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一种用于深入表征复杂肽混合物的综合定向质谱方法。

An integrated, directed mass spectrometric approach for in-depth characterization of complex peptide mixtures.

作者信息

Schmidt Alexander, Gehlenborg Nils, Bodenmiller Bernd, Mueller Lukas N, Campbell Dave, Mueller Markus, Aebersold Ruedi, Domon Bruno

机构信息

Institute of Molecular Systems Biology and section signCompetence Center for Systems Physiology and Metabolic Diseases, ETH Zurich, Wolfgang-Pauli-Str. 16, 8093 Zurich, Switzerland.

出版信息

Mol Cell Proteomics. 2008 Nov;7(11):2138-50. doi: 10.1074/mcp.M700498-MCP200. Epub 2008 May 29.

DOI:10.1074/mcp.M700498-MCP200
PMID:18511481
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2577211/
Abstract

LC-MS/MS has emerged as the method of choice for the identification and quantification of protein sample mixtures. For very complex samples such as complete proteomes, the most commonly used LC-MS/MS method, data-dependent acquisition (DDA) precursor selection, is of limited utility. The limited scan speed of current mass spectrometers along with the highly redundant selection of the most intense precursor ions generates a bias in the pool of identified proteins toward those of higher abundance. A directed LC-MS/MS approach that alleviates the limitations of DDA precursor ion selection by decoupling peak detection and sequencing of selected precursor ions is presented. In the first stage of the strategy, all detectable peptide ion signals are extracted from high resolution LC-MS feature maps or aligned sets of feature maps. The selected features or a subset thereof are subsequently sequenced in sequential, non-redundant directed LC-MS/MS experiments, and the MS/MS data are mapped back to the original LC-MS feature map in a fully automated manner. The strategy, implemented on an LTQ-FT MS platform, allowed the specific sequencing of 2,000 features per analysis and enabled the identification of more than 1,600 phosphorylation sites using a single reversed phase separation dimension without the need for time-consuming prefractionation steps. Compared with conventional DDA LC-MS/MS experiments, a substantially higher number of peptides could be identified from a sample, and this increase was more pronounced for low intensity precursor ions.

摘要

液相色谱-串联质谱(LC-MS/MS)已成为鉴定和定量蛋白质样品混合物的首选方法。对于诸如完整蛋白质组等非常复杂的样品,最常用的LC-MS/MS方法——数据依赖型采集(DDA)前体选择,效用有限。当前质谱仪有限的扫描速度以及对最强前体离子的高度冗余选择,使得已鉴定蛋白质库偏向于丰度较高的蛋白质。本文提出了一种定向LC-MS/MS方法,该方法通过将峰检测与选定前体离子的测序解耦,减轻了DDA前体离子选择的局限性。在该策略的第一阶段,从高分辨率LC-MS特征图谱或特征图谱的对齐集中提取所有可检测的肽离子信号。随后,在连续的、非冗余的定向LC-MS/MS实验中对选定的特征或其一个子集进行测序,并以全自动方式将MS/MS数据映射回原始LC-MS特征图谱。该策略在LTQ-FT MS平台上实施,每次分析可对2000个特征进行特异性测序,并且在无需耗时的预分级步骤的情况下,仅使用一个反相分离维度就能鉴定出1600多个磷酸化位点。与传统的DDA LC-MS/MS实验相比,从一个样品中可鉴定出的肽数量显著增加,并且这种增加在低强度前体离子中更为明显。

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