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首页> 外文期刊>Molecular biology of the cell >The AP-1 clathrin-adaptor is required for lysosomal enzymes sorting and biogenesis of the contractile vacuole complex in Dictyostelium cells
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The AP-1 clathrin-adaptor is required for lysosomal enzymes sorting and biogenesis of the contractile vacuole complex in Dictyostelium cells

机译:AP-1网格蛋白适配器是溶酶体分选和Dictyostelium细胞中的收缩液泡复合物的生物发生所必需的

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摘要

dAdaptor protein complexes (AP) are major components of the cytoplasmic coat found on clathrin-coated vesicles. Here, we report the molecular and functional characterization of Dictyostelium clathrin-associated AP-1 complex, which in mammalian cells, participates mainly in budding of clathrin-coated vesicles from the trans-Golgi network (TGN). The gamma-adaptin AP-1 subunit was cloned and shown to belong to a Golgi-localized 300-kDa protein complex. Time-lapse analysis of cells expressing gamma-adaptin tagged with the green-fluorescent protein demonstrates the dynamics of AP-1-coated structures leaving the Golgi apparatus and rarely moving toward the TGN. Targeted disruption of the AP-1 medium chain results in viable cells displaying a severe growth defect and a delayed developmental cycle compared with parental cells. Lysosomnal enzymes are constitutively secreted as precursors, suggesting that protein transport between the TGN and lysosomes is defective. Although endocytic protein markers are correctly localized to endosomal compartments, morphological and ultrastructural studies reveal the absence of large endosomal vacuoles and an increased number of small vacuoles. In addition, the function of the contractile vacuole complex (CV), an osmoregulatory organelle is impaired and some CV components are not correctly targeted. [References: 81]
机译:dAdaptor蛋白复合物(AP)是在网格蛋白包被的囊泡上发现的细胞质被膜的主要成分。在这里,我们报告与网藻铁蛋白网格蛋白相关的AP-1复合物的分子和功能表征,该复合物在哺乳动物细胞中主要参与反式高尔基网络(TGN)的网格蛋白涂层囊泡的出芽。克隆了gamma-adaptin AP-1亚基,显示其属于高尔基体定位的300 kDa蛋白复合体。对表达有绿色荧光蛋白标记的γ-adaptin的细胞进行时移分析表明,涂有AP-1的结构的动力学过程离开了高尔基体,很少向TGN移动。与亲代细胞相比,AP-1中链的靶向破坏导致存活细胞显示出严重的生长缺陷和发育周期延迟。溶酶体酶组成性地作为前体分泌,表明TGN和溶酶体之间的蛋白质运输存在缺陷。尽管内吞蛋白标志物正确定位于内体区室,但形态学和超微结构研究显示不存在大的内体液泡和数量增加的小液泡。此外,收缩液泡复合物(CV),渗透性细胞器的功能受损,某些CV成分未正确靶向。 [参考:81]

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