Modern strategies for protein quantification in proteome analysis: Advantages and limitations

被引:105
作者
Hamdan, M [1 ]
Righetti, PG
机构
[1] GlaxoSmithKline, Comp Analyt & Struct Sci, Verona, Italy
[2] Univ Verona, Dept Agr & Ind Biotechnol, I-37100 Verona, Italy
关键词
protein quantification; 2-D maps; multi-dimensional chromatography; fluorescence; isotope-coded tags; mass-coded tags;
D O I
10.1002/mas.10032
中图分类号
O433 [光谱学];
学科分类号
0703 ; 070302 ;
摘要
Over the last 3 years, a number of mass spectrometry-based methods for the simultaneous identification and quantification of individual proteins within complex mixtures have been reported. Most, if not all, of such strategies apply a two-step approach: the first for the separation of proteins or peptides, and the second uses mass spectrometry to identify and quantify the individual components. To simplify the outcome of both steps, certain chemicals and heavy-isotope-labeling are commonly used in the early stages of sample preparation (except in differential fluorescence labeling protocols). The ultimate goal of these strategies is to be able to identify every protein expressed in a cell or tissue, and to determine each protein's abundance, state of modification, and possible involvement in multiprotein complexes. In this review, an attempt is made to highlight the salient characteristics of the existing strategies with particular attention to their strengths and weaknesses. (C) 2003 Wiley Periodicals, Inc.
引用
收藏
页码:287 / 302
页数:16
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