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蛙肾近端肾小管细胞中缺乏KCNQ1依赖性钾离子通量。

Absence of KCNQ1-dependent K+ fluxes in proximal tubular cells of frog kidney.

作者信息

Cemerikic Dusan, Nesovic-Ostojic Jelena, Popadic Dusan, Knezevic Aleksandra, Dragovic Simon, Milovanovic Aleksandar, Milovanovic Jovica

机构信息

Department of Pathological Physiology, Medical Faculty, Dr Subotica 1/II, 11000 Belgrade, Serbia.

出版信息

Comp Biochem Physiol A Mol Integr Physiol. 2007 Nov;148(3):635-44. doi: 10.1016/j.cbpa.2007.08.010. Epub 2007 Aug 15.

Abstract

The present study was designed to investigate the functional significance of KCNQ1-mediated K+ secretory fluxes in proximal tubular cells of the frog kidney. To this end, we investigated the effects on rapid depolarization and slow repolarization of the peritubular membrane potential after luminal addition of L-phenylalanine or L-alanine plus/minus KCNQ1 channel blockers. Perfusing the lumen with 10 mmol/L L-phenylalanine plus/minus luminal 293B, a specific blocker of KCNQ1, did not modify the rapid depolarization and the rate of slow repolarization. Perfusing the lumen with 10 mmol/L L-alanine plus/minus luminal HMR-1556, a more potent KCNQ1 channel blocker, did not also alter the rapid depolarization and the rate of slow repolarization. Pretreatment (1 h) of the lumen with HMR-1556 also failed to modify rapid depolarization and rate of slow repolarization upon luminal 10 mmol/L L-alanine. Perfusing the lumen with 1 mmol/L L-alanine plus/minus luminal HMR-1556 did not change the rapid depolarization and the rate of slow repolarization. The pretreatment (1 h) with luminal HMR-1556 did not modify the rapid depolarization and the rate of slow repolarization upon luminal 1 mmol/L L-alanine. The pretreatment (1 h) of the lumen with HMR-1556 did not change transference number for K+ of peritubular cell membrane. Finally, luminal barium blunted the rapid depolarization upon application of luminal 1 mmol/L L-alanine. RT-PCR showed that KCNQ1 mRNA was not expressed in frog kidney. In conclusion, the KCNQ1-dependent K+ secretory fluxes are absent in proximal tubule of frog kidney.

摘要

本研究旨在探讨钾通道蛋白KCNQ1介导的钾离子分泌通量在蛙肾近端小管细胞中的功能意义。为此,我们研究了在管腔中添加L-苯丙氨酸或L-丙氨酸并加/减KCNQ1通道阻滞剂后,对肾小管周围膜电位快速去极化和缓慢复极化的影响。用10 mmol/L L-苯丙氨酸加/减管腔特异性KCNQ1阻滞剂293B灌注管腔,并未改变快速去极化和缓慢复极化速率。用10 mmol/L L-丙氨酸加/减管腔更有效的KCNQ1通道阻滞剂HMR-1556灌注管腔,也未改变快速去极化和缓慢复极化速率。用HMR-1556对管腔进行预处理(1小时),在管腔中加入10 mmol/L L-丙氨酸后,同样未能改变快速去极化和缓慢复极化速率。用1 mmol/L L-丙氨酸加/减管腔HMR-1556灌注管腔,未改变快速去极化和缓慢复极化速率。用管腔HMR-1556预处理(1小时),在管腔中加入1 mmol/L L-丙氨酸后,未改变快速去极化和缓慢复极化速率。用HMR-1556对管腔进行预处理(1小时),未改变肾小管周围细胞膜钾离子转移数。最后,管腔钡离子减弱了在管腔中施加1 mmol/L L-丙氨酸时的快速去极化。逆转录聚合酶链反应显示,蛙肾中未表达KCNQ1 mRNA。总之,蛙肾近端小管不存在依赖KCNQ1的钾离子分泌通量。

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