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在网格蛋白突变体中,Vps10p通过质膜在反式高尔基体网络(TGN)和晚期内体之间循环。

Vps10p cycles between the TGN and the late endosome via the plasma membrane in clathrin mutants.

作者信息

Deloche Olivier, Schekman Randy W

机构信息

Howard Hughes Medical Institute, University of California, Berkeley, California 94720-3206, USA.

出版信息

Mol Biol Cell. 2002 Dec;13(12):4296-307. doi: 10.1091/mbc.02-07-0105.

Abstract

Clathrin-coated vesicles mediate the transport of the soluble vacuolar protein CPY from the TGN to the endosomal/prevacuolar compartment. Surprisingly, CPY sorting is not affected in clathrin deletion mutant cells. Here, we have investigated the clathrin-independent pathway that allows CPY transport to the vacuole. We find that CPY transport is mediated by the endosome and requires normal trafficking of its sorting receptor, Vps10p, the steady state distribution of which is not altered in chc1 cells. In contrast, Vps10p accumulates at the cell surface in a chc1/end3 double mutant, suggesting that Vps10p is rerouted to the cell surface in the absence of clathrin. We used a chimeric protein containing the first 50 amino acids of CPY fused to a green fluorescent protein (CPY-GFP) to mimic CPY transport in chc1. In the absence of clathrin, CPY-GFP resides in the lumen of the vacuole as in wild-type cells. However, in chc1/sec6 double mutants, CPY-GFP is present in internal structures, possibly endosomal membranes, that do not colocalize with the vacuole. We propose that Vps10p must be transported to and retrieved from the plasma membrane to mediate CPY sorting to the vacuole in the absence of clathrin-coated vesicles. In this circumstance, precursor CPY may be captured by retrieved Vps10p in an early or late endosome, rather than as it normally is in the trans-Golgi, and delivered to the vacuole by the normal VPS gene-dependent process. Once relieved of cargo protein, Vps10p would be recycled to the trans-Golgi and then to the cell surface for further rounds of sorting.

摘要

网格蛋白包被小泡介导可溶性液泡蛋白羧肽酶Y(CPY)从反式高尔基体网络(TGN)运输到内体/液泡前体区室。令人惊讶的是,在网格蛋白缺失突变细胞中CPY的分选不受影响。在这里,我们研究了允许CPY运输到液泡的非网格蛋白依赖性途径。我们发现CPY运输由内体介导,并且需要其分选受体Vps10p的正常运输,其稳态分布在chc1细胞中未改变。相比之下,Vps10p在chc1/end3双突变体中积累在细胞表面,这表明在没有网格蛋白的情况下Vps10p被重新引导到细胞表面。我们使用了一种嵌合蛋白,该蛋白包含与绿色荧光蛋白融合的CPY的前50个氨基酸(CPY-GFP),以模拟chc1中的CPY运输。在没有网格蛋白的情况下,CPY-GFP如在野生型细胞中一样存在于液泡腔中。然而,在chc1/sec6双突变体中,CPY-GFP存在于内部结构中,可能是内体膜,这些结构与液泡不共定位。我们提出,在没有网格蛋白包被小泡的情况下,Vps10p必须运输到质膜并从质膜回收,以介导CPY分选到液泡中。在这种情况下,前体CPY可能在早期或晚期内体中被回收的Vps10p捕获,而不是像它通常在反式高尔基体中那样,然后通过正常的VPS基因依赖性过程被递送至液泡。一旦释放货物蛋白,Vps10p将被循环到反式高尔基体,然后到细胞表面进行进一步轮次的分选。

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