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通过增加硫糖脂组学和全甲基化聚糖的目标分析的额外维度来提高基于质谱的糖组学覆盖深度。

Increasing the depth of mass spectrometry-based glycomic coverage by additional dimensions of sulfoglycomics and target analysis of permethylated glycans.

机构信息

Institute of Biochemical Sciences, National Taiwan University, Roosevelt Road, PO Box 23-106, Taipei, 10617, Taiwan.

出版信息

Anal Bioanal Chem. 2013 Aug;405(21):6683-95. doi: 10.1007/s00216-013-7128-2.

DOI:10.1007/s00216-013-7128-2
PMID:23797909
Abstract

Hog or porcine gastric mucin resembles the human source in carrying not only blood group antigens but also the rather rare α4-GlcNAc-capped terminal epitope functionally implicated in protection against Helicobacter pylori infection. Being more readily available and reasonably well characterized, it serves as a good reagent for immunobiological studies, as well as a standard for analytical methodology developments. Current approaches in mass spectrometry (MS)-based glycomic mapping remain vastly inadequate in revealing the full complexity of glycosylation, particularly for cases such as the extremely heterogeneous O-glycosylation of mucosal mucins that can be further sulfated. We demonstrate here a novel concerted workflow that extends the conventional matrix-assisted laser desorption/ionization–mass spectrometry (MALDI-MS) mapping of permethylated glycans in positive ion mode to include a further step of sulfoglycomic analysis in negative ion mode. This was facilitated by introducing a mixed-mode solid-phase extraction step, which allows direct cleanup and simultaneous fractionation of the permethylated glycans into separate non-sulfated and sulfated pools in one single step. By distinct MALDI-MS/MS fragmentation patterns, all previously known structural features of porcine gastric mucin including the terminal epitopes and location of sulfates could be readily defined. We additionally showed that both arms of the core 2 structures could be extended via 6-O-sulfated GlcNAc to yield a series of disulfated O-glycans not previously reported, thus expanding its current glycomic coverage. However, a targeted LC-MSn analysis was required and best suited to dig even deeper into validating the occurrence of very minor structural isomers carrying the Lewis Y epitope implicated by positive antibody binding.

摘要

猪胃粘蛋白不仅携带血型抗原,还携带相当罕见的α4-GlcNAc 封端末端表位,该表位在保护免受幽门螺杆菌感染方面具有功能。由于其更容易获得且特征良好,因此它是免疫生物学研究的良好试剂,也是分析方法学发展的标准。目前基于质谱(MS)的糖组学图谱方法在揭示糖基化的全部复杂性方面仍然远远不够,特别是对于粘膜粘蛋白的极度异质 O-糖基化等情况,这种糖基化还可以进一步硫酸化。我们在这里展示了一种新颖的协同工作流程,该流程将传统的基质辅助激光解吸/电离-质谱(MALDI-MS)在正离子模式下对甲基化聚糖的图谱扩展到负离子模式下的进一步硫酸糖组学分析。这是通过引入混合模式固相萃取步骤来实现的,该步骤允许直接对甲基化聚糖进行净化,并在一个步骤中同时将其分离为非硫酸化和硫酸化的单独池。通过独特的 MALDI-MS/MS 碎裂模式,可以轻松定义猪胃粘蛋白的所有先前已知结构特征,包括末端表位和硫酸酯的位置。我们还表明,核心 2 结构的两个臂都可以通过 6-O-硫酸化 GlcNAc 扩展,从而产生一系列以前未报道的双硫酸化 O-聚糖,从而扩大其当前的糖组学覆盖范围。但是,需要进行靶向 LC-MSn 分析,并且最适合进一步深入验证携带阳性抗体结合所涉及的刘易斯 Y 表位的非常小的结构异构体的存在。

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