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WTS-1/LATS通过协同抑制F-肌动蛋白组装来调节内吞再循环。

WTS-1/LATS regulates endocytic recycling by restraining F-actin assembly in a synergistic manner.

作者信息

Zhang Hanchong, Cheng Zihang, Li Wenbo, Hu Jie, Zhao Linyue, Chen Dan, Gao Jinghu, Chen Juan, Yan Yanling, Lin Long, Shi Anbing

机构信息

Department of Biochemistry and Molecular Biology, School of Basic Medicine, Tongji Medical College, Huazhong University of Science and Technology, Wuhan 430030, Hubei, China.

Cell Architecture Research Center, Huazhong University of Science and Technology, Wuhan 430030, Hubei, China.

出版信息

J Cell Sci. 2021 Dec 15;134(24). doi: 10.1242/jcs.259085.

DOI:10.1242/jcs.259085
PMID:34817059
Abstract

The disruption of endosomal actin architecture negatively affects endocytic recycling. However, the underlying homeostatic mechanisms that regulate actin organization during recycling remain unclear. In this study, we identified a synergistic endosomal actin assembly restricting mechanism in C. elegans involving WTS-1, the homolog of LATS kinases, which is a core component of the Hippo pathway. WTS-1 resides on the sorting endosomes and colocalizes with the actin polymerization regulator PTRN-1 [the homolog of the calmodulin-regulated spectrin-associated proteins (CAMSAPs)]. We observed an increase in PTRN-1-labeled structures in WTS-1-deficient cells, indicating that WTS-1 can limit the endosomal localization of PTRN-1. Accordingly, the actin overaccumulation phenotype in WTS-1-depleted cells was mitigated by the associated PTRN-1 loss. We further demonstrated that recycling defects and actin overaccumulation in WTS-1-deficient cells were reduced by the overexpression of constitutively active UNC-60A(S3A) (a cofilin protein homolog), which aligns with the role of LATS as a positive regulator of cofilin activity. Altogether, our data confirmed previous findings, and we propose an additional model, that WTS-1 acts alongside the UNC-60A-mediated actin disassembly to restrict the assembly of endosomal F-actin by curbing PTRN-1 dwelling on endosomes, preserving recycling transport.

摘要

内体肌动蛋白结构的破坏会对胞吞循环产生负面影响。然而,在循环过程中调节肌动蛋白组织的潜在稳态机制仍不清楚。在这项研究中,我们在秀丽隐杆线虫中发现了一种协同的内体肌动蛋白组装限制机制,该机制涉及WTS-1,它是LATS激酶的同源物,而LATS激酶是Hippo信号通路的核心组成部分。WTS-1定位于分拣内体,并与肌动蛋白聚合调节剂PTRN-1(钙调蛋白调节的血影蛋白相关蛋白(CAMSAPs)的同源物)共定位。我们观察到在WTS-1缺陷细胞中,PTRN-1标记的结构增加,这表明WTS-1可以限制PTRN-1在内体的定位。因此,WTS-1缺失细胞中肌动蛋白过度积累的表型因相关的PTRN-1缺失而得到缓解。我们进一步证明,组成型活性UNC-60A(S3A)(一种丝切蛋白同源蛋白)的过表达减少了WTS-1缺陷细胞中的循环缺陷和肌动蛋白过度积累,这与LATS作为丝切蛋白活性的正向调节剂的作用一致。总之,我们的数据证实了先前的发现,并且我们提出了一个额外的模型,即WTS-1与UNC-60A介导的肌动蛋白解聚一起发挥作用,通过抑制PTRN-1在内体的停留来限制内体F-肌动蛋白的组装,从而维持循环运输。

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