PHOSPHOPEPTIDE MAPPING AND PHOSPHOAMINO ACID ANALYSIS BY ELECTROPHORESIS AND CHROMATOGRAPHY ON THIN-LAYER CELLULOSE PLATES

被引:117
作者
VANDERGEER, P [1 ]
HUNTER, T [1 ]
机构
[1] SALK INST BIOL STUDIES, MOLEC BIOL & VIROL LAB, LA JOLLA, CA 92037 USA
关键词
D O I
10.1002/elps.1150150173
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Identification of protein phosphorylation sites is essential in order to evaluate the contribution of individual sites to the regulation of a particular protein by phosphorylation. Here we review a method we have developed for the identification of phosphorylation sites based on digestion of P-32-labeled proteins with site-specific proteases and separation of the digestion products in two dimensions on thin-layer cellulose plates using electrophoresis in the first dimension followed by chromatography. This method is very sensitive, requiring only a few hundred P-32-disintegrations per minute to obtain reproducible phosphopeptide maps. We also report methods for the analysis of the phosphoamino acid content of both intact phosphoproteins and individual phosphopeptides recovered from two-dimensional separations, in which the material is subjected to partial acid hydrolysis, and the hydrolysis products are separated on thin-layer cellulose plates by electrophoresis in one or two dimensions. Finally, we describe methods for analyzing the structure of isolated phosphopeptides by secondary digestion with site-specific proteases, by manual Edman degradation, and by immunoprecipitation, and indicate how this information can be used in conjunction with the two-dimensional mobility of the peptide to deduce the identity of a phosphopeptide from the known sequence of a protein.
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收藏
页码:544 / 554
页数:11
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