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Ensa通过调节Treslin水平来控制S期的时长。

Ensa controls S-phase length by modulating Treslin levels.

作者信息

Charrasse Sophie, Gharbi-Ayachi Aicha, Burgess Andrew, Vera Jorge, Hached Khaled, Raynaud Peggy, Schwob Etienne, Lorca Thierry, Castro Anna

机构信息

Université de Montpellier, Centre de Recherche de Biologie Cellulaire de Montpellier, Equipe Labellisée 'Ligue Contre le Cancer', CNRS UMR 5237, 1919 Route de Mende, 34293, Montpellier cedex 5, France.

The Kinghorn Cancer Centre, Garvan Institute of Medical Research, Darlinghurst, NSW, 2010, Australia.

出版信息

Nat Commun. 2017 Aug 8;8(1):206. doi: 10.1038/s41467-017-00339-4.

Abstract

The Greatwall/Ensa/PP2A-B55 pathway is essential for controlling mitotic substrate phosphorylation and mitotic entry. Here, we investigate the effect of the knockdown of the Gwl substrate, Ensa, in human cells. Unexpectedly, Ensa knockdown promotes a dramatic extension of S phase associated with a lowered density of replication forks. Notably, Ensa depletion results in a decrease of Treslin levels, a pivotal protein for the firing of replication origins. Accordingly, the extended S phase in Ensa-depleted cells is completely rescued by the overexpression of Treslin. Our data herein reveal a new mechanism by which normal cells regulate S-phase duration by controlling the ubiquitin-proteasome degradation of Treslin in a Gwl/Ensa-dependent pathway.The Greatwall/Ensa/PP2A-B55 pathway controls mitotic substrate phosphorylation and mitotic entry. Here the authors show that cells regulate S phase duration by controlling the ubiquitin-proteasome degradation of Treslin in a Gwl/Ensa-dependent pathway.

摘要

长城/Ensa/PP2A-B55通路对于控制有丝分裂底物磷酸化和进入有丝分裂至关重要。在此,我们研究了在人类细胞中敲低Gwl底物Ensa的影响。出乎意料的是,敲低Ensa会促进S期显著延长,这与复制叉密度降低有关。值得注意的是,Ensa缺失导致Treslin水平下降,Treslin是启动复制起点的关键蛋白。因此,过表达Treslin可完全挽救Ensa缺失细胞中延长的S期。我们的数据揭示了一种新机制,即正常细胞通过在Gwl/Ensa依赖的途径中控制Treslin的泛素-蛋白酶体降解来调节S期持续时间。长城/Ensa/PP2A-B55通路控制有丝分裂底物磷酸化和进入有丝分裂。在此,作者表明细胞通过在Gwl/Ensa依赖的途径中控制Treslin的泛素-蛋白酶体降解来调节S期持续时间。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/dbb4/5547116/9c67d95ce12c/41467_2017_339_Fig1_HTML.jpg

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