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醛固酮对A6细胞中上皮钠通道生物合成、转运及功能表达的影响。

Effects of aldosterone on biosynthesis, traffic, and functional expression of epithelial sodium channels in A6 cells.

作者信息

Alvarez de la Rosa Diego, Li Hui, Canessa Cecilia M

机构信息

Department of Cellular and Molecular Physiology, Yale University School of Medicine, New Haven, CT 06510, USA.

出版信息

J Gen Physiol. 2002 May;119(5):427-42. doi: 10.1085/jgp.20028559.

Abstract

The collecting duct regulates Na(+) transport by adjusting the abundance/activity of epithelial Na(+) channels (ENaC). In this study we have investigated the synthesis, degradation, endocytosis, and activity of ENaC and the effects of aldosterone on these processes using endogenous channels expressed in the A6 cell line. Biochemical studies were performed with a newly raised set of specific antibodies against each of the three subunits of the amphibian ENaC. Our results indicate simultaneous transcription and translation of alpha, beta, and gamma subunits and enhancement of both processes by aldosterone: two- and fourfold increase, respectively. The biosynthesis of new channels can be followed by acquisition of endoglycosidase H-resistant oligosacharides in alpha and beta subunits and, in the case of alpha, by the appearance of a form resistant to reducing agents. The half-life of the total pool of subunits (t(1/2) 40-70 min) is longer than the fraction of channels in the apical membrane (t(1/2) 12-17 min). Aldosterone induces a fourfold increase in the abundance of the three subunits in the apical membrane without significant changes in the open probability, kinetics of single channels, or in the rate of degradation of ENaC subunits. Accordingly, the aldosterone response could be accounted by an increase in the abundance of apical channels due, at least in part, to de novo synthesis of subunits.

摘要

集合管通过调节上皮钠通道(ENaC)的丰度/活性来调控钠离子转运。在本研究中,我们利用A6细胞系中表达的内源性通道,研究了ENaC的合成、降解、内吞作用和活性,以及醛固酮对这些过程的影响。我们使用新制备的针对两栖类ENaC三个亚基的特异性抗体进行了生化研究。我们的结果表明,α、β和γ亚基同时进行转录和翻译,且醛固酮可增强这两个过程,分别增加两倍和四倍。新通道的生物合成可通过α和β亚基中获得对内切糖苷酶H有抗性的寡糖来追踪,就α亚基而言,还可通过出现对还原剂有抗性的形式来追踪。亚基总库的半衰期(t(1/2) 40 - 70分钟)长于顶端膜中通道的比例(t(1/2) 12 - 17分钟)。醛固酮使顶端膜中三个亚基的丰度增加四倍,而单通道的开放概率、动力学或ENaC亚基的降解速率均无显著变化。因此,醛固酮反应至少部分可归因于亚基的从头合成导致顶端通道丰度增加。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/59aa/2233818/290963509173/8559f1.jpg

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