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紫外线诱导的DNA损伤后,DDB2与PCNA的结合是其降解所必需的。

DDB2 association with PCNA is required for its degradation after UV-induced DNA damage.

作者信息

Cazzalini Ornella, Perucca Paola, Mocchi Roberto, Sommatis Sabrina, Prosperi Ennio, Stivala Lucia Anna

机构信息

Dipartimento di Medicina Molecolare; Unità di Immunologia e Patologia Generale; Università di Pavia; Pavia, Italy.

Istituto di Genetica Molecolare (IGM) del CNR; Pavia, Italy.

出版信息

Cell Cycle. 2014;13(2):240-8. doi: 10.4161/cc.26987. Epub 2013 Nov 4.

Abstract

DDB2 is a protein playing an essential role in the lesion recognition step of the global genome sub-pathway of nucleotide excision repair (GG-NER) process. Among the proteins involved in the DNA damage response, p21(CDKN1A) (p21) has been reported to participate in NER, but also to be removed by proteolytic degradation, thanks to its association with PCNA. DDB2 is involved in the CUL4-DDB1 complex mediating p21 degradation; however, the direct interaction between DDB2, p21 and PCNA has been never investigated. Here, we show that DDB2 co-localizes with PCNA and p21 at local UV-induced DNA-damage sites, and these proteins co-immunoprecipitate in the same complex. In addition, we provide evidence that p21 is not able to bind directly DDB2, but, to this end, the presence of PCNA is required. Direct physical association of recombinant DDB2 protein with PCNA is mediated by a conserved PIP-box present in the N-terminal region of DDB2. Mutation of the PIP-box resulted in the loss of protein interaction. Interestingly, the same mutation, or depletion of PCNA by RNA interference, greatly impaired DDB2 degradation induced by UV irradiation. These results indicate that DDB2 is a PCNA-binding protein, and that this association is required for DDB2 proteolytic degradation.

摘要

DDB2是一种在核苷酸切除修复(GG-NER)过程的全基因组子途径的损伤识别步骤中发挥关键作用的蛋白质。在参与DNA损伤反应的蛋白质中,p21(CDKN1A)(p21)已被报道参与核苷酸切除修复,但由于其与增殖细胞核抗原(PCNA)的关联,也会通过蛋白水解降解而被清除。DDB2参与介导p21降解的CUL4-DDB1复合物;然而,DDB2、p21和PCNA之间的直接相互作用从未被研究过。在这里,我们表明DDB2与PCNA和p21在局部紫外线诱导的DNA损伤位点共定位,并且这些蛋白质在同一复合物中进行共免疫沉淀。此外,我们提供证据表明p21不能直接与DDB2结合,但为此需要PCNA的存在。重组DDB2蛋白与PCNA的直接物理结合是由DDB2 N端区域中存在的保守PIP框介导的。PIP框的突变导致蛋白质相互作用丧失。有趣的是,相同的突变或通过RNA干扰使PCNA缺失,极大地损害了紫外线照射诱导的DDB2降解。这些结果表明DDB2是一种PCNA结合蛋白,并且这种关联是DDB2蛋白水解降解所必需的。

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