STUDIES INTO THE IDENTITY OF THE SITES OF INSULIN-STIMULATED INSULIN-RECEPTOR SERINE PHOSPHORYLATION - CHARACTERIZATION OF SYNTHETIC PEPTIDE-SUBSTRATES FOR THE INSULIN-STIMULATED INSULIN-RECEPTOR SERINE KINASE

被引:11
作者
CARTER, WG [1 ]
ASAMOAH, KA [1 ]
SALE, GJ [1 ]
机构
[1] UNIV SOUTHAMPTON,SCH BIOL SCI,DEPT BIOCHEM,SOUTHAMPTON SO16 7PX,HANTS,ENGLAND
关键词
D O I
10.1021/bi00029a025
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The identity of the sites of insulin-stimulated serine phosphorylation in the human insulin receptor was examined by synthesizing peptides that together encompassed all the serine residues of the cytosolic portion of the beta-subunit and testing them as substrates for phosphorylation by a preparation of human insulin receptor copurified with insulin-stimulated insulin receptor serine kinase activity. Of the 14 peptides studied, only 4 (1071-1080, 1290-1298, 1253-1271, and 1313-1329) were phosphorylated on serine, with the serine phosphorylation stimulated 2-4-fold by insulin. Peptides 1071-1080 and 1290-1298 were 3-7-fold better substrates for the serine phosphorylation than the other serine-phosphorylated peptides. Peptides 1071-1080 and 1313-1329 also exhibited insulin-stimulated phosphorylation on tyrosine. Two-dimensional thin-layer tryptic mapping of the phosphorylated insulin receptor/insulin-stimulated insulin receptor serine kinase preparation or of insulin receptor phosphorylated in human Hep G2 cells yielded two major peptides, called S1 and S2, that ran as a pair of closely migrating spots, and other lesser peptides that contained phosphoserine. S1 and S2 also contained some phosphotyrosine and gave phosphoserine/phosphotyrosine ratios of similar to 6 and 0.96-1.50 for the in vivo and in vitro labeled receptor, respectively. S1 and S2 were not cleaved by V8, Of the serine-phosphorylated peptides, only 1290-1298 and 1071-1080 should be Vs resistant; 1290-1298 contains serine sites 1293/4 and migrated distinctly from S1 and S2 in tryptic maps. Peptide 1071-1080 mimicked the production of S1 and S2 in tryptic maps yielding a doublet of phosphopeptides, each containing phosphoserine and phosphotyrosine, which comigrated exactly with S1 and S2. Comigration was confirmed at a different pH and by mixing experiments. Radiosequenation showed that serine 1078 was phosphorylated. Tyrosine 1075 was also phosphorylated, but it was no more than a minor site in vivo, It is concluded that serine 1078 of the insulin receptor is a major site of insulin-stimulated phosphorylation in vivo and in vitro. The peptide sequences provide a range of substrates to facilitate the study, purification, and characterization of the insulin-stimulated insulin receptor serine kinase or kinases, and the identification of a major site of insulin-stimulated serine phosphorylation will help elucidate the function of the insulin receptor serine phosphorylation.
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页码:9488 / 9499
页数:12
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