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中心体上破坏复合物的成核加速了β-连环蛋白的降解,并调节 Wnt 信号转导。

Nucleation of the destruction complex on the centrosome accelerates degradation of β-catenin and regulates Wnt signal transmission.

机构信息

Department of Molecular, Cellular, and Developmental Biology, University of California, Santa Barbara, CA 93106.

Neuroscience Research Institute, University of California, Santa Barbara, CA 93106.

出版信息

Proc Natl Acad Sci U S A. 2022 Sep 6;119(36):e2204688119. doi: 10.1073/pnas.2204688119. Epub 2022 Aug 29.

Abstract

Wnt signal transduction is controlled by the destruction complex (DC), a condensate comprising scaffold proteins and kinases that regulate β-catenin stability. Overexpressed DC scaffolds undergo liquid-liquid phase separation (LLPS), but DC mesoscale organization at endogenous expression levels and its role in β-catenin processing were previously unknown. Here, we find that DC LLPS is nucleated by the centrosome. Through a combination of CRISPR-engineered custom fluorescent tags, finite element simulations, and optogenetic tools that allow for manipulation of DC concentration and multivalency, we find that centrosomal nucleation drives processing of β-catenin by colocalizing DC components to a single reaction crucible. Enriching GSK3β partitioning on the centrosome controls β-catenin processing and prevents Wnt-driven embryonic stem cell differentiation to mesoderm. Our findings demonstrate the role of nucleators in controlling biomolecular condensates and suggest tight integration between Wnt signal transduction and the cell cycle.

摘要

Wnt 信号转导受破坏复合物 (DC) 的控制,该复合物由支架蛋白和激酶组成,可调节 β-连环蛋白的稳定性。过表达的 DC 支架会发生液-液相分离 (LLPS),但之前并不清楚内源性表达水平下 DC 的介观组织及其在 β-连环蛋白加工中的作用。在这里,我们发现 DC 的 LLPS 由中心体引发。通过结合 CRISPR 工程设计的定制荧光标签、有限元模拟以及光遗传学工具来操纵 DC 的浓度和多价性,我们发现中心体引发使 DC 成分在单个反应坩埚中局部化,从而促进了 β-连环蛋白的加工。富集中心体上的 GSK3β 分配控制 β-连环蛋白的加工,并防止 Wnt 驱动的胚胎干细胞向中胚层分化。我们的研究结果表明了引发剂在控制生物分子凝聚物中的作用,并提示 Wnt 信号转导与细胞周期之间的紧密整合。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d7b1/9457612/510b4c3271cd/pnas.2204688119fig01.jpg

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