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Cell-free sorting of peroxisomal membrane proteins from the endoplasmic reticulum

机译:来自内质网的过氧化物酶体膜蛋白的无细胞分选

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摘要

Several yeast and mammalian peroxisomal membrane proteins (PMPs) are delivered to peroxisomes via the endoplasmic reticulum (ER). Fluorescence microscopy showed a focused assembly of PMPs in a specialized domain of the ER, referred to as the preperox-isomal ER. It is proposed that preperoxisomal vesicles containing PMPs bud from this domain to either fuse with preexisting peroxisomes or to mature into functional peroxisomes by uptake of peroxisomal membrane and matrix proteins. However, such vesicular entities are not identified nor are the biochemical requirements for the budding process known. We developed an in vitro cell-free ER-budding assay using Pichia pastoris and followed two endogenous PMPs, Pex11p and Pex3p during their ER exit. Both the PMPs were copackaged in the ER-budded vesicles that float on a Nycodenz gradient. PMP budding from the ER was dependent on ATP, temperature, cytosol, and Pex19p and generated preperoxisomal vesicles with an incomplete complement of PMPs. Surprisingly, Pex11p budding was independent of Pex3p; however, the budded vesicles were devoid of most of the PMPs otherwise present in the wild-type vesicles and might represent peroxisomal remnants. Our findings provide a biochemical platform to uncover the mechanism of PMP budding from the ER.
机译:几种酵母和哺乳动物过氧化物酶体膜蛋白(PMP)通过内质网(ER)传递至过氧化物酶体。荧光显微镜检查显示,PMP在ER的特定域中聚焦,称为过氧化物酶体-等量ER。有人提出,含PMP的过氧化物酶体前囊泡从该结构域中萌发,或者与预先存在的过氧化物酶体融合,或者通过摄取过氧化物酶体膜和基质蛋白而成熟为功能性过氧化物酶体。然而,这种囊泡实体没有被识别,出芽过程的生化要求也未知。我们开发了一种使用巴斯德毕赤酵母的体外无细胞ER萌芽测定方法,并在其ER退出过程中遵循了两个内源性PMP,即Pex11p和Pex3p。两种PMP共同包装在漂浮在Nycodenz梯度上的ER预算囊泡中。从ER萌芽的PMP依赖于ATP,温度,细胞溶质和Pex19p,并生成过氧化物酶体前囊泡,其中PMPs不完全互补。出人意料的是,Pex11p的出芽不依赖于Pex3p。然而,发芽的囊泡中没有大多数野生型囊泡中存在的PMP,可能代表过氧化物酶体残留。我们的研究结果提供了一个生化平台,以揭示ER释放PMP的机制。

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