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果蝇中转高尔基网络中蛋白质分拣机制的功能特征。

Functional characterization of protein-sorting machineries at the trans-Golgi network in Drosophila melanogaster.

机构信息

Department of Anatomy and Histology, Fukushima Medical University, Fukushima 960-1295, Japan.

出版信息

J Cell Sci. 2010 Feb 1;123(Pt 3):460-71. doi: 10.1242/jcs.055103. Epub 2010 Jan 12.

Abstract

Targeting of proteins to their final destination is a prerequisite for living cells to maintain their homeostasis. Clathrin functions as a coat that forms transport carriers called clathrin-coated vesicles (CCVs) at the plasma membrane and post-Golgi compartments. In this study, we established an experimental system using Schneider S2 cells derived from the fruit fly, Drosophila melanogaster, as a model system to study the physiological roles of clathrin adaptors, and to dissect the processes of CCV formation. We found that a clathrin adaptor Drosophila GGA (dGGA), a homolog of mammalian GGA proteins, localizes to the trans-Golgi network (TGN) and is capable of recruiting clathrin from the cytosol onto TGN membranes. dGGA itself is recruited from the cytosol to the TGN in an ARF1 small GTPase (dARF79F)-dependent manner. dGGA recognizes the cytoplasmic acidic-cluster-dileucine (ACLL) sorting signal of Lerp (lysosomal enzyme receptor protein), a homolog of mammalian mannose 6-phosphate receptors. Moreover, both dGGA and another type of TGN-localized clathrin adaptor, AP-1 (adaptor protein-1 complex), are shown to be involved in the trafficking of Lerp from the TGN to endosomes and/or lysosomes. Taken together, our findings indicate that the protein-sorting machinery in fly cells is well conserved relative to that in mammals, enabling the use of fly cells to dissect CCV biogenesis and clathrin-dependent protein trafficking at the TGN of higher eukaryotes.

摘要

靶向蛋白质到其最终目的地是活细胞维持其体内平衡的前提。网格蛋白作为一种外壳,在质膜和高尔基体后区室形成称为网格蛋白包被小泡(CCV)的运输载体。在这项研究中,我们建立了一个使用源自果蝇的 Schneider S2 细胞的实验系统,作为研究网格蛋白衔接子生理作用的模型系统,并剖析 CCV 形成的过程。我们发现,一种网格蛋白衔接子果蝇 GGA(dGGA),是哺乳动物 GGA 蛋白的同源物,定位于反式高尔基体网络(TGN),并且能够将网格蛋白从细胞质招募到 TGN 膜上。dGGA 本身以 ARF1 小 GTP 酶(dARF79F)依赖性方式从细胞质被招募到 TGN。dGGA 识别 Lerp(溶酶体酶受体蛋白)的细胞质酸性簇亮氨酸(ACLL)分拣信号,Lerp 是哺乳动物甘露糖 6-磷酸受体的同源物。此外,dGGA 和另一种 TGN 定位的网格蛋白衔接子 AP-1(衔接蛋白-1 复合物)都被证明参与了 Lerp 从 TGN 到内体和/或溶酶体的运输。总之,我们的研究结果表明,相对于哺乳动物,果蝇细胞中的蛋白质分拣机制得到了很好的保守,使我们能够利用果蝇细胞来剖析真核生物 TGN 处的 CCV 生物发生和网格蛋白依赖性蛋白质运输。

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