰胺糖脂进行深入的结构特征描述和定量分析。

In-Depth Structural Characterization and Quantification of Cerebrosides and Glycosphingosines with Gas-Phase Ion Chemistry.

机构信息

Department of Chemistry Purdue University 560 Oval Drive West Lafayette, Indiana 47907, United States.

出版信息

Anal Chem. 2021 May 18;93(19):7332-7340. doi: 10.1021/acs.analchem.1c01021. Epub 2021 May 6.

DOI:10.1021/acs.analchem.1c01021
PMID:33957046
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC8579694/
Abstract

Cerebrosides (n-HexCer) and glycosphingosines (n-HexSph) constitute two sphingolipid subclasses. Both are comprised of a monosaccharide headgroup (glucose or galactose in mammalian cells) linked via either an α- or β-glycosidic linkage to the sphingoid backbone (n = α or β, depending upon the nature of the linkage to the anomeric carbon of the sugar). Cerebrosides have an additional amide-bonded fatty acyl chain linked to the sphingoid backbone. While differentiating the multiple isomers (i.e. glucose vs galactose, α- vs β-linkage) is difficult, it is crucial for understanding their specific biological roles in health and disease states. Shotgun tandem mass spectrometry has been a powerful tool in both lipidomics and glycomics analysis but is often limited in its ability to distinguish isomeric species. This work describes a new strategy combining shotgun tandem mass spectrometry with gas-phase ion chemistry to achieve both differentiation and quantification of isomeric cerebrosides and glycosphingosines. Briefly, deprotonated cerebrosides, [n-HexCer-H], or glycosphingosines, [n-HexSph-H], are reacted with terpyridine (Terpy) magnesium complex dications, [Mg(Terpy)], in the gas phase to produce a charge-inverted complex cation, [n-HexCer-H+MgTerpy] or [n-HexSph-H+MgTerpy]. The collision-induced dissociation (CID) of the charge-inverted complex cations leads to significant spectral differences between the two groups of isomers, α-GalCer, β-GlcCer, and β-GalCer for cerebrosides and α-GlcSph, α-GalSph, β-GlcSph, and β-GalSph for glycosphingosines, which allows for isomer distinction. Moreover, we describe a quantification strategy with the normalized percent area extracted from selected diagnostic ions that quantify either three isomeric cerebroside or four isomeric glycosphingosine mixtures. The analytical performance was also evaluated in terms of accuracy, repeatability, and interday precision. Furthermore, CID of the product ions resulting from 443 Da loss from the charge-inverted complex cations ([n-HexCer-H+MgTerpy]) has been performed and demonstrated for localization of the double-bond position on the amide-bonded monounsaturated fatty acyl chain in the cerebroside structure. The proposed strategy was successfully applied to the analysis of total cerebroside extracts from the porcine brain, providing in-depth structural information on cerebrosides from a biological mixture.

摘要

神经酰胺(n-HexCer)和神经鞘糖脂(n-HexSph)构成了两类鞘脂。两者均由单糖头基(哺乳动物细胞中的葡萄糖或半乳糖)通过α-或β-糖苷键连接到神经酰胺骨架上(n = α或β,取决于与糖的端基碳原子的连接性质)。神经酰胺还有一个通过酰胺键连接到神经酰胺骨架上的脂肪酸链。虽然区分多种异构体(即葡萄糖与半乳糖、α-与β-连接)很困难,但对于理解它们在健康和疾病状态下的特定生物学作用至关重要。串联质谱技术已成为脂质组学和糖组学分析的有力工具,但通常其区分异构体的能力有限。本工作描述了一种新策略,将串联质谱与气相离子化学相结合,实现对异构体神经酰胺和神经鞘糖脂的区分和定量。简要地说,去质子化的神经酰胺,[n-HexCer-H],或神经鞘糖脂,[n-HexSph-H],在气相中与三吡啶(Terpy)镁配合物二阳离子[Mg(Terpy)]反应,生成电荷反转的配合物阳离子,[n-HexCer-H+MgTerpy]或[n-HexSph-H+MgTerpy]。电荷反转的配合物阳离子的碰撞诱导解离(CID)导致两组异构体之间产生显著的光谱差异,对于神经酰胺,为α-GalCer、β-GlcCer 和β-GalCer,对于神经鞘糖脂,为α-GlcSph、α-GalSph、β-GlcSph 和β-GalSph,从而可以区分异构体。此外,我们描述了一种定量策略,从选定的诊断离子中提取归一化面积百分比,以定量三种异构体的神经酰胺或四种异构体的神经鞘糖脂混合物。还从准确性、重复性和日间精密度方面评估了分析性能。此外,还对电荷反转的配合物阳离子失去 443 Da 后产生的产物离子的 CID 进行了研究,并证明其可用于定位神经酰胺结构中酰胺键结合的单不饱和脂肪酸链上的双键位置。该策略已成功应用于猪脑总神经鞘糖脂提取物的分析,为生物混合物中的神经鞘糖脂提供了深入的结构信息。

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