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Simultaneous, real-time imaging of intracellular calcium and cellular traction force production

机译:同时实时成像细胞内钙和细胞牵引力

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Cells can sense and respond to different types of mechanical stimuli that can lead to changes in rate of cell division, cell orientation, cell motility, and gene expression. There is rapidly growing interest in understanding how these processes are regulated by mechano-chemical signaling mechanisms. The movement of fish epithelial keratocytes is regulated by the activation of stretch-activated calcium channels, which allow cells to trigger retraction of the rear cell margin, when forward movement is impeded. We have developed a new assay that permits imaging of intracellular calcium concentration simultaneously with the detection of traction forces generated by moving keratocytes. The assay consists of a thin sheet of gelatin embedded with a surface layer of small fluorescent marker beads, on which cells can move. The elastic properties of the gelatin substrata can be reproducibly varied over a wide range and are stable for long periods, while submerged beneath culture medium. Gelatin substrata are thin, transparent, and highly elastic, allowing real-time detection of changes in traction force production that are associated with transient increases in intracellular calcium and that occur in response to mechanical stretching.
机译:细胞可以感知并响应不同类型的机械刺激,从而导致细胞分裂速度,细胞方向,细胞运动性和基因表达发生变化。人们对理解机械化学信号机制如何调节这些过程的兴趣迅速增长。鱼上皮角质细胞的运动受拉伸激活钙通道的激活调节,当向前运动受阻时,钙通道允许细胞触发后细胞边缘的收缩。我们已经开发了一种新的测定方法,该方法可以对细胞内钙离子浓度进行成像,并检测移动的角膜细胞产生的牵引力。该测定法由一块明胶薄片组成,上面嵌有一层小的荧光标记珠,细胞可以在其上移动。明胶基质的弹性性质可以在很宽的范围内可复制地变化,并且在浸入培养基下时可以长期稳定。明胶基质很薄,透明且具有很高的弹性,因此可以实时检测与细胞内钙的瞬时增加相关的牵引力产生的变化,这些变化是由于机械拉伸而发生的。

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