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裂殖酵母中磷脂介导的Rab GDP解离抑制剂调控的遗传证据。

Genetic evidence for phospholipid-mediated regulation of the Rab GDP-dissociation inhibitor in fission yeast.

作者信息

Ma Yan, Kuno Takayoshi, Kita Ayako, Nabata Toshiya, Uno Satoshi, Sugiura Reiko

机构信息

Division of Molecular Pharmacology and Pharmacogenomics, Department of Genome Sciences, Kobe University Graduate School of Medicine, Hyogo, Japan.

出版信息

Genetics. 2006 Nov;174(3):1259-71. doi: 10.1534/genetics.106.064709. Epub 2006 Sep 15.

Abstract

We have previously identified mutant alleles of genes encoding two Rab proteins, Ypt3 and Ryh1, through a genetic screen using the immunosuppressant drug FK506 in fission yeast. In the same screen, we isolated gdi1-i11, a mutant allele of the essential gdi1+ gene encoding Rab GDP-dissociation inhibitor. In gdi1-i11, a conserved Gly267 was substituted by Asp. The Gdi1G267D protein failed to extract Rabs from membrane and Rabs were depleted from the cytosolic fraction in the gdi1-i11 mutant cells. Consistently, the Gdi1G267D protein was found mostly in the membrane fraction, whereas wild-type Gdi1 was found in both the cytosolic and the membrane fraction. Notably, overexpression of spo20+, encoding a phosphatidylcholine/phosphatidylinositol transfer protein, rescued gdi1-i11 mutation, but not ypt3-i5 or ryh1-i6. The gdi1-i11 and spo20-KC104 mutations are synthetically lethal, and the wild-type Gdi1 failed to extract Rabs from the membrane in the spo20-KC104 mutant. The phosphatidylinositol-transfer activity of Spo20 is dispensable for the suppression of the gdi1-i11 mutation, suggesting that the phosphatidylcholine-transfer activity is important for the suppression. Furthermore, knockout of the pct1+ gene encoding a choline phosphate cytidyltransferase rescued the gdi1-i11 mutation. Together, our findings suggest that Spo20 modulates Gdi1 function via regulation of phospholipid metabolism of the membranes.

摘要

我们之前通过在裂殖酵母中使用免疫抑制剂FK506进行遗传筛选,鉴定出了编码两种Rab蛋白Ypt3和Ryh1的基因突变等位基因。在同一筛选中,我们分离出了gdi1-i11,它是编码Rab GDP解离抑制剂的必需基因gdi1+的一个突变等位基因。在gdi1-i11中,保守的甘氨酸267被天冬氨酸取代。Gdi1G267D蛋白无法从膜上提取Rab,并且在gdi1-i11突变细胞的胞质部分中Rab减少。一致地,Gdi1G267D蛋白主要存在于膜部分,而野生型Gdi1则存在于胞质和膜部分。值得注意的是,编码磷脂酰胆碱/磷脂酰肌醇转移蛋白的spo20+的过表达挽救了gdi1-i11突变,但不能挽救ypt3-i5或ryh1-i6。gdi1-i11和spo20-KC104突变是合成致死的,并且野生型Gdi1在spo20-KC104突变体中无法从膜上提取Rab。Spo20的磷脂酰肌醇转移活性对于抑制gdi1-i11突变是可有可无的,这表明磷脂酰胆碱转移活性对于抑制很重要。此外,敲除编码胆碱磷酸胞苷转移酶的pct1+基因挽救了gdi1-i11突变。总之,我们的发现表明Spo20通过调节膜的磷脂代谢来调节Gdi1功能。

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