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利用被困离子淌度质谱-电子激发解离串联质谱技术准确识别同分异构体聚糖。

Accurate Identification of Isomeric Glycans by Trapped Ion Mobility Spectrometry-Electronic Excitation Dissociation Tandem Mass Spectrometry.

机构信息

Center for Biomedical Mass Spectrometry, Boston University School of Medicine, 670 Albany Street, Room 508, Boston, Massachusetts 02118, United States.

Department of Chemistry, Boston University, Boston, Massachusetts 02215, United States.

出版信息

Anal Chem. 2020 Oct 6;92(19):13211-13220. doi: 10.1021/acs.analchem.0c02374. Epub 2020 Sep 11.

Abstract

Ion mobility-mass spectrometry (IM-MS) has become a powerful tool for glycan structural characterization due to its ability to separate isomers and provide collision cross section (CCS) values that facilitate structural assignment. However, IM-based isomer analysis may be complicated by the presence of multiple gas-phase conformations of a single structure that not only increases difficulty in isomer separation but can also introduce the possibility for misinterpretation of conformers as isomers. Here, the ion mobility behavior of several sets of isomeric glycans, analyzed as their permethylated derivatives, in both nonreduced and reduced forms, was investigated by gated-trapped ion mobility spectrometry (G-TIMS). Notably, reducing-end reduction, commonly performed to remove anomerism-induced chromatographic peak splitting, did not eliminate the conformational heterogeneity of permethylated glycans in the gas phase. At a mobility resolving power of ∼100, 14 out of 22 structures showed more than one conformation. These results highlight the need to use IMS devices with high mobility resolving power for better separation of isomers and to acquire additional structural information that can differentiate isomers from conformers. Online electronic excitation dissociation (EED) MS/MS analysis of isomeric glycan mixtures following G-TIMS separation showed that EED can generate isomer-specific fragments while producing nearly identical tandem mass spectra for conformers, thus allowing confident identification of isomers with minimal evidence of any ambiguity resulting from the presence of conformers. G-TIMS EED MS/MS analysis of -linked glycans released from ovalbumin revealed that several mobility features previously thought to arise from isomeric structures were conformers of a single structure. Finally, analysis of ovalbumin -glycans from different sources showed that the G-TIMS EED MS/MS approach can accurately determine the batch-to-batch variations in glycosylation profiles at the isomer level, with confident assignment of each isomeric structure.

摘要

离子淌度-质谱(IM-MS)因其能够分离异构体并提供有助于结构分配的碰撞截面(CCS)值,已成为糖链结构表征的有力工具。然而,由于单个结构的多种气相构象的存在,基于 IM 的异构体分析可能会变得复杂,这不仅增加了异构体分离的难度,而且还可能导致将构象错误地解释为异构体。在这里,通过门控俘获离子淌度谱(G-TIMS)研究了几组合成糖,作为其全甲基化衍生物,在非还原和还原形式下的离子淌度行为。值得注意的是,通常为了消除端基异构诱导的色谱峰分裂而进行的还原端还原并没有消除气相中全甲基化糖的构象异质性。在大约 100 的淌度分辨率下,22 个结构中有 14 个显示出不止一种构象。这些结果突出表明需要使用具有高淌度分辨率的 IMS 设备来更好地分离异构体,并获取可以将异构体与构象区分开来的附加结构信息。G-TIMS 分离后对异构体糖混合物进行在线电子激发解离(EED)MS/MS 分析表明,EED 可以产生异构体特异性片段,同时为构象产生几乎相同的串联质谱,从而可以在存在构象的情况下通过最小的歧义证据来确定异构体。对来自卵清蛋白的 -连接糖进行 G-TIMS EED MS/MS 分析表明,以前认为是由异构结构引起的几个淌度特征实际上是单一结构的构象。最后,对来自不同来源的卵清蛋白 -糖的分析表明,G-TIMS EED MS/MS 方法可以准确地确定在异构体水平上糖基化谱的批间变化,并对每个异构体结构进行有信心的分配。

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