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核苷酸切除修复过程中的组蛋白修饰与染色质重塑

Histone modification and chromatin remodeling during NER.

作者信息

Waters Raymond, van Eijk Patrick, Reed Simon

机构信息

Institute of Cancer and Genetics, School of Medicine, Cardiff University, Heath Park, Cardiff CF14 4XN, UK; College of Medicine, Swansea University, Singleton Park, Swansea SA2 8PP, UK.

Institute of Cancer and Genetics, School of Medicine, Cardiff University, Heath Park, Cardiff CF14 4XN, UK.

出版信息

DNA Repair (Amst). 2015 Dec;36:105-113. doi: 10.1016/j.dnarep.2015.09.013. Epub 2015 Sep 16.

DOI:10.1016/j.dnarep.2015.09.013
PMID:26422133
Abstract

Here we review our developments of and results with high resolution studies on global genome nucleotide excision repair (GG-NER) in Saccharomyces cerevisiae. Technologies were developed to examine NER at nucleotide resolution in yeast sequences of choice and to determine how these related to local changes in chromatin. We focused on how GG-NER relates to histone acetylation for its functioning and we identified the histone acetyltransferase Gcn5 and acetylation at lysines 9/14 of histone H3 as a major factor in enabling efficient repair. Factors influencing this Gcn5-mediated event are considered which include Rad16, a GG-NER specific SWI/SNF factor and the yeast histone variant of H2AZ (Htz1). We describe results employing primarily MFA2 as a model gene, but also those with URA3 located at subtelomeric sequences. In the latter case we also see a role for acetylation at histone H4. We then consider the development of a high resolution genome-wide approach that enables one to examine correlations between histone modifications and the NER of UV-induced cyclobutane pyrimidine dimers throughout entire yeast genome. This is an approach that will enable rapid advances in understanding the complexities of how compacted chromatin in chromosomes is processed to access DNA damage before it is returned to its pre-damaged status to maintain epigenetic codes.

摘要

在此,我们回顾了我们在酿酒酵母全基因组核苷酸切除修复(GG-NER)的高分辨率研究方面的进展及成果。我们开发了相关技术,以核苷酸分辨率检测酵母特定序列中的核苷酸切除修复,并确定其与染色质局部变化的关系。我们重点研究了GG-NER在功能上如何与组蛋白乙酰化相关联,并确定组蛋白乙酰转移酶Gcn5以及组蛋白H3赖氨酸9/14位点的乙酰化是实现高效修复的主要因素。我们还考虑了影响Gcn5介导事件的因素,包括GG-NER特异性SWI/SNF因子Rad16和组蛋白H2A的酵母组蛋白变体(Htz1)。我们描述了主要以MFA2作为模型基因的研究结果,以及位于亚端粒序列的URA3的研究结果。在后一种情况下,我们还发现组蛋白H4乙酰化也发挥了作用。然后,我们考虑开发一种全基因组高分辨率方法,该方法能够检测整个酵母基因组中组蛋白修饰与紫外线诱导的环丁烷嘧啶二聚体的核苷酸切除修复之间的相关性。这种方法将有助于快速推进对染色体中紧密染色质如何在恢复到损伤前状态以维持表观遗传密码之前被处理以修复DNA损伤这一复杂过程的理解。

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