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纳米盘和电喷雾电离质谱:筛选糖脂与蛋白质相互作用的工具

Nanodiscs and electrospray ionization mass spectrometry: a tool for screening glycolipids against proteins.

机构信息

Alberta Glycomics Centre and Department of Chemistry, University of Alberta , Edmonton, Alberta T6G 2G2, Canada.

出版信息

Anal Chem. 2014 Jun 3;86(11):5271-7. doi: 10.1021/ac4041179. Epub 2014 May 14.

DOI:10.1021/ac4041179
PMID:24779922
Abstract

Electrospray ionization-mass spectrometry (ESI-MS) is extensively employed to detect and quantify protein-carbohydrate interactions in vitro and is increasingly used to screen carbohydrate libraries against target proteins. However, current ESI-MS methods are limited to carbohydrate ligands that are relatively soluble in water and are, therefore, not generally suitable for studying protein interactions with glycolipids, an important class of cellular receptors. Here, we describe a catch-and-release (CaR)-ESI-MS assay, which exploits nanodiscs (NDs) to solubilize glycolipids and mimic their natural cellular environment, suitable for screening libraries of glycosphingolipids (GSL) against proteins to identify specific interactions and to rank their relative affinities. Using the B subunit homopentamers of cholera toxin and heat labile toxin as model GSL-binding proteins, the CaR-ESI-MS was applied to NDs containing mixtures of gangliosides. The results demonstrate that the CaR-ESI-MS assay can simultaneously detect both high and low affinity GSL ligands using either a library of NDs that each contains one GSL or incorporating a mixture of GSLs into a single ND. Moreover, the relative abundances of the released ligands appear to reflect their relative affinities in solution. Application of the CaR-ESI-MS assay using NDs containing gangliosides extracted from porcine brain led to the discovery of a neolacto GSL as a cholera toxin ligand, highlighting the power of the assay for identifying specific protein-glycolipid interactions from biologically relevant mixtures.

摘要

电喷雾电离-质谱(ESI-MS)被广泛用于检测和定量体外蛋白质-碳水化合物相互作用,并且越来越多地用于筛选针对靶蛋白的碳水化合物文库。然而,目前的 ESI-MS 方法仅限于在水中相对可溶的碳水化合物配体,因此通常不适合研究蛋白质与糖脂的相互作用,糖脂是一类重要的细胞受体。在这里,我们描述了一种捕获和释放(CaR)-ESI-MS 测定法,该方法利用纳米盘(NDs)来增溶糖脂并模拟其天然细胞环境,适用于筛选糖脂(GSL)文库与蛋白质的相互作用,以鉴定特定相互作用并对其相对亲和力进行排序。使用霍乱毒素和不耐热毒素的 B 亚基五聚体作为模型 GSL 结合蛋白,将 CaR-ESI-MS 应用于含有神经节苷脂混合物的 NDs。结果表明,CaR-ESI-MS 测定法可以同时使用包含一种 GSL 的 NDs 文库或混合 GSL 混合物来检测高亲和性和低亲和性 GSL 配体。此外,释放配体的相对丰度似乎反映了它们在溶液中的相对亲和力。使用从猪脑中提取的神经节苷脂的 NDs 进行 CaR-ESI-MS 测定,发现神经节苷脂是霍乱毒素的配体,突出了该测定法从生物学相关混合物中鉴定特定蛋白质-糖脂相互作用的强大功能。

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