IDENTIFICATION OF THE THREONINE PHOSPHORYLATION SITES ON THE POLYOMAVIRUS MAJOR CAPSID PROTEIN VP1 - RELATIONSHIP TO THE ACTIVITY OF MIDDLE T-ANTIGEN

被引:23
|
作者
LI, ML
GARCEA, RL
机构
[1] DANA FARBER CANC INST,DIV PEDIAT ONCOL,BOSTON,MA 02115
[2] CHILDRENS HOSP,BOSTON,MA 02115
关键词
D O I
10.1128/JVI.68.1.320-327.1994
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
Phosphorylation of the polyomavirus major capsid protein VP1 nas examined after in vivo P-32 labeling of virus-infected cells. Two phosphorylated peptide fragments of VP1 were identified by protease digestion, high-performance liquid chromatography purification, mass spectrometry, and N-terminal sequencing. The peptides from residues 58 to 78 and residues 153 to 173 were phosphorylated on threonine. Site-directed mutations were introduced at these threonine sites, and mutant viruses were reconstructed. A threonine-to-glycine change at residue 63 (mutant G63) and a threonine-to-alanine change at residue 156 (mutant A156) resulted in viruses defective in phosphorylation of the respective peptides after in vivo labeling. Growth of the mutant G63 virus was similar to that of the wild-type virus, but the mutant A156 was inefficient in assembly of 240S viral particles. Polyomavirus nontransforming host range (hr-t) mutants are defective in VP1 threonine phosphorylation when grown in nonpermissive cells (R. L. Garcea, K. Ballmer-Hofer, and T. L. Benjamin, J. Virol. 54:311-316, 1985). Proteolytic mapping of VP1 peptides after in vivo labeling from hr-t mutant virus infections demonstrated that both residues T-63 and T-156 were affected. These results suggest that the block in virion assembly in hr-t mutant viruses is associated with a defect in phosphorylation of threonine 156.
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页码:320 / 327
页数:8
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