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Enhancer regions show high histone H3.3 turnover that changes during differentiation

机译:增强子区域显示出较高的组蛋白H3.3周转率在分化过程中会发生变化

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摘要

The organization of DNA into chromatin is dynamic; nucleosomes are frequently displaced to facilitate the ability of regulatory proteins to access specific DNA elements. To gain insight into nucleosome dynamics, and to follow how dynamics change during differentiation, we used a technique called time-ChIP to quantitatively assess histone H3.3 turnover genome-wide during differentiation of mouse ESCs. We found that, without prior assumptions, high turnover could be used to identify regions involved in gene regulation. High turnover was seen at enhancers, as observed previously, with particularly high turnover at super-enhancers. In contrast, regions associated with the repressive Polycomb-Group showed low turnover in ESCs. Turnover correlated with DNA accessibility. Upon differentiation, numerous changes in H3.3 turnover rates were observed, the majority of which occurred at enhancers. Thus, time-ChIP measurement of histone turnover shows that active enhancers are unusually dynamic in ESCs and changes in highly dynamic nucleosomes predominate at enhancers during differentiation.>DOI:
机译:DNA进入染色质的组织是动态的;核小体经常被置换以促进调节蛋白访问特定DNA元素的能力。为了深入了解核小体动力学,并追踪分化过程中的动力学变化,我们使用了一种称为time-ChIP的技术来定量评估小鼠ESC分化过程中全基因组H3.3营业额。我们发现,在没有事先假设的情况下,高周转率可用于鉴定参与基因调控的区域。如之前观察到的,增强剂的周转率很高,而超级增强剂的周转率特别高。相反,与抑制性Polycomb-Group相关的区域在ESC中显示出较低的周转率。营业额与DNA可及性相关。分化后,观察到H3.3周转率发生了许多变化,其中大部分发生在增强子上。因此,对组蛋白更新的时间ChIP测量表明,活性增强子在ESC中异常动态,而高动态核小体的变化在分化过程中主要在增强子上发生。> DOI:

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