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首页> 外文期刊>Journal of Virology >p37mos-associated serine/threonine protein kinase activity correlates with the cellular transformation function of v-mos.
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p37mos-associated serine/threonine protein kinase activity correlates with the cellular transformation function of v-mos.

机译:P37MOS相关的丝氨酸/苏氨酸蛋白激酶活性与V-MOS的细胞转化函数相关。

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A serine/threonine-specific protein kinase activity is closely associated with v-mos-encoded proteins. Experiments were conducted with several mutant forms of p37mos to determine whether or not the kinase function correlates with the biological activity of the mutant v-mos genes. Two mutants lacking cell transformation activity, one an arginine substitution for lysine-121 in the putative ATP-binding site and the other a 23-amino acid deletion from the C-terminal end of p37mos, had no kinase activity associated with their mutant proteins. However, a third mutant with reduced biological activity had drastically less kinase activity than the wild-type protein. The latter mutant was able to phosphorylate the kinase-inactive p37mos(Arg-121) protein in vitro. These results indicate that even though p37mos(Arg-121) can be phosphorylated in trans by other kinase molecules, it lacks the ability to phosphorylate itself in vitro. This provides a compelling argument that the protein kinase function of p37mos is an intrinsic property of the protein. Moreover, since the kinase function correlates with the cellular transformation activity of the v-mos gene, we predict that it is required for the biological activity of the v-mos gene.
机译:丝氨酸/苏氨酸特异性蛋白激酶活性与V-MOS编码的蛋白质密切相关。用几种突变形式的P37MOS进行实验以确定激酶功能是否与突变体V-MOS基因的生物活性相关。缺乏细胞转化活性的两个突变体,一种在推定的ATP结合位点中的赖氨酸-121的精氨酸替代物,以及来自P37MOS的C末端的另一种23-氨基酸缺失,没有与其突变蛋白相关的激酶活性。然而,具有降低的生物活性的第三个突变体大于野生型蛋白质的激酶活性。后一种突变体能够在体外磷酸化激酶 - 惰性P37MOS(ARG-121)蛋白。这些结果表明,即使P37MOS(ARG-121)可以通过其他激酶分子在反式中磷酸化,它缺乏在体外磷酸化物质的能力。这提供了令人讨厌的论点,即P37MOS的蛋白激酶功能是蛋白质的内在性质。此外,由于激酶功能与V-MOS基因的细胞转化活性相关,因此我们预测了V-MOS基因的生物活性所需的。

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