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利用光致自由基反应和电子转移二硫代二异丙基氨基甲酸盐对二硫键连接蛋白进行自上而下分析

Top-Down Analysis of Disulfide-Linked Proteins Using Photoinduced Radical Reactions and ET-DDC.

作者信息

Adhikari Sarju, Xia Yu, McLuckey Scott A

机构信息

Department of Chemistry, Purdue University, West Lafayette, IN 47907, USA.

Department of Chemistry, Tsinghua University, Beijing 100084, China.

出版信息

Int J Mass Spectrom. 2019 Oct;444. doi: 10.1016/j.ijms.2019.06.009. Epub 2019 Jul 2.

Abstract

Top-down characterization of proteins via tandem mass spectrometry (MS/MS) can be challenging due to the presence of multiple disulfide bond linkages; which significantly inhibit the backbone cleavage efficiency for the formation of structurally informative fragment ions. In this study, we present a strategy of pairing a solution-phase photoinitiating system with dipolar direct current induced collisional activation of electron transfer products (ET-DDC) of proteins for a top-down MS/MS approach. The photoinitiating system allows for a rapid scission of all the disulfide linkages in the protein (on the time scale of seconds) with high efficiency (near to complete reduction); while ET-DDC collisional activation improves the fragmentation efficiency for the protein via broadband activation of all the first-generation charge reduced precursor ions (e.g., electron transfer no-dissociation or ETnoD products) from electron transfer reactions over a wide mass-to-charge range. As a result, this approach enabled the generation of extensive sequence informative fragment ion yields for a rapid and enhanced structural characterization of disulfide-linked proteins.

摘要

由于存在多个二硫键连接,通过串联质谱(MS/MS)对蛋白质进行自上而下的表征可能具有挑战性;这会显著抑制形成结构信息丰富的碎片离子时的主链裂解效率。在本研究中,我们提出了一种策略,即将溶液相光引发系统与蛋白质的电子转移产物(ET-DDC)的偶极直流诱导碰撞活化相结合,用于自上而下的MS/MS方法。该光引发系统能够在数秒的时间尺度内高效地(接近完全还原)快速切断蛋白质中的所有二硫键连接;而ET-DDC碰撞活化通过在宽质荷比范围内对电子转移反应产生的所有第一代电荷减少的前体离子(例如,电子转移非解离或ETnoD产物)进行宽带活化,提高了蛋白质的碎片化效率。因此,这种方法能够产生大量序列信息丰富的碎片离子,从而快速且增强地对二硫键连接的蛋白质进行结构表征。

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