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反式高尔基体网络辅助蛋白p56促进含GGA/网格蛋白的运输载体的长距离移动以及溶酶体酶分选。

The trans-Golgi network accessory protein p56 promotes long-range movement of GGA/clathrin-containing transport carriers and lysosomal enzyme sorting.

作者信息

Mardones Gonzalo A, Burgos Patricia V, Brooks Doug A, Parkinson-Lawrence Emma, Mattera Rafael, Bonifacino Juan S

机构信息

Cell Biology and Metabolism Branch, National Institute of Child Health and Human Development, National Institutes of Health, Bethesda, MD 20892, USA.

出版信息

Mol Biol Cell. 2007 Sep;18(9):3486-501. doi: 10.1091/mbc.e07-02-0190. Epub 2007 Jun 27.

Abstract

The sorting of acid hydrolase precursors at the trans-Golgi network (TGN) is mediated by binding to mannose 6-phosphate receptors (MPRs) and subsequent capture of the hydrolase-MPR complexes into clathrin-coated vesicles or transport carriers (TCs) destined for delivery to endosomes. This capture depends on the function of three monomeric clathrin adaptors named GGAs. The GGAs comprise a C-terminal "ear" domain that binds a specific set of accessory proteins. Herein we show that one of these accessory proteins, p56, colocalizes and physically interacts with the three GGAs at the TGN. Moreover, overexpression of the GGAs enhances the association of p56 with the TGN, and RNA interference (RNAi)-mediated depletion of the GGAs decreases the TGN association and total levels of p56. RNAi-mediated depletion of p56 or the GGAs causes various degrees of missorting of the precursor of the acid hydrolase, cathepsin D. In the case of p56 depletion, this missorting correlates with decreased mobility of GGA-containing TCs. Transfection with an RNAi-resistant p56 construct, but not with a p56 construct lacking the GGA-ear-interacting motif, restores the mobility of the TCs. We conclude that p56 tightly cooperates with the GGAs in the sorting of cathepsin D to lysosomes, probably by enabling the movement of GGA-containing TCs.

摘要

酸性水解酶前体在反式高尔基体网络(TGN)中的分选是通过与甘露糖6-磷酸受体(MPR)结合,随后将水解酶-MPR复合物捕获到网格蛋白包被的囊泡或运输载体(TC)中实现的,这些载体 destined for delivery to endosomes。这种捕获依赖于三种名为GGA的单体网格蛋白衔接蛋白的功能。GGA包含一个C末端“耳”结构域,可结合一组特定的辅助蛋白。在此我们表明,这些辅助蛋白之一p56在TGN处与三种GGA共定位并发生物理相互作用。此外,GGA的过表达增强了p56与TGN的结合,而RNA干扰(RNAi)介导的GGA缺失会降低p56与TGN的结合以及p56的总水平。RNAi介导的p56或GGA缺失会导致酸性水解酶组织蛋白酶D前体出现不同程度的分选错误。在p56缺失的情况下,这种分选错误与含GGA的TC的移动性降低相关。用抗RNAi的p56构建体转染,但不用缺乏GGA-耳相互作用基序的p56构建体转染,可恢复TC的移动性。我们得出结论,p56在组织蛋白酶D分选到溶酶体的过程中与GGA紧密合作,可能是通过促进含GGA的TC的移动来实现的。 (原文中“destined for delivery to endosomes”表述不太完整准确,推测可能是“ destined for delivery to endosomes via...”之类意思,但按要求未做修改)

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