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核小体组装与基因组完整性:复制叉是纽带。

Nucleosome assembly and genome integrity: The fork is the link.

作者信息

Prado Félix, Clemente-Ruiz Marta

机构信息

Departamento de Biología Molecular; Centro Andaluz de Biología Molecular y Medicina Regenerativa (CABIMER); Consejo Superior de Investigaciones Científicas (CSIC); Seville, Spain.

出版信息

Bioarchitecture. 2012 Jan 1;2(1):6-10. doi: 10.4161/bioa.19737.

Abstract

Maintaining the stability of the replication forks is one of the main tasks of the DNA damage response. Specifically, checkpoint mechanisms detect stressed forks and prevent their collapse. In the published report reviewed here we have shown that defective chromatin assembly in cells lacking either H3K56 acetylation or the chromatin assembly factors CAF1 and Rtt106 affects the integrity of advancing replication forks, despite the presence of functional checkpoints. This loss of replication intermediates is exacerbated in the absence of Rad52, suggesting that collapsed forks are rescued by homologous recombination and providing an explanation for the accumulation of recombinogenic DNA damage displayed by these mutants. These phenotypes mimic those obtained by a partial reduction in the pool of available histones and are consistent with a model in which defective histone deposition uncouples DNA synthesis and nucleosome assembly, thus making the fork more susceptible to collapse. Here, we review these findings and discuss the possibility that defects in the lagging strand represent a major source of fork instability in chromatin assembly mutants.

摘要

维持复制叉的稳定性是DNA损伤应答的主要任务之一。具体而言,检查点机制可检测到处于应激状态的复制叉并防止其崩溃。在本文所综述的已发表报告中,我们发现,在缺乏H3K56乙酰化或染色质组装因子CAF1和Rtt106的细胞中,尽管存在功能性检查点,但有缺陷的染色质组装仍会影响前进中的复制叉的完整性。在缺乏Rad52的情况下,复制中间体的这种损失会加剧,这表明崩溃的复制叉可通过同源重组得到挽救,并为这些突变体所显示的重组性DNA损伤的积累提供了解释。这些表型与通过部分减少可用组蛋白池所获得的表型相似,并且与一种模型一致,在该模型中,有缺陷的组蛋白沉积使DNA合成与核小体组装解偶联,从而使复制叉更容易崩溃。在此,我们回顾这些发现,并讨论后随链缺陷可能是染色质组装突变体中复制叉不稳定的主要来源这一可能性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6074/3383716/5eb09ff709ed/bioa-2-6-g1.jpg

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