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联用电喷雾电离质谱的前沿分析毛细管电泳用于抗凝血酶/肝素五糖复合物的表征

Frontal analysis capillary electrophoresis hyphenated to electrospray ionization mass spectrometry for the characterization of the antithrombin/heparin pentasaccharide complex.

作者信息

Fermas Soraya, Gonnet Florence, Varenne Anne, Gareil Pierre, Daniel Régis

机构信息

CNRS UMR 8587, Université d'Evry-Val-d'Essonne, Laboratoire Analyse et Modélisation pour la Biologie et l'Environnement, F-91025 Evry, France.

出版信息

Anal Chem. 2007 Jul 1;79(13):4987-93. doi: 10.1021/ac070146h. Epub 2007 May 31.

DOI:10.1021/ac070146h
PMID:17536781
Abstract

The interaction of proteins with polysaccharides represents a major and challenging topic in glycobiology, since such complexes mediate fundamental biological mechanisms. A new strategy based on the hyphenation of frontal analysis capillary electrophoresis (FACE) with electrospray ionization mass spectrometry (ESIMS) is reported for the characterization of protein/carbohydrate complexes. While most of the previously reported CE-MS experiments were performed using capillary electrophoresis in zone format, we report for the first time CE-MS experiments in which CE was performed in frontal analysis (FACE-MS). We showed that the frontal mode offered a better sensitivity than zone mode and was well suited for the CE-MS coupling. This FACE-MS coupling was applied to the analysis of the complex between antithrombin and the sulfated pentasaccharide reproducing the antithrombin-binding sequence in heparin. The mixture of coincubated antithrombin and heparin pentasaccharide was continuously injected into the capillary, and the electrophoretic separation of the free and bound forms of the protein was achieved. The intact noncovalent complex antithrombin/heparin pentasaccharide was detected on-line by ESIMS in positive ionization mode and in nondenaturing sheath liquid conditions. The complex stoichiometry was determined from the mass measurement of the complex. In addition, the characterization of the sulfated pentasaccharide ligand dissociated from the complex was performed in negative ionization mode using a denaturing sheath liquid, allowing the determination of its molecular mass and sulfation features. This FACE-ESIMS strategy opens the way to ligand fishing experiments performed on heterogeneous carbohydrate mixtures and subsequent characterization of specifically bound carbohydrates.

摘要

蛋白质与多糖的相互作用是糖生物学中的一个重要且具有挑战性的课题,因为此类复合物介导着基本的生物学机制。本文报道了一种基于前沿分析毛细管电泳(FACE)与电喷雾电离质谱(ESIMS)联用的新策略,用于表征蛋白质/碳水化合物复合物。虽然此前报道的大多数CE-MS实验都是采用区带形式的毛细管电泳进行的,但我们首次报道了采用前沿分析(FACE-MS)进行CE-MS实验。我们表明,前沿模式比区带模式具有更高的灵敏度,非常适合CE-MS联用。这种FACE-MS联用技术被应用于分析抗凝血酶与模拟肝素中抗凝血酶结合序列的硫酸化五糖之间的复合物。将共孵育的抗凝血酶和肝素五糖混合物连续注入毛细管,实现了蛋白质游离形式和结合形式的电泳分离。通过ESIMS在正离子化模式和非变性鞘液条件下在线检测完整的非共价复合物抗凝血酶/肝素五糖。根据复合物的质量测量确定复合物的化学计量。此外,使用变性鞘液在负离子化模式下对从复合物中解离的硫酸化五糖配体进行表征,从而确定其分子量和硫酸化特征。这种FACE-ESIMS策略为在异质碳水化合物混合物上进行配体筛选实验以及随后对特异性结合碳水化合物的表征开辟了道路。

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