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Replication-guided nucleosome packing and nucleosome breathing expedite the formation of dense arrays

机译:复制引导的核心包装和核心呼吸加快了致密阵列的形成

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The first level of genome packaging in eukaryotic cells involves the formation of dense nucleosome arrays, with DNA coverage near 90% in yeasts. How cells achieve such high coverage within a short time, e. g. after DNA replication, remains poorly understood. It is known that random sequential adsorption of impenetrable particles on a line reaches high density extremely slowly, due to a jamming phenomenon. The nucleosome-shifting action of remodeling enzymes has been proposed as a mechanism to resolve such jams. Here, we suggest two biophysical mechanisms which assist rapid filling of DNA with nucleosomes, and we quantitatively characterize these mechanisms within mathematical models. First, we show that the 'softness' of nucleosomes, due to nucleosome breathing and stepwise nucleosome assembly, significantly alters the filling behavior, speeding up the process relative to 'hard' particles with fixed, mutually exclusive DNA footprints. Second, we explore model scenarios in which the progression of the replication fork could eliminate nucleosome jamming, either by rapid filling in its wake or via memory of the parental nucleosome positions. Taken together, our results suggest that biophysical effects promote rapid nucleosome filling, making the reassembly of densely packed nucleosomes after DNA replication a simpler task for cells than was previously thought.
机译:真核细胞中的第一级基因组包装涉及形成致密的核小阵列,酵母中的DNA覆盖率接近90%。细胞在短时间内如何实现如此高的覆盖率,例如G。在DNA复制后,仍然仍然清晰。众所周知,由于干扰现象,随机顺序吸附在线上的较高的颗粒在线上达到高密度。已经提出了重塑酶的核小体移位作用作为解决这些卡纸的机制。在这里,我们建议使用核心快速填充DNA的两种生物物理机制,并且我们在数学模型中定量表征这些机制。首先,我们表明核心的“柔软性”,由于核心呼吸和逐步的核心组装,显着改变了填充行为,加速了相对于“硬”颗粒具有固定的,相互排他性的DNA足迹。其次,我们探索模型情景,其中复制叉的进展可以通过快速填充其唤醒或通过父母核心位置的核心来消除核小胺干扰。我们的结果表明,生物物理效果促进了快速核心填充物,使DNA复制较简单的细胞任务比以前认为细胞更简单的核心的核心重新组装。

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