Functional expression of TRPV4 channels in human collecting duct cells: implications for secondary hypertension in diabetic nephropathy.

Experimental Diabetes Research Pub Date : 2012-01-01 Epub Date: 2012-09-20 DOI:10.1155/2012/936518
Claire E Hills, Rosemary Bland, Paul E Squires
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引用次数: 21

Abstract

Background: The Vanilloid subfamily of transient receptor potential (TRPV) ion channels has been widely implicated in detecting osmotic and mechanical stress. In the current study, we examine the functional expression of TRPV4 channels in cell volume regulation in cells of the human collecting duct.

Methods: Western blot analysis, siRNA knockdown, and microfluorimetry were used to assess the expression and function of TRPV4 in mediating Ca²⁺-dependent mechanical stimulation within a novel system of the human collecting duct (HCD).

Results: Native and siRNA knockdown of TRPV4 protein expression was confirmed by western blot analysis. Touch was used as a cell-directed surrogate for osmotic stress. Mechanical stimulation of HCD cells evoked a transient increase in [Ca²⁺](i) that was dependent upon thapsigargin-sensitive store release and Ca²⁺ influx. At 48 hrs, high glucose and mannitol (25 mM) reduced TRPV4 expression by 54% and 24%, respectively. Similar treatment doubled SGK1 expression. Touch-evoked changes were negated following TRPV4 knockdown.

Conclusion: Our data confirm expression of Ca²⁺-dependent TRPV4 channels in HCD cells and suggest that a loss of expression in response to high glucose attenuates the ability of the collecting duct to exhibit regulatory volume decreases, an effect that may contribute to the pathology of fluid and electrolyte imbalance as observed in diabetic nephropathy.

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TRPV4通道在人收集管细胞中的功能表达:对糖尿病肾病继发性高血压的影响
背景:瞬时受体电位(TRPV)离子通道的香草亚家族广泛参与渗透和机械应力的检测。在本研究中,我们检测了TRPV4通道在人集束管细胞体积调节中的功能表达。方法:采用Western blot分析、siRNA敲低和微荧光法评估TRPV4在介导Ca 2 +依赖性机械刺激的新型人体集管(HCD)系统中的表达和功能。结果:western blot检测证实TRPV4蛋白表达下调,siRNA表达下调。Touch被用作细胞导向的渗透应激替代物。HCD细胞的机械刺激引起了[Ca 2 +](i)的短暂增加,这取决于thapsigargin敏感的存储释放和Ca 2 +的流入。48小时时,高糖和甘露醇(25 mM)分别使TRPV4表达降低54%和24%。类似处理使SGK1表达增加。TRPV4敲除后,触摸诱发的变化被否定。结论:我们的数据证实了Ca 2 +依赖TRPV4通道在HCD细胞中的表达,并且表明高糖反应中的表达缺失减弱了集管表现出调节性体积减少的能力,这可能导致糖尿病肾病中观察到的液体和电解质失衡的病理。
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来源期刊
Experimental Diabetes Research
Experimental Diabetes Research 医学-内分泌学与代谢
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3-8 weeks
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