蛋白酶体去泛素化酶 POH1 促进双链 DNA 断裂反应。
The proteasomal de-ubiquitinating enzyme POH1 promotes the double-strand DNA break response.
机构信息
School of Cancer Sciences, College of Medical & Dental Sciences, University of Birmingham, Birmingham, UK.
出版信息
EMBO J. 2012 Oct 3;31(19):3918-34. doi: 10.1038/emboj.2012.232. Epub 2012 Aug 21.
Abstract
The regulation of Ubiquitin (Ub) conjugates generated by the complex network of proteins that promote the mammalian DNA double-strand break (DSB) response is not fully understood. We show here that the Ub protease POH1/rpn11/PSMD14 resident in the 19S proteasome regulatory particle is required for processing poly-Ub formed in the DSB response. Proteasome activity is required to restrict tudor domain-dependent 53BP1 accumulation at sites of DNA damage. This occurs both through antagonism of RNF8/RNF168-mediated lysine 63-linked poly-Ub and through the promotion of JMJD2A retention on chromatin. Consistent with this role POH1 acts in opposition to RNF8/RNF168 to modulate end-joining DNA repair. Additionally, POH1 acts independently of 53BP1 in homologous recombination repair to promote RAD51 loading. Accordingly, POH1-deficient cells are sensitive to DNA damaging agents. These data demonstrate that proteasomal POH1 is a key de-ubiquitinating enzyme that regulates ubiquitin conjugates generated in response to damage and that several aspects of the DSB response are regulated by the proteasome.
摘要
泛素(Ub)缀合物的调节由促进哺乳动物 DNA 双链断裂(DSB)反应的蛋白质复杂网络产生,但尚未完全了解。我们在这里表明,驻留在 19S 蛋白酶体调节颗粒中的 Ub 蛋白酶 POH1/rpn11/PSMD14 是 DSB 反应中形成的多 Ub 加工所必需的。蛋白酶体活性对于限制 DNA 损伤部位依赖于 tudor 结构域的 53BP1 积累是必需的。这既通过拮抗 RNF8/RNF168 介导的赖氨酸 63 连接多 Ub 发生,又通过促进 JMJD2A 在染色质上的保留发生。与该作用一致,POH1 与 RNF8/RNF168 相反作用以调节末端连接 DNA 修复。此外,POH1 在同源重组修复中独立于 53BP1 作用以促进 RAD51 加载。因此,POH1 缺陷细胞对 DNA 损伤剂敏感。这些数据表明,蛋白酶体 POH1 是一种关键的去泛素化酶,可调节损伤反应中产生的泛素缀合物,并且 DSB 反应的几个方面受蛋白酶体调节。
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