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Replication fork movement sets chromatin loop size and origin choice in mammalian cells

机译:复制叉的移动设置了哺乳动物细胞中染色质环的大小和来源选择

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Genome stability requires one, and only one, DNA duplication at each S phase. The mechanisms preventing origin firing on newly replicated DNA are well documented, but much less is known about the mechanisms controlling the spacing of initiation events, namely the completion of DNA replication. Here we show that origin use in Chinese hamster cells depends on both the movement of the replication forks and the organization of chromatin loops. We found that slowing the replication speed triggers the recruitment of latent origins within minutes, allowing the completion of S phase in a timely fashion. When slowly replicating cells are shifted to conditions of fast fork progression, although the decrease in the overall number of active origins occurs within 2 h, the cells still have to go through a complete cell cycle before the efficiency specific to each origin is restored. We observed a strict correlation between replication speed during a given S phase and the size of chromatin loops in the next G1 phase. Furthermore, we found that origins located at or near sites of anchorage of chromatin loops in G1 are activated preferentially in the following S phase. These data suggest a mechanism of origin programming in which replication speed determines the spacing of anchorage regions of chromatin loops, that, in turn, controls the choice of initiation sites.
机译:基因组稳定性在每个S期仅需要一个DNA复制。防止起源于新复制的DNA的机制已经有充分的文献记载,但是对于控制起始事件间隔(即DNA复制完成)的机制知之甚少。在这里,我们表明中国仓鼠细胞的起源使用取决于复制叉的移动和染色质环的组织。我们发现,降低复制速度会在几分钟内触发潜在来源的募集,从而使S期得以及时完成。当缓慢复制的细胞转移到快叉进展的条件下时,尽管活跃起源总数的减少发生在2小时之内,但在恢复每个起源特有的效率之前,细胞仍必须经历完整的细胞周期。我们观察到在给定的S期复制速度与下一G1期染色质环的大小之间存在严格的相关性。此外,我们发现位于G1中染色质环锚定位点处或附近的起源在随后的S期中被优先激活。这些数据表明了一种起源编程的机制,其中复制速度决定了染色质环的锚定区域的间隔,进而控制了起始位点的选择。

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