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分选连接蛋白 17(SNX17)将内体分选与 Eps15 同源结构域蛋白 1(EHD1)介导的分裂机制联系起来。

Sorting nexin 17 (SNX17) links endosomal sorting to Eps15 homology domain protein 1 (EHD1)-mediated fission machinery.

机构信息

Department of Biochemistry and Molecular Biology University of Nebraska Medical Center, Omaha, Nebraska 68198.

Department of Biochemistry and Molecular Biology University of Nebraska Medical Center, Omaha, Nebraska 68198

出版信息

J Biol Chem. 2020 Mar 20;295(12):3837-3850. doi: 10.1074/jbc.RA119.011368. Epub 2020 Feb 10.

Abstract

Following endocytosis, receptors that are internalized to sorting endosomes are sorted to different pathways, in part by sorting nexin (SNX) proteins. Notably, SNX17 interacts with a multitude of receptors in a sequence-specific manner to regulate their recycling. However, the mechanisms by which SNX17-labeled vesicles that contain sorted receptors bud and undergo vesicular fission from the sorting endosomes remain elusive. Recent studies suggest that a dynamin-homolog, Eps15 homology domain protein 1, catalyzes fission and releases endosome-derived vesicles for recycling to the plasma membrane. However, the mechanism by which EHD1 is coupled to various receptors and regulates their recycling remains unknown. Here we sought to characterize the mechanism by which EHD1 couples with SNX17 to regulate recycling of SNX17-interacting receptors. We hypothesized that SNX17 couples receptors to the EHD1 fission machinery in mammalian cells. Coimmunoprecipitation experiments and assays provided evidence that EHD1 and SNX17 directly interact. We also found that inducing internalization of a SNX17 cargo receptor, low-density lipoprotein receptor-related protein 1 (LRP1), led to recruitment of cytoplasmic EHD1 to endosomal membranes. Moreover, surface rendering and quantification of overlap volumes indicated that SNX17 and EHD1 partially colocalize on endosomes and that this overlap further increases upon LRP1 internalization. Additionally, SNX17-containing endosomes were larger in EHD1-depleted cells than in WT cells, suggesting that EHD1 depletion impairs SNX17-mediated endosomal fission. Our findings help clarify our current understanding of endocytic trafficking, providing significant additional insight into the process of endosomal fission and connecting the sorting and fission machineries.

摘要

内吞作用后,被内吞到分拣内体的受体被分拣到不同的途径,部分原因是分拣衔接蛋白(SNX)蛋白。值得注意的是,SNX17 以序列特异性的方式与多种受体相互作用,以调节它们的回收。然而,SNX17 标记的含有分拣受体的小泡出芽并从分拣内体进行囊泡分裂的机制仍然难以捉摸。最近的研究表明,一种与 dynamin 同源的蛋白,Eps15 同源结构域蛋白 1(Eps15 homology domain protein 1,EHD1),催化分裂并释放内体衍生的小泡进行回收,以返回到质膜。然而,EHD1 与各种受体结合并调节它们的回收的机制仍然未知。在这里,我们试图表征 EHD1 与 SNX17 结合以调节 SNX17 相互作用的受体回收的机制。我们假设 SNX17 将受体与 EHD1 的分裂机制偶联在哺乳动物细胞中。共免疫沉淀实验和实验提供了证据表明 EHD1 和 SNX17 直接相互作用。我们还发现,诱导 SNX17 货物受体,即低密度脂蛋白受体相关蛋白 1(low-density lipoprotein receptor-related protein 1,LRP1)的内化,导致细胞质 EHD1 募集到内体膜。此外,表面渲染和重叠体积的定量表明,SNX17 和 EHD1 在内体上部分共定位,并且这种重叠在 LRP1 内化后进一步增加。此外,在 EHD1 耗尽的细胞中,含有 SNX17 的内体比在 WT 细胞中更大,这表明 EHD1 耗竭会损害 SNX17 介导的内体分裂。我们的发现有助于澄清我们对胞吞作用的理解,为内体分裂过程提供了重要的额外见解,并连接了分拣和分裂机制。

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