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DNA-蛋白质交联:维护基因组完整性的巨大挑战。

DNA-protein cross-links: Formidable challenges to maintaining genome integrity.

机构信息

Department of Mathematical and Life Sciences, Graduate School of Science, Hiroshima University, Higashi-Hiroshima 739-8526, Japan.

Department of Mathematical and Life Sciences, Graduate School of Science, Hiroshima University, Higashi-Hiroshima 739-8526, Japan.

出版信息

DNA Repair (Amst). 2018 Nov;71:190-197. doi: 10.1016/j.dnarep.2018.08.024. Epub 2018 Aug 23.

DOI:10.1016/j.dnarep.2018.08.024
PMID:30177436
Abstract

DNA is associated with proteins that are involved in its folding and transaction processes. When cells are exposed to chemical cross-linking agents or free radical-generating ionizing radiation, DNA-associated proteins are covalently trapped within the DNA to produce DNA-protein cross-links (DPCs). DPCs produced by these agents contain cross-linked proteins in an undisrupted DNA strand. Some DNA-metabolizing enzymes that form covalent reaction intermediates can also be irreversibly trapped in the presence of inhibitors or DNA damage to give rise to abortive DPCs. The abortive DPCs often contain cross-linked proteins attached to the 5' or 3' end of a DNA strand break. In vitro studies show that steric hindrance caused by cross-linked proteins impedes the progression of DNA helicases and polymerases and of RNA polymerases. The modes and consequences by which DPCs impede replication and transcription processes are considerably different from those with conventional DNA lesions. Thus, DPCs are formidable challenges to maintaining genome integrity and faithful gene expression. Current models of DPC repair involve direct and indirect removal of DPCs. The direct mechanism works for DPCs that contain topoisomerase 2 attached to the 5' end of DNA. The Mre11-Rad50-Nbs1 complex cleaves the site internal to the DPC and directly releases a DPC-containing oligonucleotide. The indirect mechanism involves degradation of cross-linked proteins by proteasomes or the recently identified DPC proteases Wss1 and Sprtn to relieve steric hindrance of DPCs. The resulting peptide-cross-links might be processed by translesion synthesis or other canonical repair mechanisms: however, the exact mechanism remains to be elucidated.

摘要

DNA 与参与其折叠和转录过程的蛋白质相关联。当细胞暴露于化学交联剂或产生自由基的电离辐射时,DNA 相关蛋白会在 DNA 内发生共价捕获,从而产生 DNA-蛋白质交联(DPC)。这些试剂产生的 DPC 含有未被打断的 DNA 链上的交联蛋白。一些形成共价反应中间体的 DNA 代谢酶也可以在抑制剂或 DNA 损伤的存在下被不可逆地捕获,从而产生无功能的 DPC。无功能的 DPC 通常含有交联蛋白附着在 DNA 链断裂的 5'或 3'末端。体外研究表明,交联蛋白引起的空间位阻会阻碍 DNA 解旋酶和聚合酶以及 RNA 聚合酶的前进。DPC 阻碍复制和转录过程的方式和后果与传统的 DNA 损伤有很大的不同。因此,DPC 对维持基因组完整性和忠实基因表达是一个巨大的挑战。目前的 DPC 修复模型涉及 DPC 的直接和间接去除。直接机制适用于拓扑异构酶 2 附着在 DNA 5'末端的 DPC。Mre11-Rad50-Nbs1 复合物切割 DPC 内部的位点,并直接释放含有 DPC 的寡核苷酸。间接机制涉及蛋白酶体或最近发现的 DPC 蛋白酶 Wss1 和 Sprtn 对交联蛋白的降解,以消除 DPC 的空间位阻。由此产生的肽交联可能通过跨损伤合成或其他规范的修复机制进行处理:然而,确切的机制仍有待阐明。

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