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The Rpd3-Sin3 Histone Deacetylase Regulates Replication Timing and Enables Intra-S Origin Control in Saccharomyces cerevisiae

机译:Rpd3-Sin3组蛋白脱乙酰基酶调节酿酒酵母中的复制时间并启用S内源控制。

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摘要

The replication of eukaryotic genomes follows a temporally staged program, in which late origin firing often occurs within domains of altered chromatin structure(s) and silenced genes. Histone deacetylation functions in gene silencing in some late-replicating regions, prompting an investigation of the role of histone deacetylation in replication timing control in Saccharomyces cerevisiae. Deletion of the histone deacetylase Rpd3 or its interacting partner Sin3 caused early activation of late origins at internal chromosomal loci but did not alter the initiation timing of early origins or a late-firing, telomere-proximal origin. By delaying initiation relative to the earliest origins, Rpd3 enables regulation of late origins by the intra-S replication checkpoint. RPD3 deletion suppresses the slow S phase of clb5Δ cells by enabling late origins to fire earlier, suggesting that Rpd3 modulates the initiation timing of many origins throughout the genome. Examination of factors such as Ume6 that function together with Rpd3 in transcriptional repression indicates that Rpd3 regulates origin initiation timing independently of its role in transcriptional repression. This supports growing evidence that for much of the S. cerevisiae genome transcription and replication timing are not linked.
机译:真核基因组的复制遵循一个暂时的程序,在该程序中,晚期起源激发通常发生在染色质结构和沉默基因改变的域内。组蛋白脱乙酰基在某些晚期复制区的基因沉默中起作用,促使人们对组蛋白脱乙酰基在酿酒酵母中复制时机控制中的作用进行了研究。组蛋白脱乙酰基酶Rpd3或其相互作用的伴侣Sin3的删除导致内部染色体基因座上的早期起源的早期激活,但不会改变早期起源或端粒近端起源的启动时间。通过延迟相对于最早起点的启动,Rpd3可以通过S内复制检查点调节晚期起点。 RPD3缺失通过使较晚的起源更早激发而抑制了clb5Δ细胞的慢S期,这表明Rpd3调节了整个基因组中许多起源的起始时间。对诸如Ume6等与Rpd3一起在转录抑制中起作用的因素的研究表明,Rpd3调节起始起始时间,与其在转录抑制中的作用无关。这支持了越来越多的证据,表明酿酒酵母的许多基因组的转录和复制时间没有联系。

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