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基于改进的基于MRM方法的靶向蛋白质组学对人肝脏蛋白质组中缺失蛋白质的筛选

Screening of missing proteins in the human liver proteome by improved MRM-approach-based targeted proteomics.

作者信息

Chen Chen, Liu Xiaohui, Zheng Weimin, Zhang Lei, Yao Jun, Yang Pengyuan

机构信息

Department of Chemistry, Fudan University , Shanghai 200032, P. R. China.

出版信息

J Proteome Res. 2014 Apr 4;13(4):1969-78. doi: 10.1021/pr4010986. Epub 2014 Mar 20.

Abstract

To completely annotate the human genome, the task of identifying and characterizing proteins that currently lack mass spectrometry (MS) evidence is inevitable and urgent. In this study, as the first effort to screen missing proteins in large scale, we developed an approach based on SDS-PAGE followed by liquid chromatography-multiple reaction monitoring (LC-MRM), for screening of those missing proteins with only a single peptide hit in the previous liver proteome data set. Proteins extracted from normal human liver were separated in SDS-PAGE and digested in split gel slice, and the resulting digests were then subjected to LC-schedule MRM analysis. The MRM assays were developed through synthesized crude peptides for target peptides. In total, the expressions of 57 target proteins were confirmed from 185 MRM assays in normal human liver tissues. Among the proved 57 one-hit wonders, 50 proteins are of the minimally redundant set in the PeptideAtlas database, 7 proteins even have none MS-based information previously in various biological processes. We conclude that our SDS-PAGE-MRM workflow can be a powerful approach to screen missing or poorly characterized proteins in different samples and to provide their quantity if detected. The MRM raw data have been uploaded to ISB/SRM Atlas/PASSEL (PXD000648).

摘要

为了完全注释人类基因组,识别和表征目前缺乏质谱(MS)证据的蛋白质的任务是不可避免且紧迫的。在本研究中,作为大规模筛选缺失蛋白质的首次尝试,我们开发了一种基于十二烷基硫酸钠-聚丙烯酰胺凝胶电泳(SDS-PAGE)随后进行液相色谱-多反应监测(LC-MRM)的方法,用于筛选在先前肝脏蛋白质组数据集中仅有一个肽段匹配的那些缺失蛋白质。从正常人肝脏中提取的蛋白质在SDS-PAGE中分离,并在凝胶切片中消化,然后将所得消化产物进行LC-定时MRM分析。通过合成针对目标肽段的粗肽来开发MRM检测方法。总共,在正常人肝脏组织中通过185次MRM检测确认了57种目标蛋白质的表达。在已证实的57种“单次命中奇迹”蛋白质中,50种蛋白质在肽图集数据库中属于最低冗余集,7种蛋白质在之前的各种生物学过程中甚至没有基于MS的信息。我们得出结论,我们的SDS-PAGE-MRM工作流程可以成为一种强大的方法,用于筛选不同样品中缺失或表征不佳的蛋白质,并在检测到它们时提供其数量。MRM原始数据已上传至ISB/SRM Atlas/PASSEL(PXD000648)。

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