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发动蛋白突变揭示了果蝇血细胞原代培养中不同的不依赖发动蛋白和依赖发动蛋白的内吞途径。

Shibire mutations reveal distinct dynamin-independent and -dependent endocytic pathways in primary cultures of Drosophila hemocytes.

作者信息

Guha A, Sriram V, Krishnan K S, Mayor S

机构信息

National Center for Biological Sciences, Tata Institute of Fundamental Research, GKVK, Bangalore 560 065, India.

出版信息

J Cell Sci. 2003 Aug 15;116(Pt 16):3373-86. doi: 10.1242/jcs.00637.

DOI:10.1242/jcs.00637
PMID:12857788
Abstract

We have developed a primary cell culture system derived from embryonic and larval stages of Drosophila. This allows for high-resolution imaging and genetic analyses of endocytic processes. Here, we have investigated endocytic pathways of three types of molecules: an endogenous receptor that binds anionic ligands (ALs), glycosylphosphatidylinositol (GPI)-anchored protein (GPI-AP), and markers of the fluid phase in primary hemocytes. We find that the endogenous AL-binding receptor (ALBR) is internalized into Rab5-positive endosomes, whereas the major portion of the fluid phase is taken up into Rab5-negative endosomes; GPI-APs are endocytosed into both classes of endosomes. ALBR and fluid-phase-containing early endosomes subsequently fuse to yield a population of Rab7-positive late endosomes. In primary culture, the endocytic phenotype of ALBR internalization in cells carrying mutations in Drosophila Dynamin (dDyn) at the shibire locus (shits) parallels the temperature-sensitive behavior of shits animals. At the restrictive temperature in shits cells, receptor-bound ALs remain completely surface accessible, localized to clathrin and alpha-adaptin-positive structures. On lowering the temperature, ALs are rapidly sequestered, suggesting a reversible block at a late step in dDyn-dependent endocytosis. By contrast, GPI-AP and fluid-phase endocytosis are quantitatively unaffected at the restrictive temperature in shits hemocytes, demonstrating a constitutive dDyn and Rab5-independent endocytic pathway in Drosophila.

摘要

我们开发了一种源自果蝇胚胎和幼虫阶段的原代细胞培养系统。这使得对内吞过程进行高分辨率成像和基因分析成为可能。在这里,我们研究了三种类型分子的内吞途径:一种结合阴离子配体(ALs)的内源性受体、糖基磷脂酰肌醇(GPI)锚定蛋白(GPI-AP)以及原代血细胞中液相的标志物。我们发现内源性AL结合受体(ALBR)被内化到Rab5阳性的内体中,而液相的主要部分被摄取到Rab5阴性的内体中;GPI-APs被内吞到这两类内体中。ALBR和含有液相的早期内体随后融合,产生一群Rab7阳性的晚期内体。在原代培养中,携带果蝇发动蛋白(dDyn)在麻痹位点(shits)发生突变的细胞中ALBR内化的内吞表型与shits动物的温度敏感行为相似。在shits细胞的限制温度下,受体结合的ALs完全保持在细胞表面可及,定位于网格蛋白和α-衔接蛋白阳性结构上。降低温度时,ALs迅速被隔离,这表明在依赖dDyn的内吞作用的后期步骤存在可逆性阻断。相比之下,在shits血细胞的限制温度下,GPI-AP和液相内吞在数量上不受影响,这表明果蝇中存在一条不依赖dDyn和Rab5的组成型内吞途径。

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