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酿酒酵母Nedd4样泛素连接酶Rsp5p在环境应激条件下对质膜蛋白的质量控制

Quality control of plasma membrane proteins by Saccharomyces cerevisiae Nedd4-like ubiquitin ligase Rsp5p under environmental stress conditions.

作者信息

Shiga Takeki, Yoshida Nobuyuki, Shimizu Yuko, Suzuki Etsuko, Sasaki Toshiya, Watanabe Daisuke, Takagi Hiroshi

机构信息

Graduate School of Biological Sciences, Nara Institute of Science and Technology, Ikoma, Nara, Japan.

Graduate School of Biological Sciences, Nara Institute of Science and Technology, Ikoma, Nara, Japan

出版信息

Eukaryot Cell. 2014 Sep;13(9):1191-9. doi: 10.1128/EC.00104-14. Epub 2014 Jul 7.

Abstract

In Saccharomyces cerevisiae, when a rich nitrogen source such as ammonium is added to the culture medium, the general amino acid permease Gap1p is ubiquitinated by the yeast Nedd4-like ubiquitin ligase Rsp5p, followed by its endocytosis to the vacuole. The arrestin-like Bul1/2p adaptors for Rsp5p specifically mediate this process. In this study, to investigate the downregulation of Gap1p in response to environmental stresses, we determined the intracellular trafficking of Gap1p under various stress conditions. An increase in the extracellular ethanol concentration induced ubiquitination and trafficking of Gap1p from the plasma membrane to the vacuole in wild-type cells, whereas Gap1p remained stable on the plasma membrane under the same conditions in rsp5(A401E) and Δend3 cells. A (14)C-labeled citrulline uptake assay using a nonubiquitinated form of Gap1p (Gap1p(K9R/K16R)) revealed that ethanol stress caused a dramatic decrease of Gap1p activity. These results suggest that Gap1p is inactivated and ubiquitinated by Rsp5p for endocytosis when S. cerevisiae cells are exposed to a high concentration of ethanol. It is noteworthy that this endocytosis occurs in a Bul1/2p-independent manner, whereas ammonium-triggered downregulation of Gap1p was almost completely inhibited in Δbul1/2 cells. We also found that other environmental stresses, such as high temperature, H₂O₂, and LiCl, also promoted endocytosis of Gap1p. Similar intracellular trafficking caused by ethanol occurred in other plasma membrane proteins (Agp1p, Tat2p, and Gnp1p). Our findings suggest that stress-induced quality control is a common process requiring Rsp5p for plasma membrane proteins in yeast.

摘要

在酿酒酵母中,当向培养基中添加丰富的氮源(如铵)时,通用氨基酸通透酶Gap1p会被酵母Nedd4样泛素连接酶Rsp5p泛素化,随后被内吞至液泡中。Rsp5p的类抑制蛋白Bul1/2p衔接蛋白特异性介导这一过程。在本研究中,为了探究Gap1p在环境应激下的下调情况,我们测定了在各种应激条件下Gap1p的细胞内运输。细胞外乙醇浓度的增加诱导野生型细胞中Gap1p从质膜泛素化并运输至液泡,而在rsp5(A401E)和Δend3细胞中,Gap1p在相同条件下在质膜上保持稳定。使用非泛素化形式的Gap1p(Gap1p(K9R/K16R))进行的¹⁴C标记瓜氨酸摄取试验表明,乙醇应激导致Gap1p活性显著降低。这些结果表明,当酿酒酵母细胞暴露于高浓度乙醇时,Gap1p会被Rsp5p失活并泛素化以进行内吞作用。值得注意的是,这种内吞作用以不依赖Bul1/2p的方式发生,而在Δbul1/2细胞中,铵触发的Gap1p下调几乎完全受到抑制。我们还发现,其他环境应激,如高温、H₂O₂和LiCl,也促进了Gap1p的内吞作用。乙醇引起的类似细胞内运输也发生在其他质膜蛋白(Agp1p、Tat2p和Gnp1p)中。我们的研究结果表明,应激诱导的质量控制是酵母中质膜蛋白需要Rsp5p的常见过程。

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