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弗林蛋白酶在反式高尔基体网络中的分选。胞质尾部分选信号与AP-1高尔基体特异性组装蛋白的相互作用。

Sorting of furin at the trans-Golgi network. Interaction of the cytoplasmic tail sorting signals with AP-1 Golgi-specific assembly proteins.

作者信息

Teuchert M, Schäfer W, Berghöfer S, Hoflack B, Klenk H D, Garten W

机构信息

Institut für Virologie der Philipps-Universität Marburg, Robert-Koch-Strasse 17, 35037 Marburg, Germany.

出版信息

J Biol Chem. 1999 Mar 19;274(12):8199-207. doi: 10.1074/jbc.274.12.8199.

DOI:10.1074/jbc.274.12.8199
PMID:10075724
Abstract

The eukaryotic subtilisin-like endoprotease furin is found predominantly in the trans-Golgi network (TGN) and cycles between this compartment, the cell surface, and the endosomes. There is experimental evidence for endocytosis from the plasma membrane and transport from endosomes to the TGN, but direct exit from the TGN to endosomes via clathrin-coated vesicles has only been discussed but not directly shown so far. Here we present data showing that expression of furin promotes the first step of clathrin-coat assembly at the TGN, the recruitment of the Golgi-specific assembly protein AP-1 on Golgi membranes. Further, we report that furin indeed is present in isolated clathrin-coated vesicles. Packaging into clathrin-coated vesicles requires signal components in the furin cytoplasmic domain which can be recognized by AP-1 assembly proteins. We found that besides depending on the phosphorylation state of a casein kinase II site, interaction of the furin tail with AP-1 and its mu1subunit is mediated by a tyrosine motif and to less extent by a leucine-isoleucine signal, whereas a monophenylalanine motif is only involved in binding to the intact AP-1 complex. This study implies that high affinity interaction of AP-1 or mu1 with the cytoplasmic tail of furin needs a complex interplay of signal components rather than one distinct signal.

摘要

真核枯草杆菌蛋白酶样内切蛋白酶弗林蛋白酶主要存在于反式高尔基体网络(TGN)中,并在该区室、细胞表面和内体之间循环。有实验证据表明其可从质膜进行内吞作用,并可从内体转运至TGN,但迄今为止,关于通过网格蛋白包被小泡从TGN直接转运至内体的过程仅在讨论中,尚未得到直接证实。在此,我们展示的数据表明,弗林蛋白酶的表达促进了TGN处网格蛋白包被组装的第一步,即高尔基体特异性组装蛋白AP-1在高尔基体膜上的募集。此外,我们报告弗林蛋白酶确实存在于分离出的网格蛋白包被小泡中。包装到网格蛋白包被小泡中需要弗林蛋白酶胞质结构域中的信号成分,这些成分可被AP-1组装蛋白识别。我们发现,除了依赖酪蛋白激酶II位点的磷酸化状态外,弗林蛋白酶尾部与AP-1及其μ1亚基的相互作用由一个酪氨酸基序介导,在较小程度上由一个亮氨酸-异亮氨酸信号介导,而一个单苯丙氨酸基序仅参与与完整AP-1复合物的结合。这项研究表明,AP-1或μ1与弗林蛋白酶胞质尾部的高亲和力相互作用需要信号成分的复杂相互作用,而不是一个独特的信号。

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