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通过液相色谱-质谱联用技术对糖蛋白中N-连接和O-连接寡糖进行选择性鉴定与区分

Selective identification and differentiation of N- and O-linked oligosaccharides in glycoproteins by liquid chromatography-mass spectrometry.

作者信息

Carr S A, Huddleston M J, Bean M F

机构信息

Department of Physical and Structural Chemistry, SmithKline Beecham Pharmaceuticals, King of Prussia, Pennsylvania 19406.

出版信息

Protein Sci. 1993 Feb;2(2):183-96. doi: 10.1002/pro.5560020207.

Abstract

A mass spectrometry method has been developed for selective detection of glycopeptides at the low (< or = 25) picomole level during chromatography of glycoprotein digests and for differentiation of O-linked from N-linked oligosaccharides. The technique involves observation of diagnostic sugar oxonium-ion fragments, particularly the HexNAc+ fragment at m/z 204, from collisionally excited glycopeptides. Collision-induced fragmentation can be accomplished in either of two regions of a triple quadrupole mass spectrometer equipped with an atmospheric pressure, electrospray (ES) ionization source. If collisions before the first quadrupole are chosen, it is possible to enhance formation of carbohydrate-related fragment ions without distorting the distribution of peptide and glycopeptide signals by increasing the collisional excitation potential only during that portion of each scan in which the low mass carbohydrate-related ions are being detected. This procedure, requiring only a single quadrupole instrument, identifies putative glycopeptide-containing fractions in the chromatogram but suffers from a lack of specificity in the case of co-eluting peptides. Increased specificity is obtained by selectively detecting only those parent ions that fragment in Q2, the second collision region of the triple quadrupole, to produce an ion at m/z 204 (HexNAc+). Only (M + H)+ ions of glycopeptides are observed in these liquid chromatography-electrospray tandem mass spectrometry (LC-ESMS/MS) "parent-scan" spectra. N-linked carbohydrates are differentiated from O-linked by LC-ESMS/MS analysis of the digested glycoprotein prior to and after selective removal of N-linked carbohydrates by peptide N:glycosidase F. These methods, which constitute the first liquid chromatography-mass spectrometry (LC-MS)-based strategies for selective identification of glycopeptides in complex mixtures, facilitate location and preparative fractionation of glycopeptides for further structural characterization. In addition, these techniques may be used to assess the compositional heterogeneity at specific attachment sites, and to define the sequence context of the attachment site in proteins of known sequence. The strategy is demonstrated for bovine fetuin, a 42-kDa glycoprotein containing three N-linked, and at least three O-linked carbohydrates. Over 90% of the fetuin protein sequence was also corroborated by these LC-ESMS studies.

摘要

已开发出一种质谱方法,用于在糖蛋白消化物色谱分析过程中,在低(≤25)皮摩尔水平选择性检测糖肽,并区分O-连接和N-连接的寡糖。该技术涉及观察经碰撞激发的糖肽的诊断性糖鎓离子碎片,特别是m/z 204处的己糖胺离子(HexNAc⁺)。碰撞诱导裂解可在配备大气压电喷雾(ES)电离源的三重四极杆质谱仪的两个区域中的任一区域完成。如果选择在第一个四极杆之前进行碰撞,则可以通过仅在每次扫描中检测低质量碳水化合物相关离子的那部分时间内增加碰撞激发电位,来增强与碳水化合物相关的碎片离子的形成,而不会扭曲肽和糖肽信号的分布。此程序仅需一台四极杆仪器,可识别色谱图中假定含糖肽的馏分,但在共洗脱肽的情况下缺乏特异性。通过仅选择性检测那些在三重四极杆的第二个碰撞区域Q2中裂解以产生m/z 204(HexNAc⁺)离子的母离子,可提高特异性。在这些液相色谱-电喷雾串联质谱(LC-ESMS/MS)“母扫描”光谱中仅观察到糖肽的(M + H)⁺离子。通过在肽N:糖苷酶F选择性去除N-连接的碳水化合物之前和之后,对消化的糖蛋白进行LC-ESMS/MS分析,可区分N-连接和O-连接的碳水化合物。这些方法构成了基于液相色谱-质谱(LC-MS)的首批用于在复杂混合物中选择性鉴定糖肽的策略,有助于糖肽的定位和制备分馏,以进行进一步的结构表征。此外,这些技术可用于评估特定连接位点的组成异质性,并确定已知序列蛋白质中连接位点的序列上下文。以牛胎球蛋白为例展示了该策略,牛胎球蛋白是一种42 kDa的糖蛋白,含有三个N-连接和至少三个O-连接的碳水化合物。这些LC-ESMS研究还证实了超过90%的胎球蛋白蛋白质序列。

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