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腺病毒2型DNA结合蛋白磷酸部分的进一步特性研究。

Further characterization of the phosphate moiety of the adenovirus type 2 DNA-binding protein.

作者信息

Linné T, Philipson L

出版信息

Eur J Biochem. 1980 Jan;103(2):259-70. doi: 10.1111/j.1432-1033.1980.tb04310.x.

DOI:10.1111/j.1432-1033.1980.tb04310.x
PMID:6244944
Abstract

The adenovirus type 2 DNA-binding protein is phosphorylated. Alkaline phosphatase treatment removes phosphate groups resulting in a decrease in molecular weight from 72000 to 70000. The dephosphorylated protein binds to single-stranded and double-stranded DNA as well as the phosphorylated protein does. Controlled chymotrypsin treatment cleaves the DNA-binding protein into two subspecies of Mr about 45000 and 25000. The 45000-Mr polypeptide contains most of the methionine residues but no phosphate and binds to DNA. The 25000-Mr polypeptide contains all the phosphate groups and shows no binding to DNA. Isoelectric focusing gels show heterogeneity of the DNA-binding protein and 15 subspecies with different charges can be observed after partial dephosphorylation by alkaline phosphatase. After extensive dephosphorylation two or three basic species with a molecular weight around 70000 are observed. Quantitative immunoprecipitation from cells labeled to equilibrium with inorganic 32PO4 gives a molar ratio of phosphate to protein of 4--7 and direct chemical determination of the phosphate residues yields 4 mol Pi/mol protein. These results suggest that there exist subspecies of the protein moiety of the adenovirus DNA-binding protein. The DNA-binding protein isolated from infected cells after a short 'pulse' of [35S]methionine has a molecular weight which corresponds to that of the dephosphorylated protein. After a 'chase' period the molecular weight increases to 72000, but alkaline phosphatase treatment converts it to a species with the same molecular weight as the newly synthesized DNA-binding protein, indicating that the modification of the protein is due to phosphorylation.

摘要

腺病毒2型DNA结合蛋白发生了磷酸化。碱性磷酸酶处理可去除磷酸基团,导致分子量从72000降至70000。去磷酸化的蛋白与单链和双链DNA的结合能力与磷酸化蛋白相同。用胰凝乳蛋白酶进行可控处理可将DNA结合蛋白切割成两个亚类,分子量分别约为45000和25000。分子量为45000的多肽含有大部分甲硫氨酸残基,但不含磷酸基团,能与DNA结合。分子量为25000的多肽含有所有磷酸基团,不与DNA结合。等电聚焦凝胶显示DNA结合蛋白具有异质性,碱性磷酸酶部分去磷酸化后可观察到15种带不同电荷的亚类。广泛去磷酸化后,可观察到两三种分子量约为70000的碱性蛋白。用无机32PO4标记细胞至平衡后进行定量免疫沉淀,得到的磷酸与蛋白的摩尔比为4 - 7,直接化学测定磷酸残基得到的结果是每摩尔蛋白含4摩尔无机磷酸。这些结果表明腺病毒DNA结合蛋白的蛋白部分存在亚类。用[35S]甲硫氨酸进行短时间“脉冲”标记后,从感染细胞中分离出的DNA结合蛋白的分子量与去磷酸化蛋白的分子量相对应。“追踪”一段时间后,分子量增加到72000,但碱性磷酸酶处理可将其转化为与新合成的DNA结合蛋白分子量相同的一种蛋白,这表明蛋白的修饰是由于磷酸化所致。

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