Mechanically activated ion channels are biological transducers that convert mechanical stimuli such as stretch or shear forces into electrical and biochemical signals. In mammals, mechanically activated channels are essential for the detection of external and internal stimuli in processes as diverse as touch sensation, hearing, red blood cell volume regulation, basal blood pressure regulation, and the sensation of urinary bladder fullness. While the function of mechanically activated ion channels has been extensively studied in the in vitro setting using the patch-clamp technique, assessing their function in their native environment remains a difficult task, often because of limited access to the sites of expression of these channels (e.g., afferent terminals, Merkel cells, baroreceptors, and kidney tubules) or difficulties applying the patch-clamp technique (e.g., the apical surfaces of urothelial umbrella cells). This protocol describes a procedure to assess mechanically evoked Ca(2+) transients using the fluorescent sensor GCaMP5G in an ex vivo urothelial preparation, a technique that could be readily adapted for the study of mechanically evoked Ca(2+) events in other native tissue preparations.
Ex Vivo Analysis of Mechanically Activated Ca2+ Transients in Urothelial Cells.
体外分析尿路上皮细胞中机械激活的Ca2+瞬变
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作者:Carattino Marcelo D, Ruiz Wily G, Apodaca Gerard
| 期刊: | Jove-Journal of Visualized Experiments | 影响因子: | 1.000 |
| 时间: | 2022 | 起止号: | 2022 Sep 28; (187):10 |
| doi: | 10.3791/64532 | 研究方向: | 细胞生物学 |
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