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The ATP binding site of the chromatin remodeling homolog Lsh is required for nucleosome density and de novo DNA methylation at repeat sequences

机译:染色质重塑同源物Lsh的ATP结合位点是核小体密度和重复序列DNA从头甲基化所必需的

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摘要

Lsh, a chromatin remodeling protein of the SNF2 family, is critical for normal heterochromatin structure. In particular, DNA methylation at repeat elements, a hallmark of heterochromatin, is greatly reduced in Lsh−/− (KO) cells. Here, we examined the presumed nucleosome remodeling activity of Lsh on chromatin in the context of DNA methylation. We found that dynamic CG methylation was dependent on Lsh in embryonic stem cells. Moreover, we demonstrate that ATP function is critical for de novo methylation at repeat sequences. The ATP binding site of Lsh is in part required to promote stable association of the DNA methyltransferase 3b with the repeat locus. By performing nucleosome occupancy assays, we found distinct nucleosome occupancy in KO ES cells compared to WT ES cells after differentiation. Nucleosome density was restored to wild-type level by re-expressing wild-type Lsh but not the ATP mutant in KO ES cells. Our results suggest that ATP-dependent nucleosome remodeling is the primary molecular function of Lsh, which may promote de novo methylation in differentiating ES cells.
机译:Lsh是SNF2家族的染色质重塑蛋白,对于正常的异染色质结构至关重要。尤其是,Lsh -/-(KO)细胞中重复元件处的DNA甲基化(异染色质的标志)大大降低。在这里,我们检查了在DNA甲基化的背景下,Lsh对染色质的推测核小体重塑活性。我们发现动态CG甲基化依赖于胚胎干细胞中的Lsh。此外,我们证明ATP功能对于重复序列的从头甲基化至关重要。 Lsh的ATP结合位点是促进DNA甲基转移酶3b与重复基因座稳定缔合的一部分。通过进行核小体占用分析,我们发现分化后与WT ES细胞相比,KO ES细胞中的核小体占用率明显不同。通过在KO ES细胞中重新表达野生型Lsh而不是ATP突变体,使核小体密度恢复至野生型水平。我们的结果表明,ATP依赖性核小体重塑是Lsh的主要分子功能,它可能促进分化的ES细胞从头甲基化。

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