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通过串联质谱法分析碳水化合物结构异构体。

Carbohydrate structural isomers analyzed by sequential mass spectrometry.

作者信息

Ashline David J, Lapadula Anthony J, Liu Yan-Hui, Lin Mei, Grace Mike, Pramanik Birendra, Reinhold Vernon N

机构信息

The Glycomics Center, Department of Biochemistry and Molecular Biology, University of New Hampshire, Durham, New Hampshire 03824, USA.

出版信息

Anal Chem. 2007 May 15;79(10):3830-42. doi: 10.1021/ac062383a. Epub 2007 Mar 31.

Abstract

Consistent with the goals of a comprehensive carbohydrate sequencing strategy, we extend earlier reports to include the characterization of structural (constitutional) isomers. Protocols were developed around ion trap instrumentation providing sequential mass spectrometry (MSn) and supported with automation and related computational tools. These strategies have been built on the principle that for a single structure all product spectra upon sequential fragmentation are reproducible and each stage represents a rational spectrum of its precursor; i.e., all major fragments should be accounted for. Anomalous ions at any stage are clues indicating the presence of structural isomers. Gas-phase isolation and subsequent fragmentation of such ions provide an opportunity to specifically resolve selected structures for their detailed characterization. Importantly, some isomers were not detected following MS2 and required multiple (MSn>2) stages for their characterization. Derivatization remains critical to position substructures in a glycan array since product ions carry fragmentation "scars" throughout the MSn tree. Equally as important are the pathway relationships between each stage and the greater yield of fragments with the smaller number of oscillators. Applications were directed to the structural isomers in ovalbumin and IgG, where, in the latter case, several previously unreported glycans were detected. Procedures were supported with bioinformatics tools for assimilating structure from the MSn data sets.

摘要

与全面的碳水化合物测序策略目标一致,我们扩展了早期报告,以纳入结构(构型)异构体的表征。围绕提供串联质谱(MSn)的离子阱仪器开发了方案,并辅以自动化和相关计算工具。这些策略基于这样的原则:对于单一结构,连续碎片化后的所有产物谱都是可重复的,并且每个阶段都代表其前体的合理谱;即,所有主要碎片都应得到解释。任何阶段出现的异常离子都是表明存在结构异构体的线索。对这些离子进行气相分离并随后碎片化,为具体解析选定结构以进行详细表征提供了机会。重要的是,一些异构体在MS2之后未被检测到,需要多个(MSn>2)阶段来进行表征。衍生化对于在聚糖阵列中定位亚结构仍然至关重要,因为产物离子在整个MSn树中都带有碎片化“痕迹”。每个阶段之间的途径关系以及使用较少振荡器获得更高产量的碎片同样重要。应用针对卵清蛋白和IgG中的结构异构体,在后一种情况下,检测到了几种先前未报道的聚糖。使用生物信息学工具来从MSn数据集中提取结构,为这些程序提供了支持。

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