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首页> 外文期刊>Frontiers in Cell and Developmental Biology >USP44 Stabilizes DDB2 to Facilitate Nucleotide Excision Repair and Prevent Tumors
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USP44 Stabilizes DDB2 to Facilitate Nucleotide Excision Repair and Prevent Tumors

机译:USP44稳定DDB2以促进核苷酸切除修复和预防肿瘤

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Nucleotide excision repair (NER) is a pathway involved in the repair of a variety of potentially mutagenic lesions that distort the DNA double helix. The ubiquitin E3-ligase complex UV-DDB is required for the recognition and repair of UV-induced cyclobutane pyrimidine dimers (CPDs) lesions through NER. DDB2 directly binds CPDs and subsequently undergoes ubiquitination and proteasomal degradation. DDB2 must remain on damaged chromatin, however, for sufficient time to recruit and hand-off lesions to XPC, a factor essential in the assembly of downstream repair components. Here we show that the tumor suppressor USP44 directly deubiquitinates DDB2 to prevent its premature degradation and is selectively required for CPD repair. Cells lacking USP44 have impaired DDB2 accumulation on DNA lesions with subsequent defects in XPC retention. The physiological importance of this mechanism is evident in that mice lacking Usp44 are prone to tumors induced by NER lesions introduced by DMBA or UV light. These data reveal the requirement for highly regulated ubiquitin addition and removal in the recognition and repair of helix-distorting DNA damage and identify another mechanism by which USP44 protects genomic integrity and prevents tumors.
机译:核苷酸切除修复(ner)是一种涉及修复各种潜在的诱变病变的途径,扭曲DNA双螺旋。泛素E3-Cigase复合酶复合UV-DDB是通过Ner识别和修复UV诱导的环丁烷嘧啶二聚体(CPD)病变的识别和修复。 DDB2直接结合CPD,随后经过泛素化和蛋白酶体降解。 DDB2必须保持在受损的染色质上,然而,对于足够的时间来募集和切除损伤到XPC,这是下游修复部件组装中必需的因素。在这里,我们表明肿瘤抑制器USP44直接脱硫蛋白酶DDB2,以防止其过早降解,并选择性地需要CPD修复。缺乏USP44的细胞对DNA病变的DDB2积累受损,随后XPC潴留缺陷。这种机制的生理重要性在缺乏USP44的小鼠中是易于由DMBA或UV光引入的鼻病变诱导的肿瘤。这些数据揭示了对高度监管的泛素添加和去除在螺旋扭曲DNA损伤的识别和修复中的要求,并确定USP44保护基因组完整性并防止肿瘤的另一种机制。

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