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在DNA损伤检查点启动过程中,检查点钳激活Mec1激酶。

The checkpoint clamp activates Mec1 kinase during initiation of the DNA damage checkpoint.

作者信息

Majka Jerzy, Niedziela-Majka Anita, Burgers Peter M J

机构信息

Department of Biochemistry and Molecular Biophysics, Washington University School of Medicine, St. Louis, Missouri 63110, USA.

出版信息

Mol Cell. 2006 Dec 28;24(6):891-901. doi: 10.1016/j.molcel.2006.11.027.

Abstract

Yeast Mec1/Ddc2 protein kinase, the ortholog of human ATR/ATRIP, plays a central role in the DNA damage checkpoint. The PCNA-like clamp Rad17/Mec3/Ddc1 (the 9-1-1 complex in human) and its loader Rad24-RFC are also essential components of this signal transduction pathway. Here we have studied the role of the clamp in regulating Mec1, and we delineate how the signal generated by DNA lesions is transduced to the Rad53 effector kinase. The checkpoint clamp greatly activates the kinase activity of Mec1, but only if the clamp is appropriately loaded upon partial duplex DNA. Activated Mec1 phosphorylates the Ddc1 and Mec3 subunits of the clamp, the Rad24 subunit of the loader, and the Rpa1 and Rpa2 subunits of RPA. Phosphorylation of Rad53, and of human PHAS-1, a nonspecific target, also requires a properly loaded clamp. Phosphorylation and binding studies with individual clamp subunits indicate that the Ddc1 subunit mediates the functional interactions with Mec1.

摘要

酵母Mec1/Ddc2蛋白激酶是人类ATR/ATRIP的直系同源物,在DNA损伤检查点中起核心作用。类增殖细胞核抗原(PCNA)钳夹蛋白Rad17/Mec3/Ddc1(人类中的9-1-1复合物)及其加载因子Rad24-RFC也是该信号转导途径的重要组成部分。在此,我们研究了钳夹蛋白在调节Mec1中的作用,并阐述了DNA损伤产生的信号是如何转导至Rad53效应激酶的。检查点钳夹蛋白极大地激活了Mec1的激酶活性,但前提是该钳夹蛋白要适当地加载到部分双链DNA上。被激活的Mec1会磷酸化钳夹蛋白的Ddc1和Mec3亚基、加载因子的Rad24亚基以及复制蛋白A(RPA)的Rpa1和Rpa2亚基。Rad53以及非特异性靶点人类PHAS-1的磷酸化也需要一个加载正确的钳夹蛋白。对单个钳夹蛋白亚基的磷酸化和结合研究表明,Ddc1亚基介导了与Mec1的功能相互作用。

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