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GTPase cross talk regulates TRAPPII activation of Rab11 homologues during vesicle biogenesis

机译:GTPase Cross谈论在囊泡生物发生期间调节Rab11同源物的Trappii激活

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摘要

Rab guanosine triphosphatases (GTPases) control cellular trafficking pathways by regulating vesicle formation, transport, and tethering. Rab11 and its paralogs regulate multiple secretory and endocytic recycling pathways, yet the guanine nucleotide exchange factor (GEF) that activates Rab11 in most eukaryotic cells is unresolved. The large multisubunit transport protein particle (TRAPP) II complex has been proposed to act as a GEF for Rab11 based on genetic evidence, but conflicting biochemical experiments have created uncertainty regarding Rab11 activation. Using physiological Rab-GEF reconstitution reactions, we now provide definitive evidence that TRAPPII is a bona fide GEF for the yeast Rab11 homologues Ypt31/32. We also uncover a direct role for Arf1, a distinct GTPase, in recruiting TRAPPII to anionic membranes. Given the known role of Ypt31/32 in stimulating activation of Arf1, a bidirectional cross talk mechanism appears to drive biogenesis of secretory and endocytic recycling vesicles. By coordinating simultaneous activation of two essential GTPase pathways, this mechanism ensures recruitment of the complete set of effectors needed for vesicle formation, transport, and tethering.
机译:Rab鸟苷三磷酸酶(GTP酶)通过调节囊泡形成,运输和束缚来控制细胞流量途径。 Rab11及其副病毒调节多种分泌和内吞再循环途径,但在大多数真核细胞中激活Rab11的鸟嘌呤核苷酸交换因子(GEF)是未解决的。已经提出了大型多管迁移蛋白颗粒(TraPh)II综合体基于遗传证据作为RAB11的全球环境基金,但生化实验的矛盾已经产生了关于RAB11活化的不确定性。使用生理RAB-GEF重建反应,我们现在提供了明确的证据,即Trappii是酵母RAB11同源物YPT31 / 32的真正GEF。我们还发现ARF1,一种不同的GTP酶,招募Trappii至阴离子膜的直接作用。鉴于YPT31 / 32在刺激ARF1的激活中的已知作用,似乎似乎驱动了分泌和内吞再循环囊泡的生物发生的双向交叉谈话机制。通过协调两种必需的GTP酶途径的同时激活,该机制可确保囊泡形成,运输和束缚所需的完整效果仪的招募。

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