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离子淌度质谱法可直接从糖链释放后的孵育混合物中提取 N-糖链的谱图:应用于完整折叠 HIV gp120 工程糖型的糖链。

Ion mobility mass spectrometry for extracting spectra of N-glycans directly from incubation mixtures following glycan release: application to glycans from engineered glycoforms of intact, folded HIV gp120.

机构信息

Oxford Glycobiology Institute, Department of Biochemistry, University of Oxford, South Parks Road, Oxford, OX1 3QU, UK.

出版信息

J Am Soc Mass Spectrom. 2011 Mar;22(3):568-81. doi: 10.1007/s13361-010-0053-0. Epub 2011 Feb 8.

DOI:10.1007/s13361-010-0053-0
PMID:21472575
Abstract

The analysis of glycosylation from native biological sources is often frustrated by the low abundances of available material. Here, ion mobility combined with electrospray ionization mass spectrometry have been used to extract the spectra of N-glycans released with PNGase F from a serial titration of recombinantly expressed envelope glycoprotein, gp120, from the human immunodeficiency virus (HIV). Analysis was also performed on gp120 expressed in the α-mannosidase inhibitor, and in a matched mammalian cell line deficient in GlcNAc transferase I. Without ion mobility separation, ESI spectra frequently contained no observable ions from the glycans whereas ions from other compounds such as detergents and residual buffer salts were abundant. After ion mobility separation on a Waters T-wave ion mobility mass spectrometer, the N-glycans fell into a unique region of the ion mobility/m/z plot allowing their profiles to be extracted with good signal:noise ratios. This method allowed N-glycan profiles to be extracted from crude incubation mixtures with no clean-up even in the presence of surfactants such as NP40. Furthermore, this technique allowed clear profiles to be obtained from sub-microgram amounts of glycoprotein. Glycan profiles were similar to those generated by MALDI-TOF MS although they were more susceptible to double charging and fragmentation. Structural analysis could be accomplished by MS/MS experiments in either positive or negative ion mode but negative ion mode gave the most informative spectra and provided a reliable approach to the analysis of glycans from small amounts of glycoprotein.

摘要

从天然生物来源中分析糖基化常常受到可用材料丰度低的阻碍。在这里,离子淌度结合电喷雾电离质谱已被用于从人免疫缺陷病毒(HIV)中重组表达的包膜糖蛋白 gp120 的连续滴定中提取 PNGase F 释放的 N-糖链的谱图。还对在 α-甘露糖苷酶抑制剂中表达的 gp120 以及在缺乏 GlcNAc 转移酶 I 的匹配哺乳动物细胞系中表达的 gp120 进行了分析。如果没有离子淌度分离,ESI 谱图中通常没有可观察到的聚糖离子,而洗涤剂和残留缓冲盐等其他化合物的离子则很丰富。在 Waters T-wave 离子淌度质谱仪上进行离子淌度分离后,N-聚糖落入离子淌度/m/z 图的独特区域,允许以良好的信噪比提取其谱图。即使存在表面活性剂(如 NP40),这种方法也允许从未经纯化的粗孵育混合物中提取 N-聚糖谱图,而无需进行清洁。此外,该技术允许从小至微克级的糖蛋白中获得清晰的谱图。聚糖谱图与 MALDI-TOF MS 生成的谱图相似,但它们更容易发生双重电荷和碎片化。通过正离子或负离子模式下的 MS/MS 实验可以进行结构分析,但负离子模式提供了最具信息量的谱图,并为从小量糖蛋白中分析聚糖提供了可靠的方法。

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