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利用气相氢/氘交换质谱法探究蛋白质复合物的结合界面

Probing the Binding Interfaces of Protein Complexes Using Gas-Phase H/D Exchange Mass Spectrometry.

作者信息

Mistarz Ulrik H, Brown Jeffery M, Haselmann Kim F, Rand Kasper D

机构信息

Department of Pharmacy, University of Copenhagen, Universitetsparken 2, Copenhagen 2100, Denmark.

Waters MS Technologies Centre, Waters Corporation, Altrincham Road, Wilmslow SK9 4AX, UK.

出版信息

Structure. 2016 Feb 2;24(2):310-8. doi: 10.1016/j.str.2015.11.013. Epub 2015 Dec 31.

Abstract

Fast gas-phase hydrogen/deuterium exchange mediated by ND3 gas and measured by mass spectrometry (gas-phase HDX-MS) is a largely unharnessed, fast, and sensitive method for probing primary- and higher-order polypeptide structure. Labeling of heteroatom-bound non-amide hydrogens in a sub-millisecond time span after electrospray ionization by ND3 gas can provide structural insights into protein conformers present in solution. Here, we have explored the use of gas-phase HDX-MS for probing the higher-order structure and binding interfaces of protein complexes originating from native solution conditions. Lysozyme ions bound by an oligosaccharide incorporated less deuterium than the unbound ion. Similarly, trypsin ions showed reduced deuterium uptake when bound by the peptide ligand vasopressin. Our results are in good agreement with crystal structures of the native protein complexes, and illustrate that gas-phase HDX-MS can provide a sensitive and simple approach to measure the number of heteroatom-bound non-amide side-chain hydrogens involved in the binding interface of biologically relevant protein complexes.

摘要

由ND₃气体介导并通过质谱法测量的快速气相氢/氘交换(气相HDX-MS)是一种很大程度上未被利用的、快速且灵敏的探测一级和高级多肽结构的方法。在电喷雾电离后,通过ND₃气体在亚毫秒时间跨度内对杂原子结合的非酰胺氢进行标记,可为溶液中存在的蛋白质构象异构体提供结构见解。在此,我们探索了使用气相HDX-MS来探测源自天然溶液条件的蛋白质复合物的高级结构和结合界面。与寡糖结合的溶菌酶离子比未结合的离子结合的氘更少。同样,当胰蛋白酶离子与肽配体加压素结合时,其氘摄取减少。我们的结果与天然蛋白质复合物的晶体结构高度一致,并表明气相HDX-MS可以提供一种灵敏且简单的方法来测量参与生物学相关蛋白质复合物结合界面的杂原子结合的非酰胺侧链氢的数量。

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