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A Rab Requirement Is Not Bypassed in SLY1-20 Suppression

机译:在SLY1-20抑制中不违反Rab要求

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摘要

The Rab GTPase Ypt1p and the large homodimer Uso1p are both required for tethering endoplasmic reticulum-derived vesicles to early Golgi compartments in yeast. Loss-of-function ypt1 and uso1 mutations are suppressed by SLY1-20, a dominant allele that encodes the Sed5p-associated protein, Sly1p. Here, we investigate the mechanism of SLY1-20 suppression. In wild-type strains, Ypt1p can be coimmunoprecipitated with Uso1p; however, in a ypt1Δ/SLY1-20 strain, which lacks this complex, membrane binding of Uso1p was reduced. In spite of Ypt1p depletion, Uso1p-dependent vesicle tethering was not bypassed under the ypt1Δ/SLY1-20 condition. Moreover, tethering and fusion assays with ypt1Δ/SLY1-20 membranes remained sensitive to Rab GDP dissociation inhibitor. These results indicate that an alternative Rab protein satisfies the Ypt1p requirement in Uso1p-dependent tethering when SLY1-20 is expressed. Further genetic and biochemical tests revealed that a related Rab protein, Ypt6, might substitute for Ypt1p in ypt1Δ/SLY1-20 cells. Additional experimentation to address the mechanism of SLY1-20 suppression in a cog2Δ [sec35Δ] strain indicated that the Cog2p subunit of the conserved oligomeric Golgi complex is either functionally redundant or is not directly required for anterograde transport to the Golgi complex.
机译:Rab GTPase Ypt1p和大同型二聚体Uso1p都是将内质网来源的囊泡束缚到酵母中早期高尔基体的必需条件。功能丧失的ypt1和uso1突变被SLY1-20抑制,SLY1-20是编码Sed5p相关蛋白Sly1p的主要等位基因。在这里,我们研究了SLY1-20抑制的机制。在野生型菌株中,Ypt1p可与Uso1p共免疫沉淀。然而,在缺乏这种复合物的ypt1Δ/ SLY1-20菌株中,Uso1p的膜结合减少。尽管Ypt1p耗竭,但在ypt1Δ/ SLY1-20条件下并未绕过Uso1p依赖的囊泡束缚。此外,使用ypt1Δ/ SLY1-20膜进行的束缚和融合测定仍对Rab GDP离解抑制剂敏感。这些结果表明,当表达SLY1-20时,替代的Rab蛋白可以满足Uso1p依赖系链中Ypt1p的要求。进一步的遗传和生化测试表明,相关的Rab蛋白Ypt6可能替代ypt1Δ/ SLY1-20细胞中的Ypt1p。解决cog2Δ[sec35Δ]菌株中SLY1-20抑制机制的其他实验表明,保守的寡聚高尔基体的Cog2p亚基在功能上是多余的,也不是顺行转运至高尔基体的直接必需。

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