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肌球蛋白II在嗜铬细胞囊泡运输与融合过程中的新作用

New roles of myosin II during vesicle transport and fusion in chromaffin cells.

作者信息

Neco Patricia, Giner Daniel, Viniegra Salvador, Borges Ricardo, Villarroel Alvaro, Gutiérrez Luis M

机构信息

Instituto de Neurociencias, Centro Mixto CSIC-Universidad Miguel Hernandez, E-03550 Alicante, Spain.

出版信息

J Biol Chem. 2004 Jun 25;279(26):27450-7. doi: 10.1074/jbc.M311462200. Epub 2004 Apr 6.

DOI:10.1074/jbc.M311462200
PMID:15069078
Abstract

Modified herpes virus (amplicons) were used to express myosin regulatory light chain (RLC) chimeras with green fluorescent protein (GFP) in cultured bovine chromaffin cells to study myosin II implication in secretion. After infection, RLC-GFP constructs were clearly identified in the cytoplasm and accumulated in the cortical region, forming a complex network that co-localized with cortical F-actin. Cells expressing wild type RLC-GFP maintained normal vesicle mobility, whereas cells expressing an unphosphorylatable form (T18A/S19A RLC-GFP) presented severe restrictions in granule movement as measured by individual tracking in dynamic confocal microscopy studies. Interestingly, the overexpression of this mutant form of RLC also affected the initial secretory burst elicited by either high K(+) or BaCl(2), as well as the secretion induced by fast release of calcium from caged compounds in individual cells. Moreover, T18A/S19A RLC-GFP-infected cells presented slower fusion kinetics of individual granules compared with controls as measured by analysis of amperometric spikes. Taken together, our results demonstrate the implication of myosin II in the transport of vesicles, and, surprisingly, in the final phases of exocytosis involving transitions affecting the activity of docked granules, and therefore uncovering a new role for this cytoskeletal element.

摘要

修饰的疱疹病毒(扩增子)用于在培养的牛嗜铬细胞中表达带有绿色荧光蛋白(GFP)的肌球蛋白调节轻链(RLC)嵌合体,以研究肌球蛋白II在分泌中的作用。感染后,RLC-GFP构建体在细胞质中清晰可见,并在皮质区域积累,形成与皮质F-肌动蛋白共定位的复杂网络。表达野生型RLC-GFP的细胞维持正常的囊泡移动性,而表达不可磷酸化形式(T18A/S19A RLC-GFP)的细胞在动态共聚焦显微镜研究中通过个体追踪测量显示颗粒运动受到严重限制。有趣的是,这种突变形式的RLC的过表达也影响了由高钾(+)或氯化钡引发的初始分泌爆发,以及单个细胞中笼形化合物快速释放钙诱导的分泌。此外,通过分析电流尖峰测量,与对照相比,T18A/S19A RLC-GFP感染的细胞单个颗粒的融合动力学较慢。综上所述,我们的结果证明了肌球蛋白II在囊泡运输中的作用,并且令人惊讶的是,在涉及影响停靠颗粒活性转变的胞吐作用的最后阶段,从而揭示了这种细胞骨架元件的新作用。

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