Quantitative protein profiling is an essential part of proteomics and requires new technologies that accurately, reproducibly, and comprehensively identify and quantify the proteins contained in biological samples. We describe a new strategy for quantitative protein profiling that is based on the separation of proteins labeled with isotopecoded affinity tag reagents by two-dimensional gel electrophoresis and their identification and quantification by mass spectrometry. The method is based on the observation that proteins labeled with isotopically different isotope-coded affinity tag reagents precisely co-migrate during two-dimensional gel electrophoresis and that therefore two or more isotopically encoded samples can be separated concurrently in the same gel. By analyzing changes in the proteome of yeast (Saccharomyces cerevisiae) induced by a metabolic shift we show that this simple method accurately quantifies changes in protein abundance even in cases in which multiple proteins migrate to the same gel coordinates. The method is particularly useful for the quantitative analysis and structural characterization of differentially processed or post-translationally modified forms of a protein and is therefore expected to find wide application in proteomics research.
机构:Univ Calif San Francisco, Dept Pharmaceut Chem, San Francisco, CA 94143 USA
Clauser, KR
Baker, P
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机构:Univ Calif San Francisco, Dept Pharmaceut Chem, San Francisco, CA 94143 USA
Baker, P
Burlingame, AL
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机构:
Univ Calif San Francisco, Dept Pharmaceut Chem, San Francisco, CA 94143 USAUniv Calif San Francisco, Dept Pharmaceut Chem, San Francisco, CA 94143 USA
机构:Univ Calif San Francisco, Dept Pharmaceut Chem, San Francisco, CA 94143 USA
Clauser, KR
Baker, P
论文数: 0引用数: 0
h-index: 0
机构:Univ Calif San Francisco, Dept Pharmaceut Chem, San Francisco, CA 94143 USA
Baker, P
Burlingame, AL
论文数: 0引用数: 0
h-index: 0
机构:
Univ Calif San Francisco, Dept Pharmaceut Chem, San Francisco, CA 94143 USAUniv Calif San Francisco, Dept Pharmaceut Chem, San Francisco, CA 94143 USA