4.8 Article

Cohesin mediates DNA loop extrusion by a swing and clamp mechanism

期刊

CELL
卷 184, 期 21, 页码 5448-+

出版社

CELL PRESS
DOI: 10.1016/j.cell.2021.09.016

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资金

  1. EMBO
  2. HFSP
  3. European Union [721874]
  4. Vienna Science and Technology Fund [LS19-029]
  5. Boehringer Ingelheim
  6. Austrian Research Promotion Agency [FFG-852936]
  7. European Research Council under the European Union [693949]
  8. Human Frontier Science Program [RGP0057/2018]
  9. Marie Curie Actions (MSCA) [721874] Funding Source: Marie Curie Actions (MSCA)
  10. European Research Council (ERC) [693949] Funding Source: European Research Council (ERC)

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The study analyzed how human cohesin-NIPBL complexes mediate loop extrusion, identifying DNA binding sites and large-scale conformational changes required for this process. Results indicate that DNA is translocated by a specific structural element of the cohesin complex to achieve loop extrusion. These findings reveal mechanistic principles of how cohesin-NIPBL and other SMC complexes mediate loop extrusion.
Structural maintenance of chromosomes (SMC) complexes organize genome topology in all kingdoms of life and have been proposed to perform this function by DNA loop extrusion. How this process works is unknown. Here, we have analyzed how loop extrusion is mediated by human cohesin-NIPBL complexes, which enable chromatin folding in interphase cells. We have identified DNA binding sites and large-scale conformational changes that are required for loop extrusion and have determined how these are coordinated. Our results suggest that DNA is translocated by a spontaneous 50 nm-swing of cohesin's hinge, which hands DNA over to the ATPase head of SMC3, where upon binding of ATP, DNA is clamped by NIPBL. During this process, NIPBL jumps ship from the hinge toward the SMC3 head and might thereby couple the spontaneous hinge swing to ATP-dependent DNA clamping. These results reveal mechanistic principles of how cohesin-NIPBL and possibly other SMC complexes mediate loop extrusion.

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