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在转运至PC12细胞表面过程中的分选:突触小泡蛋白与分泌颗粒蛋白的差异

Sorting during transport to the surface of PC12 cells: divergence of synaptic vesicle and secretory granule proteins.

作者信息

Cutler D F, Cramer L P

机构信息

Department of Biochemistry, Wolfson Laboratories, Imperial College, London, England.

出版信息

J Cell Biol. 1990 Mar;110(3):721-30. doi: 10.1083/jcb.110.3.721.

Abstract

PC12 cells, a cell line derived from a rat pheochromocytoma, have both regulated and constitutive secretory pathways. Regulated secretion occurs via large dense core granules, which are related to chromaffin granules and are abundant in these cells. In addition, PC12 cells also contain small electron-lucent vesicles, whose numbers increase in response to nerve growth factor and which may be related to cholinergic synaptic vesicles. These could characterize a second regulated secretory pathway. We have investigated the trafficking of protein markers for both these organelles. We have purified and characterized the large dense core granules from these cells using sequential velocity and equilibrium gradients. We demonstrate the copurification of the major PC12 soluble regulated secretory protein (secretogranin II) with this organelle. As a marker for the synaptic vesicle-like organelles in this system, we have used the integral membrane glycoprotein p38 or synaptophysin. We show that the p38-enriched fraction of PC12 cells comigrates with rat brain synaptic vesicles on an equilibrium gradient. We also demonstrate that p38 purifies away from the dense core granules; less than 5% of this protein is found in our dense granule fraction. Finally we show that p38 does not pass through the dense granule fraction in pulse-chase experiments. These results rule out the possibility of p38 reaching the small clear vesicles via mature dense granules and imply that these cells may have two independently derived regulated pathways.

摘要

PC12细胞系源自大鼠嗜铬细胞瘤,具有调节性和组成性分泌途径。调节性分泌通过大的致密核心颗粒发生,这些颗粒与嗜铬颗粒相关且在这些细胞中丰富。此外,PC12细胞还含有小的电子透明囊泡,其数量会因神经生长因子而增加,并且可能与胆碱能突触囊泡有关。这些可能表征了第二条调节性分泌途径。我们研究了这两种细胞器的蛋白质标志物的运输。我们使用连续速度和平衡梯度从这些细胞中纯化并表征了大的致密核心颗粒。我们证明了主要的PC12可溶性调节性分泌蛋白(分泌粒蛋白II)与这种细胞器共纯化。作为该系统中突触囊泡样细胞器的标志物,我们使用了整合膜糖蛋白p38或突触素。我们表明,PC12细胞中富含p38的部分在平衡梯度上与大鼠脑突触囊泡共迁移。我们还证明p38从致密核心颗粒中纯化出来;在我们的致密颗粒部分中发现的这种蛋白质不到5%。最后,我们表明在脉冲追踪实验中p38不会通过致密颗粒部分。这些结果排除了p38通过成熟的致密颗粒到达小的清亮囊泡的可能性,并暗示这些细胞可能有两条独立衍生的调节途径。

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