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Analysis of Sec22p in endoplasmic reticulum/golgi transport reveals cellular redundancy in SNARE protein function

机译:内质网/高尔基体运输中的Sec22p的分析显示SNARE蛋白功能的细胞冗余。

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Membrane-bound soluble N-ethylmaleimide-sensitive factor attachment protein receptor (SNARE) proteins form heteromeric complexes that are required for intracellular membrane fusion and are proposed to encode compartmental specificity. In yeast, the R-SNARE protein Sec22p acts in transport between the endoplasmic reticulum (ER) and Golgi compartments but is not essential for cell growth. Other SNARE proteins that function in association with Sec22p (i.e., Sed5p, Bos1p, and Bet1p) are essential, leading us to question how transport through the early secretory pathway is sustained in the absence of Sec22p. In wild-type strains, we show that Sec22p is directly required for fusion of ER-derived vesicles with Golgi acceptor membranes. In sec22Delta strains, Ykt6p, a related R-SNARE protein that operates in later stages of the secretory pathway, is up-regulated and functionally substitutes for Sec22p. In vivo combination of the sec22Delta mutation with a conditional ykt6-1 allele results in lethality, consistent with a redundant mechanism. Our data indicate that the requirements for specific SNARE proteins in intracellular membrane fusion are less stringent than appreciated and suggest that combinatorial mechanisms using both upstream-targeting elements and SNARE proteins are required to maintain an essential level of compartmental organization. [References: 59]
机译:膜结合的可溶性N-乙基马来酰亚胺敏感因子附着蛋白受体(SNARE)蛋白形成细胞内膜融合所需的异源复合物,并提议编码隔室特异性。在酵母中,R-SNARE蛋白Sec22p在内质网(ER)和高尔基体区室之间的转运中起作用,但对于细胞生长不是必需的。与Sec22p关联的其他SNARE蛋白(即Sed5p,Bos1p和Bet1p)是必不可少的,这使我们质疑在没有Sec22p的情况下如何维持通过早期分泌途径的转运。在野生型菌株中,我们显示Sec22p是ER来源的囊泡与高尔基体受体膜融合的直接需要。在sec22Delta菌株中,Ykt6p(一种在分泌途径后期起作用的相关R-SNARE蛋白)被上调并在功能上替代了Sec22p。 sec22Delta突变与条件性ykt6-1等位基因的体内结合可导致致死性,与冗余机制一致。我们的数据表明细胞内膜融合中对特定SNARE蛋白的要求不如人们所理解的严格,并且表明使用上游靶向元件和SNARE蛋白的组合机制对于维持必要的区室组织水平是必需的。 [参考:59]

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