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导致人类遗传疾病的复杂多核苷酸取代突变揭示了对跨损伤合成DNA聚合酶作用的新见解。

Complex Multiple-Nucleotide Substitution Mutations Causing Human Inherited Disease Reveal Novel Insights into the Action of Translesion Synthesis DNA Polymerases.

作者信息

Chen Jian-Min, Férec Claude, Cooper David N

机构信息

Institut National de la Santé et de la Recherche Médicale (INSERM), U1078, Brest, France.

Etablissement Français du Sang (EFS) - Bretagne, Brest, France.

出版信息

Hum Mutat. 2015 Nov;36(11):1034-8. doi: 10.1002/humu.22831. Epub 2015 Aug 3.

Abstract

Translesion synthesis (TLS) DNA polymerases allow the bypass of unrepaired lesions during DNA replication. Based upon mutational signatures of a subtype of multiple-nucleotide substitution (MNS) mutations causing human inherited disease, we have recently postulated two properties of TLS DNA polymerases in DNA repair, namely, the generation of neo-microhomologies potentiating strand-misalignment, and additional microlesions within the templated inserts when recruited to stalled replication forks. To provide further support for this postulate, we analyzed the mutational signatures of a new and complex subtype of pathogenic MNS mutation. Several mutations containing long templated inserts (8-19 bp) that are highly informative with regard to their underlying mutational mechanisms, harbor imprints of TLS DNA polymerase action. Dissecting the mechanism underlying the generation of the 19-bp insert implicated repeated participation of TLS DNA polymerases in the conversion of a damaged base into a complex MNS lesion through a process of successive template switching and bypass repair.

摘要

跨损伤合成(TLS)DNA聚合酶可使DNA复制过程中未修复的损伤得以跨越。基于导致人类遗传性疾病的多核苷酸替换(MNS)突变亚型的突变特征,我们最近推测了TLS DNA聚合酶在DNA修复中的两个特性,即产生增强链错配的新微同源性,以及在被招募到停滞的复制叉时模板插入片段内产生额外的微损伤。为了进一步支持这一假设,我们分析了一种新的复杂致病MNS突变亚型的突变特征。几个包含长模板插入片段(8 - 19 bp)的突变,就其潜在的突变机制而言具有高度信息性,带有TLS DNA聚合酶作用的印记。剖析19 bp插入片段产生的潜在机制表明,TLS DNA聚合酶通过连续的模板切换和旁路修复过程,反复参与将受损碱基转化为复杂MNS损伤的过程。

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