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酵母中核小体DNA在第二个时间尺度上的快速可及性。

Rapid accessibility of nucleosomal DNA in yeast on a second time scale.

作者信息

Bucceri Andrea, Kapitza Kristin, Thoma Fritz

机构信息

Institut für Zellbiologie, ETH Zürich, Zürich, Switzerland.

出版信息

EMBO J. 2006 Jul 12;25(13):3123-32. doi: 10.1038/sj.emboj.7601196. Epub 2006 Jun 15.

Abstract

Packaging DNA in nucleosomes and higher-order chromatin structures restricts its accessibility and constitutes a barrier for all DNA transactions including gene regulation and DNA repair. How and how fast proteins find access to DNA buried in chromatin of living cells is poorly understood. To address this question in a real time in vivo approach, we investigated DNA repair by photolyase in yeast. We show that overexpressed photolyase, a light-dependent DNA-repair enzyme, recognizes and repairs UV-damaged DNA within seconds. Rapid repair was observed in various nucleosomal regions of the genome including inactive and active genes and repressed promoters. About 50% of cyclobutane pyrimidine dimers were removed in 5 s, >80% in 90 s. Heterochromatin was repaired within minutes, centromeres were not repaired. Consistent with fast conformational transitions of nucleosomes observed in vitro, this rapid repair strongly suggests that spontaneous unwrapping of nucleosomes rather than histone dissociation or chromatin remodeling provides DNA access. The data impact our view on the repressive and dynamic nature of chromatin and illustrate how proteins like photolyase can access DNA in structurally and functionally diverse chromatin regions.

摘要

将DNA包装在核小体和更高阶的染色质结构中会限制其可及性,并对包括基因调控和DNA修复在内的所有DNA相关活动构成障碍。目前对于蛋白质如何以及多快能够找到埋在活细胞染色质中的DNA,我们还知之甚少。为了通过实时体内实验方法解决这个问题,我们研究了酵母中光解酶介导的DNA修复过程。我们发现,过表达的光解酶(一种光依赖的DNA修复酶)能够在数秒内识别并修复紫外线损伤的DNA。在基因组的各种核小体区域,包括沉默基因、活跃基因和受抑制的启动子区域,均观察到了快速修复现象。约50%的环丁烷嘧啶二聚体在5秒内被去除,90秒内超过80%被去除。异染色质在数分钟内得以修复,而着丝粒则未被修复。这一快速修复现象与体外观察到的核小体快速构象转变一致,强烈表明核小体的自发解旋而非组蛋白解离或染色质重塑为DNA提供了可及性。这些数据影响了我们对染色质抑制性和动态性质的看法,并说明了像光解酶这样的蛋白质如何能够在结构和功能各异的染色质区域中接触到DNA。

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