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Multiple ER-Golgi SNARE transmembrane domains are dispensable for trafficking but required for SNARE recycling

机译:多个ER-Golgi SNARE跨膜域可用于贩运,但对于SNARE回收是必需的

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摘要

The formation of soluble N-ethylmaleimide-sensitive factor attachment protein receptor (SNARE) complexes between opposing membranes is an essential prerequisite for fusion between vesicles and their target compartments. The composition and length of a SNARE's transmembrane domain (TMD) is also an indicator for their steady-state distribution in cells. The evolutionary conservation of the SNARE TMD, together with the strict requirement of this feature for membrane fusion in biochemical studies, implies that the TMD represents an essential protein module. Paradoxically, we find that for several essential ER-and Golgi-localized SNAREs, a TMD is unnecessary. Moreover, in the absence of a covalent membrane tether, such SNAREs can still support ER-Golgi vesicle transport and recapitulate established genetic interactions. Transport anomalies appear to be restricted to retrograde trafficking, but these defects are overcome by the attachment of a C-terminal lipid anchor to the SNARE. We conclude that the TMD functions principally to support the recycling of Qb-, Qc-, and R-SNAREs and, in so doing, retrograde transport.
机译:在相对膜之间形成可溶性N-乙基马来酰亚胺敏感性因子附着蛋白受体(SNARE)复合物是囊泡与其靶标区室融合的必要前提。 SNARE跨膜结构域(TMD)的组成和长度也是其在细胞中稳态分布的指标。 SNARE TMD的进化保守性以及在生化研究中对膜融合功能的严格要求,意味着TMD代表了必需的蛋白质模块。矛盾的是,我们发现对于一些基本的ER和高尔基体定位的SNARE,TMD是不必要的。此外,在不存在共价膜系链的情况下,此类SNARE仍可支持ER-高尔基体小泡运输并概括已建立的遗传相互作用。运输异常似乎仅限于逆行运输,但这些缺陷可以通过将C末端脂质锚固定在SNARE上而克服。我们得出结论,TMD的主要作用是支持Qb-,Qc-和R-SNARE的回收,并在此过程中支持逆行运输。

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