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Secretory vesicles in live cells are not free-floating but tethered to filamentous structures: A study using photonic force microscopy

机译:活细胞中的分泌囊泡不是自由漂浮的,而是束缚在丝状结构上:一项使用光子力显微镜的研究

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摘要

It is well established that actin and microtubule cytoskeletal systems are involved in organelle transport and membrane trafficking in cells. This is also true for the transport of secretory vesicles in neuroendocrine cells and neurons. It was however unclear whether secretory vesicles remain free-floating, only to associate with such cytoskeletal systems when needing transport. This hypothesis was tested using live pancreatic acinar cells in physiological buffer solutions, using the photonic force microscope (PFM). When membrane-bound secretory vesicles (0.2-1.2 urn in diameter) in live pancreatic acinar cells were trapped at the laser focus of the PFM and pulled, they were all found tethered to filamentous structures. Mild exposure of cells to nocodazole and cytochalasin B, disrupts the tether. Immunoblot analysis of isolated secretory vesicles, further demonstrated the association of actin, myosin V, and kinesin. These studies demonstrate for the first time that secretory vesicles in live pancreatic acinar cells are tethered and not free-floating, suggesting that following vesicle biogenesis, they are placed on their own railroad track, ready to be transported to their final destination within the cell when required. This makes sense, since precision and regulation are the hallmarks of all cellular process, and therefore would hold true for the transport and localization of subcellular organelles such as secretory vesicles.
机译:众所周知,肌动蛋白和微管细胞骨架系统参与细胞的细胞器运输和膜运输。对于神经内分泌细胞和神经元中分泌小泡的运输也是如此。然而,尚不清楚分泌性囊泡是否保持自由漂浮,仅在需要运输时才与这种细胞骨架系统结合。使用光子力显微镜(PFM)在生理缓冲溶液中使用活胰腺腺泡细胞测试了该假设。当活的胰腺腺泡细胞中膜结合的分泌囊泡(直径为0.2-1.2微米)被捕获在PFM的激光焦点处并被拉出时,它们全部被束缚成丝状结构。细胞轻度暴露于诺考达唑和细胞松弛素B会破坏系链。分离的分泌小泡的免疫印迹分析进一步证明了肌动蛋白,肌球蛋白V和驱动蛋白的关联。这些研究首次证明了活的胰腺腺泡细胞中的分泌囊泡是束缚的而不是自由漂浮的,这表明在囊泡生物发生之后,它们被置于自己的铁轨上,准备在运输时被转运到细胞内的最终目的地。需要。这是有道理的,因为精确度和调节是所有细胞过程的标志,因此对于亚细胞细胞器(例如分泌小泡)的运输和定位都是正确的。

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