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DNA损伤介导的转录停滞:以退为进。

DNA damage mediated transcription arrest: Step back to go forward.

作者信息

Mullenders Leon

机构信息

Department of Human Genetics, Leiden University Medical Center, Leiden, The Netherlands.

出版信息

DNA Repair (Amst). 2015 Dec;36:28-35. doi: 10.1016/j.dnarep.2015.09.005. Epub 2015 Sep 10.

Abstract

The disturbance of DNA helix conformation by bulky DNA damage poses hindrance to transcription elongating due to stalling of RNA polymerase at transcription blocking lesions. Stalling of RNA polymerase provokes the formation of R-loops, i.e. the formation of a DNA-RNA hybrid and a displaced single stranded DNA strand as well as displacement of spliceosomes. R-loops are processed into DNA single and double strand breaks by NER factors depending on TC-NER factors leading to genome instability. Moreover, stalling of RNA polymerase induces a strong signal for cell cycle arrest and apoptosis. These toxic and mutagenic effects are counteracted by a rapid recruitment of DNA repair proteins to perform transcription coupled nucleotide excision repair (TC-NER) to remove the blocking DNA lesions and to restore transcription. Recent studies have highlighted the role of backtracking of RNA polymerase to facilitate TC-NER and identified novel factors that play key roles in TC-NER and in restoration of transcription. On the molecular level these factors facilitate stability of the repair complex by promotion and regulation of various post-translational modifications of NER factors and chromatin substrate. In addition, the continuous flow of new factors that emerge from screening assays hints to several regulatory levels to safeguard the integrity of transcription elongation after disturbance by DNA damage that have yet to be explored.

摘要

由于RNA聚合酶在转录阻断损伤处停滞,大分子DNA损伤导致的DNA螺旋构象紊乱会阻碍转录延伸。RNA聚合酶的停滞会引发R环的形成,即DNA-RNA杂交体、置换的单链DNA链的形成以及剪接体的置换。R环由依赖于TC-NER因子的NER因子加工成DNA单链和双链断裂,导致基因组不稳定。此外,RNA聚合酶的停滞会诱导细胞周期停滞和凋亡的强烈信号。这些毒性和诱变作用可通过快速招募DNA修复蛋白来进行转录偶联核苷酸切除修复(TC-NER)来抵消,以去除阻断性DNA损伤并恢复转录。最近的研究强调了RNA聚合酶回溯在促进TC-NER中的作用,并鉴定了在TC-NER和转录恢复中起关键作用的新因子。在分子水平上,这些因子通过促进和调节NER因子和染色质底物的各种翻译后修饰来促进修复复合物的稳定性。此外,从筛选试验中不断涌现的新因子提示了几个调节水平,以保护DNA损伤干扰后转录延伸的完整性,而这些调节水平尚未被探索。

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