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Role of clathrin in dense core vesicle biogenesis

机译:Clathrin在致密核心囊泡生物发生中的作用

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The dense core vesicles (DCVs) of neuroendocrine cells are a rich source of bioactive molecules such as peptides, hormones, and neurotransmitters, but relatively little is known about how they are formed. Using fractionation profiling, a method that combines subcellular fractionation with mass spectrometry, we identified similar to 1200 proteins in PC12 cell vesicle-enriched fractions, with DCV-associated proteins showing distinct profiles from proteins associated with other types of vesicles. To investigate the role of clathrin in DCV biogenesis, we stably transduced PC12 cells with an inducible short hairpin RNA targeting clathrin heavy chain, resulting in similar to 85% protein loss. DCVs could still be observed in the cells by electron microscopy, but mature profiles were approximately fourfold less abundant than in mock-treated cells. By quantitative mass spectrometry, DCV-associated proteins were found to be reduced approximately twofold in clathrin-depleted cells as a whole and approximately fivefold in vesicle-enriched fractions. Our combined data sets enabled us to identify new candidate DCV components. Secretion assays revealed that clathrin depletion causes a near-complete block in secretagogue-induced exocytosis. Taken together, our data indicate that clathrin has a function in DCV biogenesis beyond its established role in removing unwanted proteins from the immature vesicle.
机译:神经内分泌细胞的致密核心囊泡(DCVs)是丰富的生物活性分子源,如肽,激素和神经递质,但是关于它们的形成方式相对较少。使用分馏分析,将亚细胞分馏与质谱分析相结合的方法,我们将类似于PC12细胞浓缩粒子囊泡的馏分中的1200蛋白鉴定,DCV相关蛋白质显示出与与其他类型囊泡相关的蛋白质不同的曲线。为了探讨Clathrin在DCV生物生成中的作用,我们用靶向Clathrin重链的诱导短发夹RNA稳定地转导PC12细胞,导致类似于85%的蛋白质损失。通过电子显微镜仍然可以在细胞中观察到DCV,但是成熟的曲线大约超过模拟处理细胞中的少于四倍。通过定量质谱法,发现DCV-相关的蛋白质在克拉棘含量的细胞中减少大约两倍,并且在富塞氏部分中的大约五倍。我们的组合数据集使我们能够识别新的候选DCV组件。分泌物测定显示,克拉辛耗竭导致分泌术诱导的外毒性的近完全嵌段。我们的数据表明,Clathrin在DCV生物发生中的功能超出了其在从未成熟囊泡中除去不需要的蛋白质的作用。

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