首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Acetylation in the globular core of histone H3 on lysine-56 promotes chromatin disassembly during transcriptional activation
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Acetylation in the globular core of histone H3 on lysine-56 promotes chromatin disassembly during transcriptional activation

机译:赖氨酸56上组蛋白H3球状核心中的乙酰化促进转录激活过程中的染色质分解

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摘要

Promoter chromatin disassembly is a widely used mechanism to regulate eukaryotic transcriptional induction. Delaying histone H3/H4 removal from the yeast PHO5 promoter also leads to delayed removal of histones H2A/H2B, suggesting a constant equilibrium of assembly and disassembly of H2A/H2B, whereas H3/H4 disassembly is the highly regulated step. Toward understanding how H3/H4 disassembly is regulated, we observe a drastic increase in the levels of histone H3 acetylated on lysine-56 (K56ac) during promoter chromatin disassembly. Indeed, promoter chromatin disassembly is driven by Rtt109 and Asf1-dependent acetylation of H3 K56. Conversely, promoter chromatin reassembly during transcriptional repression is accompanied by decreased levels of histone H3 acetylated on lysine-56, and a mutation that prevents K56 acetylation increases the rate of transcriptional repression. As such, H3 K56 acetylation drives chromatin toward the disassembled state during transcriptional activation, whereas loss of H3 K56 acetylation drives the chromatin toward the assembled state.
机译:启动子染色质拆卸是调节真核转录诱导的广泛使用的机制。延迟从酵母PHO5启动子中去除组蛋白H3 / H4也会导致组蛋白H2A / H2B的去除延迟,这表明H2A / H2B的组装和分解始终处于平衡状态,而H3 / H4的分解是高度受控的步骤。为了了解如何调节H3 / H4的拆卸,我们观察到在启动子染色质拆卸过程中,赖氨酸56(K56ac)上乙酰化的组蛋白H3的含量急剧增加。实际上,启动子染色质的分解是由H3 K56的Rtt109和Asf1依赖性乙酰化驱动的。相反,在转录抑制过程中启动子染色质重组伴随着在赖氨酸56上乙酰化的组蛋白H3水平降低,而阻止K56乙酰化的突变增加了转录抑制率。这样,在转录激活过程中,H3 K56乙酰化将染色质推向分解状态,而H3 K56乙酰化的丧失则将染色质推向组装状态。

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