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Vps41磷酸化和Rab Ypt7控制HOPS复合物靶向内体-液泡融合位点。

Vps41 phosphorylation and the Rab Ypt7 control the targeting of the HOPS complex to endosome-vacuole fusion sites.

作者信息

Cabrera Margarita, Ostrowicz Clemens W, Mari Muriel, LaGrassa Tracy J, Reggiori Fulvio, Ungermann Christian

机构信息

Biochemistry Section, Department of Biology, University of Osnabrück, 49076 Osnabrück, Germany.

出版信息

Mol Biol Cell. 2009 Apr;20(7):1937-48. doi: 10.1091/mbc.e08-09-0943. Epub 2009 Feb 4.

Abstract

Membrane fusion depends on multisubunit tethering factors such as the vacuolar HOPS complex. We previously showed that the vacuolar casein kinase Yck3 regulates vacuole biogenesis via phosphorylation of the HOPS subunit Vps41. Here, we link the identified Vps41 phosphorylation site to HOPS function at the endosome-vacuole fusion site. The nonphosphorylated Vps41 mutant (Vps41 S-A) accumulates together with other HOPS subunits on punctate structures proximal to the vacuole that expand in a class E mutant background and that correspond to in vivo fusion sites. Ultrastructural analysis of this mutant confirmed the presence of tubular endosomal structures close to the vacuole. In contrast, Vps41 with a phosphomimetic mutation (Vps41 S-D) is mislocalized and leads to multilobed vacuoles, indicative of a fusion defect. These two phenotypes can be rescued by overproduction of the vacuolar Rab Ypt7, revealing that both Ypt7 and Yck3-mediated phosphorylation modulate the Vps41 localization to the endosome-vacuole junction. Our data suggest that Vps41 phosphorylation fine-tunes the organization of vacuole fusion sites and provide evidence for a fusion "hot spot" on the vacuole limiting membrane.

摘要

膜融合依赖于多亚基拴系因子,如液泡HOPS复合体。我们之前表明,液泡酪蛋白激酶Yck3通过磷酸化HOPS亚基Vps41来调节液泡生物发生。在这里,我们将已确定的Vps41磷酸化位点与内体-液泡融合位点处的HOPS功能联系起来。非磷酸化的Vps41突变体(Vps41 S-A)与其他HOPS亚基一起聚集在液泡近端的点状结构上,这些结构在E类突变背景下会扩展,且对应于体内融合位点。对该突变体的超微结构分析证实了靠近液泡处存在管状内体结构。相比之下,具有模拟磷酸化突变的Vps41(Vps41 S-D)定位错误,并导致液泡出现多叶现象,这表明存在融合缺陷。这两种表型可通过过量表达液泡Rab蛋白Ypt7来挽救,这表明Ypt7和Yck3介导的磷酸化都调节Vps41在内体-液泡连接处的定位。我们的数据表明,Vps41磷酸化可微调液泡融合位点的组织,并为液泡限制膜上的融合“热点”提供了证据。

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