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组蛋白H3变体决定染色质组装模式。

Histone H3 variants specify modes of chromatin assembly.

作者信息

Ahmad Kami, Henikoff Steven

机构信息

Fred Hutchinson Cancer Research Center, 1100 Fairview Avenue North, A1-162, Seattle, WA 98109, USA.

出版信息

Proc Natl Acad Sci U S A. 2002 Dec 10;99 Suppl 4(Suppl 4):16477-84. doi: 10.1073/pnas.172403699. Epub 2002 Aug 12.

DOI:10.1073/pnas.172403699
PMID:12177448
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC139911/
Abstract

Histone variants have been known for 30 years, but their functions and the mechanism of their deposition are still largely unknown. Drosophila has three versions of histone H3. H3 packages the bulk genome, H3.3 marks active chromatin and may be essential for gene regulation, and Cid is the characteristic structural component of centromeric chromatin. We have characterized the properties of these histones by using a Drosophila cell-line system that allows precise analysis of both DNA replication and histone deposition. The deposition of H3 is restricted to replicating DNA. In striking contrast, H3.3 and Cid deposit throughout the cell cycle. Deposition of H3.3 occurs without any corresponding DNA replication. To confirm that the deposition of Cid is also replication-independent (RI), we examined centromere replication in cultured cells and neuroblasts. We found that centromeres replicate out of phase with heterochromatin and display replication patterns that may limit H3 deposition. This confirms that both variants undergo RI deposition, but at different locations in the nucleus. How variant histones accomplish RI deposition is unknown, and raises basic questions about the stability of nucleosomes, the machinery that accomplishes nucleosome assembly, and the functional organization of the nucleus. The different in vivo properties of H3, H3.3, and Cid set the stage for identifying the mechanisms by which they are differentially targeted. Here we suggest that local effects of "open" chromatin and broader effects of nuclear organization help to guide the two different H3 variants to their target sites.

摘要

组蛋白变体已被发现30年了,但其功能及其沉积机制仍大多未知。果蝇有三种组蛋白H3变体。H3包裹大部分基因组,H3.3标记活性染色质且可能对基因调控至关重要,而Cid是着丝粒染色质的特征性结构成分。我们通过使用一种果蝇细胞系系统来表征这些组蛋白的特性,该系统能够精确分析DNA复制和组蛋白沉积。H3的沉积仅限于正在复制的DNA。与之形成鲜明对比的是,H3.3和Cid在整个细胞周期中都有沉积。H3.3的沉积在没有任何相应DNA复制的情况下发生。为了证实Cid的沉积也是不依赖复制(RI)的,我们研究了培养细胞和成神经细胞中的着丝粒复制。我们发现着丝粒与异染色质不同步复制,并呈现出可能限制H3沉积的复制模式。这证实了这两种变体都经历RI沉积,但在细胞核的不同位置。变体组蛋白如何完成RI沉积尚不清楚,这也引发了关于核小体稳定性、完成核小体组装的机制以及细胞核功能组织的基本问题。H3、H3.3和Cid在体内的不同特性为确定它们被差异靶向的机制奠定了基础。在这里我们提出,“开放”染色质的局部效应和核组织的更广泛效应有助于将两种不同的H3变体引导至其靶位点。

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本文引用的文献

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The histone variant H3.3 marks active chromatin by replication-independent nucleosome assembly.组蛋白变体H3.3通过不依赖复制的核小体组装标记活性染色质。
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