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NCK1/2 衔接蛋白的蛋白质组学分析揭示了同工基因特异性相互作用,这些相互作用揭示了 NCK2 在细胞有丝分裂末期细胞分离中的新作用。

Proteomic Analysis of NCK1/2 Adaptors Uncovers Paralog-specific Interactions That Reveal a New Role for NCK2 in Cell Abscission During Cytokinesis.

机构信息

From the ‡Centre de recherche du Centre Hospitalier Universitaire (CHU) de Québec-Université Laval, Axe Oncologie, Québec G1R 2J6, QC, Canada.

§Centre de recherche sur le cancer de l'Université Laval, Québec G1R 2J6, QC, Canada.

出版信息

Mol Cell Proteomics. 2018 Oct;17(10):1979-1990. doi: 10.1074/mcp.RA118.000689. Epub 2018 Jul 12.

Abstract

Signals from cell surface receptors are often relayed via adaptor proteins. NCK1 and NCK2 are Src-Homology (SH) 2 and 3 domain adaptors that regulate processes requiring a remodeling of the actin cytoskeleton. Evidence from gene inactivation in mouse suggests that NCK1 and NCK2 are functionally redundant, although recent reports support the idea of unique functions for NCK1 and NCK2. We sought to examine this question further by delineating NCK1- and NCK2-specific signaling networks. We used both affinity purification-mass spectrometry and BioID proximity labeling to identify NCK1/2 signaling networks comprised of 98 proteins. Strikingly, we found 30 proteins restricted to NCK1 and 28 proteins specifically associated with NCK2, suggesting differences in their function. We report that , but not mouse embryo fibroblasts (MEFs) are multinucleated and display extended protrusions reminiscent of intercellular bridges, which correlate with an extended time spent in cytokinesis as well as a failure of a significant proportion of cells to complete abscission. Our data also show that the midbody of NCK2-deficient cells is not only increased in length, but also altered in composition, as judged by the mislocalization of AURKB, PLK1 and ECT2. Finally, we show that NCK2 function during cytokinesis requires its SH2 domain. Taken together, our data delineate the first high-confidence interactome for NCK1/2 adaptors and highlight several proteins specifically associated with either protein. Thus, contrary to what is generally accepted, we demonstrate that NCK1 and NCK2 are not completely redundant, and shed light on a previously uncharacterized function for the NCK2 adaptor protein in cell division.

摘要

细胞表面受体的信号通常通过衔接蛋白传递。NCK1 和 NCK2 是 Src 同源(SH)2 和 3 结构域衔接蛋白,它们调节需要重塑肌动蛋白细胞骨架的过程。来自小鼠基因失活的证据表明,NCK1 和 NCK2 在功能上是冗余的,尽管最近的报告支持 NCK1 和 NCK2 具有独特功能的观点。我们试图通过描绘 NCK1 和 NCK2 特异性信号网络来进一步研究这个问题。我们使用亲和纯化-质谱和 BioID 邻近标记来鉴定由 98 种蛋白质组成的 NCK1/2 信号网络。引人注目的是,我们发现 30 种蛋白质仅限于 NCK1,28 种蛋白质与 NCK2 特异性相关,这表明它们的功能存在差异。我们报告说,而不是 鼠胚胎成纤维细胞(MEFs)是多核的,并显示出延伸的突起,类似于细胞间桥,这与细胞分裂期延长以及相当一部分细胞无法完成分离有关。我们的数据还表明,NCK2 缺陷细胞的中体不仅长度增加,而且组成也发生改变,这可以从 AURKB、PLK1 和 ECT2 的定位错误判断出来。最后,我们表明,NCK2 在细胞分裂过程中的功能需要其 SH2 结构域。总之,我们的数据描绘了 NCK1/2 衔接蛋白的第一个高可信度互作组,并突出了与两种蛋白质都特异性相关的几种蛋白质。因此,与普遍接受的观点相反,我们证明了 NCK1 和 NCK2 并非完全冗余,并揭示了 NCK2 衔接蛋白在细胞分裂中以前未被表征的功能。

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