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MYO1A (brush border myosin I) dynamics in the brush border of LLC-PK1-CL4 cells.

机译:LLC-PK1-CL4细胞刷状边界中的MYO1A(刷状边界肌球蛋白I)动力学。

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摘要

The kidney epithelial cell line, LLC-PK1-CL4 (CL4), forms a well ordered brush border (BB) on its apical surface. CL4 cells were used to examine the dynamics of MYO1A (M1A; formerly BB myosin I) within the BB using GFP-tagged MIA (GFP-M1A), MIA motor domain (GFP-MDIQ), and tail domain (GFP-Tail). GFP-beta-actin (GFP-Actin) was used to assess actin dynamics within the BB. GFP-M1A, GFP-Tail, but not GFP-MDIQ localized to the BB, indicating that the tail is sufficient for apical targeting of M1A. GFP-Actin targeted to all the actin domains of the cell including the BB. Fluorescence recovery after photobleaching analysis revealed that GFP-M1A and GFP-Tail turnover in the BB is rapid, approximately 80% complete in <1 min. As expected for an actin-based motor, ATP depletion resulted in significant inhibition of GFP-M1A turnover yet had little effect on GFP-Tail exchange. Rapid turnover of GFP-M1A and GFP-Tail was not due to actin turnover as GFP-Actin turnover in the BB was much slower. These results indicate that the BB population of M1A turns over rapidly, while its head and tail domains interact transiently with the core actin and plasma membrane, respectively. This rapidly exchanging pool of M1A envelops an actin core bundle that, by comparison, is static in structure.
机译:肾脏上皮细胞系LLC-PK1-CL4(CL4)在其顶端表面形成有序的刷状缘(BB)。使用GFP标记的MIA(GFP-M1A),MIA运动域(GFP-MDIQ)和尾部域(GFP-Tail),使用CL4细胞检查BB内MYO1A(M1A;以前为BB肌球蛋白I)的动力学。 GFP-β-肌动蛋白(GFP-肌动蛋白)用于评估BB中的肌动蛋白动力学。 GFP-M1A,GFP-Tail,但不定位于BB的GFP-MDIQ,表明该尾巴足以对M1A进行根尖靶向。 GFP-肌动蛋白靶向细胞的所有肌动蛋白域,包括BB。光漂白分析后的荧光恢复表明,BB中的GFP-M1A和GFP-Tail转换迅速,在不到1分钟的时间内完成了约80%的转换。如基于肌动蛋白的运动所预期的那样,ATP消耗导致GFP-M1A转换的显着抑制,而对GFP-尾巴交换几乎没有影响。 GFP-M1A和GFP-Tail的快速周转并非由于肌动蛋白周转,因为BB中的GFP-肌动蛋白周转慢得多。这些结果表明,M1A的BB群体快速翻身,而其头和尾结构域分别与核心肌动蛋白和质膜短暂相互作用。 M1A的这种快速交换池包围了肌动蛋白核心束,相比之下,肌动蛋白核心束在结构上是静态的。

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