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O-糖基化肽段的电子捕获解离:自由基位点诱导的糖苷键断裂

Electron capture dissociation of O-glycosylated peptides: radical site-induced fragmentation of glycosidic bonds.

作者信息

Mormann Michael, Paulsen Hans, Peter-Katalinić Jasna

机构信息

Institute for Medical Physics and Biophysics, Biomedical Analysis Department, University of Münster, Robert-Koch-Str. 31, D-48149 Münster, Germany.

出版信息

Eur J Mass Spectrom (Chichester). 2005;11(5):497-511. doi: 10.1255/ejms.738.

DOI:10.1255/ejms.738
PMID:16322656
Abstract

Glycosylation of proteins represents one of the most important post-translational modifications. The structural characterisation of glycoproteins--especially with respect to the determination of the glycosylation site--by direct mass spectrometric methods still remains an elusive goal. We have applied the low energy dissociation method electron capture dissociation (ECD) in a 9.4 T Fourier transform ion cyclotron resonance mass spectrometer to the structural elucidation of mucin-derived peptides glycosylated with glycans of different core types. Capture of an electron by multiply protonated precursor ions M + nH resulted in the formation of reduced odd electron radical cations M + nH+*. Subsequent cleavage of the N-Calpha bonds of the peptide chain, mostly without loss of the labile sugar moiety, represents a major fragmentation pathway allowing unambiguous assignment of the glycosylation site. In addition to peptide backbone cleavages, loss of acetyl radicals from the N-acetyl group of the HexNAc glycans is observed. Radical site induced elimination processes of the glycan moieties initiated by hydrogen transfer, from the glycan to the peptide backbone and vice versa give rise to signals in the ECD spectra. The different sugar core types exhibit different fragmentation patterns driven by the stability of the resulting fragments allowing the discrimination of isomeric glycans.

摘要

蛋白质糖基化是最重要的翻译后修饰之一。通过直接质谱方法对糖蛋白进行结构表征——尤其是确定糖基化位点——仍然是一个难以实现的目标。我们在一台9.4 T傅里叶变换离子回旋共振质谱仪中应用低能解离方法电子捕获解离(ECD),对源自粘蛋白且被不同核心类型聚糖糖基化的肽段进行结构解析。多个质子化前体离子M + nH捕获一个电子,导致形成还原的奇数电子自由基阳离子[M + nH](n - 1)+*。随后肽链的N - Cα键断裂,大多数情况下不会损失不稳定的糖部分,这是一种主要的碎裂途径,可明确确定糖基化位点。除了肽主链断裂外,还观察到HexNAc聚糖的N - 乙酰基上的乙酰基自由基丢失。由氢转移引发的聚糖部分的自由基位点诱导消除过程,从聚糖到肽主链以及反之亦然,在ECD谱中产生信号。不同的糖核心类型表现出不同的碎裂模式,这由所得碎片的稳定性驱动,从而能够区分异构体聚糖。

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