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高覆盖度二硫键图谱分析方法的建立:基于程序化二硫键-烯反应的自上而下蛋白质分析工作流程。

High-Coverage Disulfide Mapping Enabled by Programmable Disulfide-Ene Reaction Integrated onto a Bottom-Up Protein Analysis Workflow.

机构信息

MOE Key Laboratory of Bioorganic Phosphorus Chemistry & Chemical Biology, Department of Chemistry, Tsinghua University, Beijing 10084, China.

出版信息

Anal Chem. 2024 Oct 29;96(43):17396-17404. doi: 10.1021/acs.analchem.4c04257. Epub 2024 Oct 19.

Abstract

Mapping disulfide linkages is crucial for characterizing pharmaceutical proteins during drug development and quality control. Traditional bottom-up protein analysis workflows often suffer from incomplete mapping for tryptic peptides consisting of multiple disulfide bonds. Although the employment of a partial reduction of disulfide bonds can improve disulfide mapping, it becomes a bottleneck of analysis because individual tuning is often needed. Herein, we have developed an online disulfide-ene reaction system in which the composition of the reaction solvent can be programmed to achieve optimal partial reduction of tryptic disulfide peptides after liquid chromatography separation. By coupling this system onto a bottom-up protein analysis workflow, high coverage for sequencing (71-83%) and disulfide mapping (84-100%) was achieved for standard proteins consisting of 4-19 disulfide bonds. The analytical capability was further demonstrated by mapping 13 scrambled disulfide bonds in lysozyme and achieving compositional analysis of IgG isotypes (κ and λ) and subclasses (IgG1-IgG4) from human plasma.

摘要

在药物开发和质量控制过程中,对药物进行药物分析,对二硫键进行定位至关重要。传统的自下而上的蛋白质分析工作流程通常因含有多个二硫键的胰蛋白酶肽不完全定位而受到影响。虽然部分还原二硫键的应用可以改善二硫键的定位,但由于需要进行单独的调整,它成为了分析的瓶颈。在此,我们开发了一种在线二硫键-烯反应系统,该系统可以对反应溶剂的组成进行编程,以在液相色谱分离后实现最佳的胰蛋白酶二硫键肽部分还原。通过将该系统与自下而上的蛋白质分析工作流程相结合,对于由 4-19 个二硫键组成的标准蛋白质,实现了高测序覆盖率(71-83%)和二硫键定位覆盖率(84-100%)。该分析能力通过对溶菌酶中 13 个错配二硫键进行定位以及对人血浆中的 IgG 同型(κ 和 λ)和亚型(IgG1-IgG4)进行组成分析得到了进一步证明。

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