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钙动员刺激盘基网柄菌剪切流诱导的细胞运动。

Calcium mobilization stimulates Dictyostelium discoideum shear-flow-induced cell motility.

作者信息

Fache Sébastien, Dalous Jérémie, Engelund Mads, Hansen Christian, Chamaraux François, Fourcade Bertrand, Satre Michel, Devreotes Peter, Bruckert Franz

机构信息

Structures et Propriétés des Architectures Moléculaires (UMR 5919 CNRS), Département de Recherche Fondamentale sur la Matière Condensée, CEA-Grenoble, DRFMC/SI3M, 17 rue des Martyrs, 38054 Grenoble Cedex 09, France.

出版信息

J Cell Sci. 2005 Aug 1;118(Pt 15):3445-57. doi: 10.1242/jcs.02461.

DOI:10.1242/jcs.02461
PMID:16079287
Abstract

Application of hydrodynamic mild shear stress to adherent Dictyostelium discoideum vegetative cells triggers active actin cytoskeleton remodeling resulting in net cell movement along the flow. The average cell speed is strongly stimulated by external calcium (Ca2+, K50%=22 microM), but the directionality of the movement is almost unaffected. This calcium concentration is ten times higher than the one promoting cell adhesion to glass surfaces (K50%=2 microM). Addition of the calcium chelator EGTA or the Ca2+-channel blocker gadolinium (Gd3+) transiently stops cell movement. Monitoring the evolution of cell-surface contact area with time reveals that calcium stimulates cell speed by increasing the amplitude of both protrusion and retraction events at the cell edge, but not the frequency. As a consequence, with saturating external calcium concentrations, cells are sensitive to very low shear forces (20 pN; sigma=0.1 Pa). Moreover, a null-mutant lacking the unique Gbeta subunit does not respond to external Ca2+ changes (K50%>1000 microM), although the directionality of the movement is comparable with that of wild-type cells. Furthermore, cells lacking the inositol 1,4,5-trisphosphate receptor (IP3-receptor) exhibit a markedly reduced Ca2+ sensitivity. Thus, calcium release from internal stores and calcium entry through the plasma membrane modulate cell speed in response to shear stress.

摘要

对黏附的盘基网柄菌营养细胞施加流体动力学温和剪切应力会触发活跃的肌动蛋白细胞骨架重塑,导致细胞沿流动方向净移动。外部钙(Ca2+,K50% = 22 microM)能强烈刺激细胞的平均移动速度,但移动的方向性几乎不受影响。这个钙浓度比促进细胞黏附到玻璃表面的钙浓度(K50% = 2 microM)高十倍。添加钙螯合剂乙二醇双四乙酸(EGTA)或Ca2+通道阻滞剂钆(Gd3+)会使细胞移动暂时停止。监测细胞表面接触面积随时间的变化发现,钙通过增加细胞边缘突出和回缩事件的幅度来刺激细胞速度,而不是频率。因此,在外部钙浓度饱和的情况下,细胞对非常低的剪切力(20 pN;σ = 0.1 Pa)敏感。此外,缺乏独特Gβ亚基的无义突变体对外部Ca2+变化无反应(K50%>1000 microM),尽管其移动的方向性与野生型细胞相当。此外,缺乏肌醇1,4,5 - 三磷酸受体(IP3受体)的细胞对Ca2+的敏感性明显降低。因此,从内部储存释放的钙和通过质膜进入的钙会调节细胞对剪切应力的速度反应。

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