Separation of Sialylated Glycan Isomers by Differential Mobility Spectrometry

被引:28
|
作者
Lane, Catherine S. [1 ]
McManus, Kirsty [2 ]
Widdowson, Philip [2 ]
Flowers, Sarah A. [3 ]
Powell, Gerard [2 ]
Anderson, Ian [2 ]
Campbell, J. Larry [4 ]
机构
[1] SCIEX Ltd, Phoenix House,Ctr Pk, Warrington WA1 1RX, Cheshire, England
[2] Allergan Biol Ltd, 12 Estuary Banks, Liverpool L24 8RB, Merseyside, England
[3] Georgetown Univ, Washington, DC USA
[4] SCIEX Ltd, 71 Four Valley Dr, Concord, ON L4K 4V8, Canada
基金
美国国家卫生研究院;
关键词
NEGATIVE-ION FRAGMENTATION; MASS-SPECTROMETRY; N-GLYCANS; QUANTITATIVE-ANALYSIS; ACID LINKAGE; SIALIC ACIDS; GLYCOPEPTIDE; IDENTIFICATION; GLYCOSYLATION; GLYCOPROTEIN;
D O I
10.1021/acs.analchem.9b01595
中图分类号
O65 [分析化学];
学科分类号
070302 ; 081704 ;
摘要
Mass spectrometry has proven itself to be an important technology for characterizing intact glycoproteins, glycopeptides, and released glycans. However, these molecules often present significant challenges during analysis. For example, glycans of identical molecular weights can be present in many isomeric forms, with one form having dramatically more biological activity than the others. Discriminating among these isomeric forms using mass spectrometry alone can be daunting, which is why orthogonal techniques, such as ion mobility spectrometry, have been explored. Here, we demonstrate the use of differential mobility spectrometry (DMS) to separate isomeric glycans differing only in the linkages of sialic acid groups (e.g., alpha 2,3 versus alpha 2,6). This ability extends from a small trisaccharide species to larger biantennary systems and is driven, in part, by the role of intramolecular solvation of the charge site(s) on these ions within the DMS environment.
引用
收藏
页码:9916 / 9924
页数:9
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