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Optical Recording Reveals Novel Properties of GSK1016790A-Induced Vanilloid Transient Receptor Potential Channel TRPV4 Activity in Primary Human Endothelial Cells

机译:光学记录揭示了人类原代内皮细胞中GSK1016790A诱导的类香草酸瞬时受体潜在通道TRPV4活性的新特性。

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摘要

Critical functions of the vascular endothelium are regulated by changes in intracellular [Ca2+]. Endothelial dysfunction is tightly associated with cardiovascular disease, and improved understanding of Ca2+ entry pathways in these cells will have a significant impact on human health. However, much about Ca2+ influx channels in endothelial cells remains unknown because they are difficult to study using conventional patch-clamp electrophysiology. Here we describe a novel, highly efficient method for recording and analyzing Ca2+-permeable channel activity in primary human endothelial cells using a unique combination of total internal reflection fluorescence microscopy (TIRFM), custom software-based detection, and selective pharmacology. Our findings indicate that activity of the vanilloid (V) transient receptor potential (TRP) channel TRPV4 can be rapidly recorded and characterized at the single-channel level using this method, providing novel insight into channel function. Using this method, we show that although TRPV4 protein is evenly distributed throughout the plasma membrane, most channels are silent even during maximal stimulation with the potent TRPV4 agonist N-((1S)-1-{[4-((2S)-2-{[(2,4-dichlorophenyl)sulfonyl]amino}-3-hydroxypropanoyl)-1-piperazinyl]carbonyl}-3-methylbutyl)-1-benzothiophene-2-carboxamide (GSK1016790A). Furthermore, our findings indicate that GSK1016790A acts by recruiting previously inactive channels, rather than through increasing elevation of basal activity.
机译:血管内皮的关键功能受细胞内[Ca 2 + ]变化的调节。内皮功能障碍与心血管疾病紧密相关,对这些细胞中Ca 2 + 进入途径的了解的改善将对人类健康产生重大影响。然而,内皮细胞中Ca 2 + 的大量流入通道仍是未知的,因为很难使用常规的膜片钳电生理学对其进行研究。在这里,我们描述了一种新颖的,高效的方法,该方法使用全内反射荧光显微镜(TIRFM)(基于定制软件)的独特组合来记录和分析原代人内皮细胞中Ca 2 + 的通道活性检测和选择性药理学。我们的发现表明,使用这种方法可以在单通道水平上快速记录和表征类香草酸(V)瞬态受体电位(TRP)通道TRPV4的活性,从而提供对通道功能的新颖见解。使用这种方法,我们显示,尽管TRPV4蛋白均匀地分布在整个质膜上,但是即使在有效的TRPV4激动剂N-((1S)-1-{[4-((2S)-2 -{[((2,4-二氯苯基)磺酰基]氨基} -3-羟基丙酰基)-1-哌嗪基]羰基} -3-甲基丁基)-1-苯并噻吩-2-羧酰胺(GSK1016790A)。此外,我们的发现表明,GSK1016790A通过募集以前不活跃的通道而不是通过增加基础活性来发挥作用。

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