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A Two-Photon FRAP Analysis of the Cytoskeleton Dynamics in the Microvilli of Intestinal Cells

机译:两光子FRAP分析肠道细胞微绒毛中的细胞骨架动力学。

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摘要

The molecular structure of the brush-border of enterocytes has been investigated since the 1980s, but the dynamics of this highly specialized subcellular domain have been difficult to study due to its small size. To perform a detailed analysis of the dynamics of cytoskeleton proteins in this domain, we developed two-photon fluorescence recovery after photobleaching and a theoretical framework for data analysis. With this method, fast dynamics of proteins in the microvilli of the brush border of epithelial intestinal cells can be measured on the millisecond timescale in volumes smaller than 1 μm3. Two major proteins of the cytoskeleton of the microvilli, actin and myosin 1a (Myo1a; formerly named brush border myosin I), are mobile in the brush-border of Caco-2 cells, an enterocyte-like cellular model. However, the mobility of actin is very different from that of Myo1a and they appear to be unrelated (diffusion coefficient of 15 μm2 s−1 with a mobile fraction of 60% for actin, and 4 μm2 s−1 with a mobile fraction of 90% for Myo1a). Furthermore, we show for the first time, in vivo, that the dynamics of Myo1a in microvilli reflect its motor activity.
机译:自1980年代以来,已经研究了肠上皮细胞刷状边界的分子结构,但是由于其尺寸小,很难研究这种高度专业化的亚细胞结构域的动力学。为了对该域中细胞骨架蛋白的动力学进行详细分析,我们开发了光漂白后的双光子荧光恢复和用于数据分析的理论框架。使用这种方法,可以在毫秒时间尺度上以小于1μm 3 的体积测量上皮肠细胞刷状缘微绒毛中蛋白质的快速动态。微绒毛的细胞骨架的两个主要蛋白,肌动蛋白和肌球蛋白1a(Myo1a;以前称为刷状边界肌球蛋白I)在Caco-2细胞(一种肠上皮细胞样细胞模型)的刷边界中移动。但是,肌动蛋白的迁移率与Myo1a的迁移率非常不同,并且似乎无关(扩散系数为15μm 2 s -1 ,移动率为60%肌动蛋白的浓度为4μm 2 s -1 ,其中Myo1a的移动率为90%。此外,我们首次在体内显示出微绒毛中Myo1a的动力学反映了其运动活性。

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