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在 -Golgi 网络中,Frizzled6 和 Vangl2 平面细胞极性蛋白的差异分拣机制。

A mechanism for differential sorting of the planar cell polarity proteins Frizzled6 and Vangl2 at the -Golgi network.

机构信息

From the Division of Life Science, Hong Kong University of Science and Technology, Clear Water Bay, Kowloon, Hong Kong, China.

the Centre for Cell and Developmental Biology, State Key Laboratory of Agrobiotechnology, School of Life Sciences, Chinese University of Hong Kong, Shatin, New Territories, Hong Kong, China.

出版信息

J Biol Chem. 2018 Jun 1;293(22):8410-8427. doi: 10.1074/jbc.RA118.001906. Epub 2018 Apr 17.

Abstract

In planar cell polarity (PCP), the epithelial cells are polarized along the plane of the cell surface perpendicular to the classical apical-basal axis, a process mediated by several conserved signaling receptors. Two PCP-signaling proteins, VANGL planar cell polarity protein 2 (Vangl2) and Frizzled6 (Fzd6), are located asymmetrically on opposite boundaries of the cell. Examining sorting of these two proteins at the -Golgi network (TGN), we demonstrated previously that the GTP-binding protein ADP-ribosylation factor-related protein 1 (Arfrp1) and the clathrin-associated adaptor protein complex 1 (AP-1) are required for Vangl2 transport from the TGN. In contrast, TGN export of Frizzled6 does not depend on Arfrp1 or AP-1. Here, to further investigate the TGN sorting process in mammalian cells, we reconstituted release of Vangl2 and Frizzled6 from the TGN into vesicles Immunoblotting of released vesicles indicated that Vangl2 and Frizzled6 exit the TGN in separate compartments. Knockdown analysis revealed that a clathrin adaptor, epsinR, regulates TGN export of Frizzled6 but not of Vangl2. Protein interaction analysis suggested that epsinR forms a stable complex with clathrin and that this complex interacts with a conserved polybasic motif in the Frizzled6 cytosolic domain to package Frizzled6 into transport vesicles. Moreover, we found that Frizzled6-epsinR binding dissociates epsinR from AP-1, which may separate these two cargo adaptors from each other to perform distinct cargo-sorting functions. Our results suggest that Vangl2 and Frizzled6 are packaged into separate vesicles that are regulated by different clathrin adaptors at the TGN, which may contribute to their asymmetric localizations.

摘要

在平面细胞极性 (PCP) 中,上皮细胞沿垂直于经典顶底轴的细胞表面平面极化,这一过程由几个保守的信号受体介导。两种 PCP 信号蛋白,VANGL 平面细胞极性蛋白 2 (Vangl2) 和 Frizzled6 (Fzd6),不对称地位于细胞的相对边界上。在检查这些两种蛋白在高尔基体网络 (TGN) 的分选时,我们之前证明了 G 蛋白结合蛋白 ADP-核糖基化因子相关蛋白 1 (Arfrp1) 和网格蛋白相关衔接蛋白复合物 1 (AP-1) 是 Vangl2 从 TGN 运输所必需的。相比之下,Frizzled6 的 TGN 输出不依赖于 Arfrp1 或 AP-1。在这里,为了进一步研究哺乳动物细胞中的 TGN 分选过程,我们重新构建了 Vangl2 和 Frizzled6 从 TGN 释放到囊泡中的过程。免疫印迹分析表明,Vangl2 和 Frizzled6 从 TGN 中以不同的隔室释放。敲低分析表明,网格蛋白衔接蛋白 epsinR 调节 Frizzled6 的 TGN 输出,但不调节 Vangl2。蛋白相互作用分析表明,epsinR 与网格蛋白形成稳定的复合物,该复合物与 Frizzled6 胞质域中的保守多碱性基序相互作用,将 Frizzled6 包装到运输囊泡中。此外,我们发现 Frizzled6-epsinR 结合将 epsinR 从 AP-1 上解离下来,这可能将这两种货物衔接蛋白彼此分开,以执行不同的货物分选功能。我们的结果表明,Vangl2 和 Frizzled6 被包装到不同的囊泡中,这些囊泡由 TGN 中的不同网格蛋白衔接蛋白调节,这可能有助于它们的不对称定位。

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