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删除二酰甘油激酶Dgk1可通过增加Ypt7活性和改变膜流动性来增强酵母液泡融合。

Deleting the DAG kinase Dgk1 augments yeast vacuole fusion through increased Ypt7 activity and altered membrane fluidity.

作者信息

Miner Gregory E, Starr Matthew L, Hurst Logan R, Fratti Rutilio A

机构信息

Department of Biochemistry, University of Illinois at Urbana-Champaign, Urbana, Illinois.

Center for Biophysics and Quantitative Biology, University of Illinois at Urbana-Champaign, Urbana, Illinois.

出版信息

Traffic. 2017 May;18(5):315-329. doi: 10.1111/tra.12479. Epub 2017 Apr 4.

Abstract

Diacylglycerol (DAG) is a fusogenic lipid that can be produced through phospholipase C activity on phosphatidylinositol 4,5-bisphosphate [PI(4,5)P ], or through phosphatidic acid (PA) phosphatase activity. The fusion of Saccharomyces cerevisiae vacuoles requires DAG, PA and PI(4,5)P , and the production of these lipids is thought to provide temporally specific stoichiometries that are critical for each stage of fusion. Furthermore, DAG and PA can be interconverted by the DAG kinase Dgk1 and the PA phosphatase Pah1. Previously we found that pah1 Δ vacuoles were fragmented, blocked in SNARE priming and showed arrested endosomal maturation. In other pathways the effects of deleting PAH1 can be compensated for by additionally deleting DGK1 ; however, deleting both genes did not rescue the pah1 Δ vacuolar defects. Deleting DGK1 alone caused a marked increase in vacuole fusion that was attributed to elevated DAG levels. This was accompanied by a gain in resistance to the inhibitory effects of PA as well as inhibitors of Ypt7 activity. Together these data show that Dgk1 function can act as a negative regulator of vacuole fusion through the production of PA at the cost of depleting DAG and reducing Ypt7 activity.

摘要

二酰基甘油(DAG)是一种促融脂质,可通过磷脂酶C对磷脂酰肌醇4,5 - 二磷酸[PI(4,5)P₂]的作用产生,或通过磷脂酸(PA)磷酸酶的活性产生。酿酒酵母液泡的融合需要DAG、PA和PI(4,5)P₂,这些脂质的产生被认为提供了时间特异性的化学计量比,这对融合的每个阶段都至关重要。此外,DAG和PA可以通过DAG激酶Dgk1和PA磷酸酶Pah1相互转化。之前我们发现,缺失Pah1的液泡碎片化,在SNARE引发过程中受阻,并显示内体成熟停滞。在其他途径中,删除PAH1的影响可以通过额外删除DGK1来补偿;然而,同时删除这两个基因并不能挽救缺失Pah1的液泡缺陷。单独删除DGK1会导致液泡融合显著增加,这归因于DAG水平升高。这伴随着对PA以及Ypt7活性抑制剂抑制作用的抗性增加。这些数据共同表明,Dgk1的功能可以通过以消耗DAG和降低Ypt7活性为代价产生PA,作为液泡融合的负调节因子。

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