首页> 美国卫生研究院文献>The Journal of Neuroscience >Organization of cortical cytoskeleton of cultured chromaffin cells and involvement in secretion as revealed by quick-freeze deep-etching and double-label immunoelectron microscopy
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Organization of cortical cytoskeleton of cultured chromaffin cells and involvement in secretion as revealed by quick-freeze deep-etching and double-label immunoelectron microscopy

机译:快速冷冻深蚀刻和双标记免疫电子显微镜显示培养的嗜铬细胞的皮质细胞骨架的组织和分泌的参与

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摘要

We have studied the organization of the cytoskeleton in both unstimulated and stimulated cultured chromaffin cells, as well as its relationship with their secretory process by exocytosis. We found the spatial heterogeneity in the intensity of cortical rhodamine-phalloidin staining within a cell. The overall staining pattern or intensity was minimally altered after stimulation, although dopamine-beta-hydroxylase (DBH) antigen, a marker for the chromaffin granule membrane, was exposed preferentially on the plasma membrane areas with lower intensity of rhodamine-phalloidin staining. Using the quick-freeze, deep-etch technique, we found the heterogeneity in the organization of cortical cytoskeletal networks--some regions have actin filament bundles running parallel to the plasma membrane interspersed between granules and the plasma membrane, while others have few actin filaments beneath the plasma membrane before stimulation. Actin filaments were rarely observed in the inner cytoplasm. We did not observe the overall change in its organization after stimulation. Double-label immunogold EM using anti-DBH antibody and anti-actin antibody combined with statistical analysis showed that (1) DBH was exposed on the plasma membrane preferentially where actin was sparse after stimulation (significant at less than 0.1%), although (2) regions having sparse actin were not always the sites for DBH exposure, and (3) the cortical actin zone was sometimes disrupted at the DBH-exposed sites after stimulation. The present data suggested that (1) secretion is related to heterogeneous organization of cortical cytoskeleton after stimulation and (2) massive synchronized reorganization of the cytoskeleton in the whole cell is not necessary for secretion, although small changes of the cytoskeleton might occur under local regulation at each exocytotic site at the moment of the release.
机译:我们已经研究了未刺激和刺激培养的嗜铬细胞中细胞骨架的组织,及其与胞吐作用分泌过程的关系。我们发现细胞内皮质若丹明-鬼笔环肽染色强度的空间异质性。尽管多巴胺-β-羟化酶(DBH)抗原(一种嗜铬粒颗粒膜的标记)抗原优先暴露于质膜区域,但若丹明-鬼笔环肽染色强度较低,但刺激后总体染色模式或强度变化很小。使用快速冷冻的深蚀刻技术,我们发现皮质细胞骨架网络的组织存在异质性-一些区域的肌动蛋白丝束平行于质膜,散布在颗粒和质膜之间,而另一些区域的肌动蛋白丝很少在刺激之前质膜下方。肌动蛋白丝很少在内部细胞质中观察到。我们没有观察到刺激后组织的整体变化。使用抗DBH抗体和抗肌动蛋白抗体的双标记免疫金EM结合统计分析表明,(1)DBH优先暴露在质膜上,刺激后肌动蛋白稀疏(显着低于0.1%),尽管(2 )肌动蛋白稀疏的区域并非始终是DBH暴露的部位,(3)刺激后,在暴露于DBH的部位有时会破坏皮质肌动蛋白区。目前的数据表明,(1)分泌与刺激后皮质细胞骨架的异质组织有关;(2)整个细胞中细胞骨架的大规模同步重组对于分泌不是必需的,尽管在局部调控下可能会发生细微的细胞骨架变化。在释放时在每个胞吐部位。

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