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醛固酮通过1型血管紧张素受体依赖性机制下调延迟整流钾电流。

Aldosterone downregulates delayed rectifier potassium currents through an angiotensin type 1 receptor-dependent mechanism.

作者信息

Lv Yankun, Wang Yanjun, Zhu Xiaoran, Zhang Hua

机构信息

Heart Center, Hebei General Hospital Shijiazhuang, China.

Department of Acupuncture and Moxibustion, Affiliated Hospital of Hebei University of Chinese Medicine Shijiazhuang, China.

出版信息

Am J Transl Res. 2018 May 15;10(5):1413-1421. eCollection 2018.

Abstract

We have previously shown that aldosterone downregulates delayed rectifier potassium currents (I) via activation of the mineralocorticoid receptor (MR) in adult guinea pig cardiomyocytes. Here, we investigate whether angiotensin II/angiotensin type 1 receptor (AngII/AT1R) and intracellular calcium also play a role in these effects. Ventricular cardiomyocytes were isolated from adult guinea pigs and incubated with aldosterone (1 μmol·L) either alone or in combination with enalapril (1 μmol·L), losartan (1 μmol·L), nimodipine (1 μmol·L), or BAPTA-AM (2.5 μmol·L) for 24 h. We used the conventional whole cell patch-clamp technique to record the I component. In addition, we evaluated expression of the I subunits KCNQ1 and KCNE1 using Western blotting. Our results showed that both enalapril and losartan, but not nimodipine or BAPTA-AM, completely reversed the aldosterone-induced inhibition of I and its effects on KCNQ1/KCNE1 protein levels. Furthermore, we found that AngII/AT1R mediates the inhibitory effects of aldosterone on I. Finally, the downregulation of I induced by aldosterone did not occur secondarily to a change in intracellular calcium concentrations. Taken together, our findings demonstrate that crosstalk between MR and AT1R underlies the effects of aldosterone, and provide new insights into the mechanism underlying potassium channels.

摘要

我们之前已经表明,在成年豚鼠心肌细胞中,醛固酮通过激活盐皮质激素受体(MR)来下调延迟整流钾电流(I)。在此,我们研究血管紧张素II/血管紧张素1型受体(AngII/AT1R)和细胞内钙是否也在这些效应中发挥作用。从成年豚鼠中分离出心室肌细胞,单独用醛固酮(1μmol·L)或与依那普利(1μmol·L)、氯沙坦(1μmol·L)、尼莫地平(1μmol·L)或BAPTA-AM(2.5μmol·L)联合孵育24小时。我们使用传统的全细胞膜片钳技术记录I成分。此外,我们使用蛋白质印迹法评估I亚基KCNQ1和KCNE1的表达。我们的结果表明,依那普利和氯沙坦,但不是尼莫地平或BAPTA-AM,完全逆转了醛固酮诱导的I抑制及其对KCNQ1/KCNE1蛋白水平的影响。此外,我们发现AngII/AT1R介导了醛固酮对I的抑制作用。最后,醛固酮诱导的I下调并非继发于细胞内钙浓度的变化。综上所述,我们的研究结果表明,MR和AT1R之间的相互作用是醛固酮效应的基础,并为钾通道的潜在机制提供了新的见解。

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