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Rab11-FIP2影响极化的MDCK细胞内体系统的多个组成部分。

Rab11-FIP2 influences multiple components of the endosomal system in polarized MDCK cells.

作者信息

Ducharme Nicole A, Ham Amy-Joan L, Lapierre Lynne A, Goldenring James R

机构信息

Departments of Surgery and Cell & Developmental Biology; Vanderbilt University School of Medicine; Nashville, TN USA.

出版信息

Cell Logist. 2011 Mar;1(2):57-68. doi: 10.4161/cl.1.2.15289.

Abstract

The Rab11 Family Interacting Proteins (Rab11-FIPs) are hypothesized to regulate sequential steps in the apical recycling and transcytotic pathways of polarized epithelial cells. Previous studies have suggested that Rab11-FIP proteins assemble into multi-protein complexes regulating plasma membrane recycling. Rab11-FIP2 interacts with both myosin Vb and Rab11. Recent investigations have noted that that Rab11-FIP2 mutants [Rab11-FIP2(129-512), also designated Rab11-FIP2(ΔC2) and Rab11-FIP2(S229A, R413G), also designated Rab11-FIP2(SARG)], are potent inhibitors of transcytosis in polarized MDCK cells. Interestingly, Rab11-FIP2(ΔC2), but not Rab11-FIP2(SARG), also altered the morphology of the EEA-1 positive early endosomal compartment. These findings suggested that Rab11-FIP2 mutants could differentiate different points along the recycling pathway. We therefore sought to investigate whether Rab11-FIP2 is a general regulator of the early endosomal system. Both Rab11-FIP2 mutants altered the localization and co-localized with dynein heavy chain. In contrast, both clathrin heavy chain and AP-1 accumulated with membranes containing Rab11-FIP2(SARG), but not with Rab11-FIP2(ΔC2). Expression of Rab11-FIP2(ΔC2), but not Rab11-FIP2(SARG), caused clustering of early endosomal markers Rab5b, Epsin 4 and IQGAP1, around a collapsed Rab11-FIP2 containing membranous cisternum. Interestingly, neither Rab11-FIP2 mutant had any effect on the distribution of Rab5a, a classical early endosome marker. The results support the view that Rab11-FIP2 may influence microtubule-dependent centripetal movement of subsets of early endosomes as well as processing through the common and recycling endosomal systems.

摘要

Rab11家族相互作用蛋白(Rab11-FIPs)被认为在极化上皮细胞的顶端回收和转胞吞途径中调节一系列步骤。先前的研究表明,Rab11-FIP蛋白组装成多蛋白复合物来调节质膜回收。Rab11-FIP2与肌球蛋白Vb和Rab11都相互作用。最近的研究指出,Rab11-FIP2突变体[Rab11-FIP2(129 - 512),也称为Rab11-FIP2(ΔC2)和Rab11-FIP2(S229A, R413G),也称为Rab11-FIP2(SARG)]是极化MDCK细胞中转胞吞作用的有效抑制剂。有趣的是,Rab11-FIP2(ΔC2),而非Rab11-FIP2(SARG),也改变了EEA-1阳性早期内体区室的形态。这些发现表明,Rab11-FIP2突变体可以区分回收途径中的不同点。因此,我们试图研究Rab11-FIP2是否是早期内体系统的一般调节因子。两种Rab11-FIP2突变体都改变了定位并与动力蛋白重链共定位。相比之下,网格蛋白重链和AP-1在含有Rab11-FIP2(SARG)的膜上积累,但在含有Rab11-FIP2(ΔC2)的膜上不积累。Rab11-FIP2(ΔC2)的表达,而非Rab11-FIP2(SARG)的表达,导致早期内体标记物Rab5b、Epsin 4和IQGAP1聚集在一个塌陷的含有Rab11-FIP2的膜池周围。有趣的是,两种Rab11-FIP2突变体对经典早期内体标记物Rab5a的分布均无影响。结果支持了这样一种观点,即Rab11-FIP2可能影响早期内体亚群的微管依赖性向心运动以及通过共同和回收内体系统的加工过程。

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