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p34cdc2/p33cdk2激活激酶p40MO15的细胞周期调控

Cell cycle regulation of the p34cdc2/p33cdk2-activating kinase p40MO15.

作者信息

Poon R Y, Yamashita K, Howell M, Ershler M A, Belyavsky A, Hunt T

机构信息

Imperial Cancer Research Fund, Clare Hall Laboratories, South Mimms, Herts, UK.

出版信息

J Cell Sci. 1994 Oct;107 ( Pt 10):2789-99. doi: 10.1242/jcs.107.10.2789.

Abstract

A key component of Cdc2/Cdk2-activating kinase (CAK) is p40MO15, a protein kinase subunit that phosphorylates the T161/T160 residues of p34cdc2/p33cdk2. The level and activity of p40MO15 were essentially constant during cleavage of fertilised Xenopus eggs and in growing mouse 3T3 cells, but serum starvation of these cells reduced both the level and activity of p40MO15. Although the level and activity of endogenous p40MO15 did not vary in the cell cycle, we found that bacterially expressed p40MO15 was activated more rapidly by M-phase cell extracts than by interphase cell extracts. Bacterially expressed p40MO15 was phosphorylated mainly on serine 170 (a p34cdc2 phosphorylation site) by mitotic cell extracts, but mutation of S170 to alanine did not affect the activation of p40MO15, whereas mutation of T176 (the equivalent site to T161/T160 in p34cdc2/p33cdk2) abolished the activation of P40MO15. These studies suggest that the level and activity of p40MO15 is probably not a major determinant of p34cdc2/p33cdk2 activity in the cell cycle, and that the activation of p40MO15 may require phosphorylation on T176.

摘要

细胞周期蛋白依赖性激酶2激活激酶(CAK)的一个关键组分是p40MO15,它是一种蛋白激酶亚基,可磷酸化p34cdc2/p33cdk2的T161/T160残基。在非洲爪蟾受精卵的卵裂过程中以及在生长的小鼠3T3细胞中,p40MO15的水平和活性基本保持恒定,但这些细胞的血清饥饿会降低p40MO15的水平和活性。尽管内源性p40MO15的水平和活性在细胞周期中没有变化,但我们发现,与间期细胞提取物相比,M期细胞提取物能更快地激活细菌表达的p40MO15。有丝分裂细胞提取物主要在丝氨酸170(p34cdc2的一个磷酸化位点)上使细菌表达的p40MO15发生磷酸化,但将S170突变为丙氨酸并不影响p40MO15的激活,而将T176(p34cdc2/p33cdk2中与T161/T160相当的位点)突变则消除了p40MO15的激活。这些研究表明,p40MO15的水平和活性可能不是细胞周期中p34cdc2/p33cdk2活性的主要决定因素,并且p40MO15的激活可能需要T176位点的磷酸化。

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