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首页> 外文期刊>Molecular biology of the cell >A novel tribasic Golgi export signal directs cargo protein interaction with activated Rab11 and AP-1-dependent Golgi-plasma membrane trafficking
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A novel tribasic Golgi export signal directs cargo protein interaction with activated Rab11 and AP-1-dependent Golgi-plasma membrane trafficking

机译:一个新型的三基性高尔基体出口信号指导货物蛋白与活化的Rab11和依赖AP-1的高尔基体-质膜运输相互作用

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摘要

The reovirus fusion-associated small transmembrane (FAST) proteins comprise a unique family of viral membrane fusion proteins dedicated to inducing cell-cell fusion. We recently reported that a polybasic motif (PBM) in the cytosolic tail of reptilian reovirus p14 FAST protein functions as a novel tribasic Golgi export signal. Using coimmunoprecipitation and fluorescence resonance energy transfer (FRET) assays, we now show the PBM directs interaction of p14 with GTP-Rab11. Overexpression of dominant-negative Rab11 and RNA interference knockdown of endogenous Rab11 inhibited p14 plasma membrane trafficking and resulted in p14 accumulation in the Golgi complex. This is the first example of Golgi export to the plasma membrane that is dependent on the interaction of membrane protein cargo with activated Rab11. RNA interference and immunofluorescence microscopy further revealed that p14 Golgi export is dependent on AP-1 (but not AP-3 or AP-4) and that Rab11 and AP-1 both colocalize with p14 at the TGN. Together these results imply the PBM mediates interactions of p14 with activated Rab11 at the TGN, resulting in p14 sorting into AP1-coated vesicles for anterograde TGN-plasma membrane transport.
机译:呼肠孤病毒融合相关的小跨膜(FAST)蛋白包含一个独特的病毒膜融合蛋白家族,专门用于诱导细胞-细胞融合。我们最近报道,在爬行动物呼肠孤病毒p14 FAST蛋白的胞质尾巴中的多元基序(PBM)作为一种新型的三基性高尔基体输出信号。使用共免疫沉淀和荧光共振能量转移(FRET)分析,我们现在显示PBM指导p14与GTP-Rab11的相互作用。显性负性Rab11的过表达和内源性Rab11的RNA干扰敲低抑制p14质膜运输,并导致p14在高尔基体中积累。这是高尔基体向质膜输出的第一个例子,这取决于膜蛋白货物与活化的Rab11的相互作用。 RNA干扰和免疫荧光显微镜进一步揭示p14高尔基体的输出依赖于AP-1(但不依赖于AP-3或AP-4),并且Rab11和AP-1都与p14在TGN处共定位。这些结果共同表明,PBM在TGN介导p14与活化的Rab11的相互作用,导致p14进入AP1包被的囊泡中进行顺行性TGN-质膜转运。

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