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EphA2 驱动 Ras 转化的上皮细胞与其正常邻居分离。

EphA2 Drives the Segregation of Ras-Transformed Epithelial Cells from Normal Neighbors.

机构信息

European Cancer Stem Cell Research Institute, Cardiff University, Hadyn Ellis Building, Maindy Road, Cardiff CF24 4HQ, UK.

Division of Molecular Oncology, Institute for Genetic Medicine, Hokkaido University Graduate School of Chemical Sciences and Engineering, Kita 15, Nishi 7, Kita-ku, Sapporo, Hokkaido 060-0815, Japan.

出版信息

Curr Biol. 2016 Dec 5;26(23):3220-3229. doi: 10.1016/j.cub.2016.09.037. Epub 2016 Nov 10.

DOI:10.1016/j.cub.2016.09.037
PMID:27839970
Abstract

In epithelial tissues, cells expressing oncogenic Ras (hereafter RasV12 cells) are detected by normal neighbors and as a result are often extruded from the tissue [1-6]. RasV12 cells are eliminated apically, suggesting that extrusion may be a tumor-suppressive process. Extrusion depends on E-cadherin-based cell-cell adhesions and signaling to the actin-myosin cytoskeleton [2, 6]. However, the signals underlying detection of the RasV12 cell and triggering extrusion are poorly understood. Here we identify differential EphA2 signaling as the mechanism by which RasV12 cells are detected in epithelial cell sheets. Cell-cell interactions between normal cells and RasV12 cells trigger ephrin-A-EphA2 signaling, which induces a cell repulsion response in RasV12 cells. Concomitantly, RasV12 cell contractility increases in an EphA2-dependent manner. Together, these responses drive the separation of RasV12 cells from normal cells. In the absence of ephrin-A-EphA2 signals, RasV12 cells integrate with normal cells and adopt a pro-invasive morphology. We also show that Drosophila Eph (DEph) is detected in segregating clones of RasV12 cells and is functionally required to drive segregation of RasV12 cells in vivo, suggesting that our in vitro findings are conserved in evolution. We propose that expression of RasV12 in single or small clusters of cells within a healthy epithelium creates ectopic EphA2 boundaries, which drive the segregation and elimination of the transformed cell from the tissue. Thus, deregulation of Eph/ephrin would allow RasV12 cells to go undetected and expand within an epithelium.

摘要

在上皮组织中,表达致癌 Ras 的细胞(以下简称 RasV12 细胞)会被正常的相邻细胞检测到,因此这些细胞常常被挤出组织[1-6]。RasV12 细胞从顶端被挤出,表明挤出可能是一种肿瘤抑制过程。挤出依赖于基于 E-钙粘蛋白的细胞-细胞黏附以及向肌动蛋白-肌球蛋白细胞骨架的信号传导[2,6]。然而,检测 RasV12 细胞并触发挤出的信号基础理解得还很差。在这里,我们确定 EphA2 信号的差异是 RasV12 细胞在上皮细胞片中被检测到的机制。正常细胞与 RasV12 细胞之间的细胞-细胞相互作用触发了 Ephrin-A-EphA2 信号传导,从而在 RasV12 细胞中诱导细胞排斥反应。同时,RasV12 细胞的收缩性以 EphA2 依赖的方式增加。这些反应共同促使 RasV12 细胞与正常细胞分离。在没有 Ephrin-A-EphA2 信号的情况下,RasV12 细胞与正常细胞整合并采用促侵袭的形态。我们还表明,果蝇 Eph(DEph)在 RasV12 细胞的分离克隆中被检测到,并且在体内驱动 RasV12 细胞的分离是功能性必需的,这表明我们的体外发现在上皮组织中是保守的。我们提出,在健康上皮组织中的单个或小簇细胞中表达 RasV12 会产生异位 EphA2 边界,从而驱动转化细胞从组织中分离和消除。因此,Eph/ephrin 的失调将允许 RasV12 细胞未被检测到并在上皮组织中扩张。

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