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豚鼠前列腺慢波活动的钾离子通道调节

K+ channel modulation of slow wave activity in the guinea-pig prostate.

作者信息

Nguyen D-T T, Lang R J, Exintaris B

机构信息

Department of Pharmaceutical Biology and Pharmacology, Prostate Research Co-operative, Victorian College of Pharmacy, Monash University, Parkville Victoria, Australia.

出版信息

Br J Pharmacol. 2007 Jul;151(6):828-36. doi: 10.1038/sj.bjp.0707283. Epub 2007 May 29.

Abstract

BACKGROUND AND PURPOSE

The aim of this study was to investigate the role of different K(+) channel populations and the inhibitory effect of various exogenously applied K(+) channel openers in the regulation of slow wave activity in the guinea-pig prostate.

EXPERIMENTAL APPROACH

Recordings of membrane potential were made using intracellular microelectrodes.

KEY RESULTS

Tetraethylammonium (TEA 300 micro M and 1 mM), iberiotoxin (150 nM) and 4-aminopyridine (4-AP 1 mM) increased the frequency of slow wave discharge. Apamin (1-200 nM) and glibenclamide (1 micro M) had no effect on slow wave activity. Lemakalim (1 micro M) and PCO-400 (1 micro M) abolished the slow waves, as did sodium nitroprusside (SNP 10 micro M) and calcitonin gene-related peptide (CGRP 100 nM). The inhibitory effect of these agents was independent of a significant change in membrane potential. In the presence of 4-AP (1 mM), TEA (1 mM) or glibenclamide (1 micro M) the inhibitory actions of SNP (10 micro M) were attenuated. The inhibitory actions of CGRP (100 nM) were also reversed by glibenclamide (1 micro M). In contrast, isoprenaline (1 micro M) did not alter the frequency of slow wave discharge.

CONCLUSIONS AND IMPLICATIONS

These results demonstrate that BK(Ca) and 4-AP-sensitive K(+) channels regulate the frequency of prostatic slow wave discharge. SNP and CGRP abolish slow waves in a hyperpolarisation-independent manner, partially via opening of K(ATP) channels. BK(Ca) and 4-AP-sensitive K(+) channels also play an important role in the SNP-induced inhibition of slow wave activity. The lack of membrane hyperpolarisation associated with the SNP- and CGRP-induced inhibition implies that the channels involved in this action are not predominantly located on the smooth muscle cells.

摘要

背景与目的

本研究旨在探讨不同钾离子通道群体的作用以及各种外源性应用的钾离子通道开放剂对豚鼠前列腺慢波活动调节的抑制作用。

实验方法

使用细胞内微电极记录膜电位。

主要结果

四乙铵(300 μM和1 mM)、iberiotoxin(150 nM)和4-氨基吡啶(4-AP 1 mM)增加了慢波放电频率。蜂毒明肽(1 - 200 nM)和格列本脲(1 μM)对慢波活动无影响。雷马卡林(1 μM)和PCO - 400(1 μM)消除了慢波,硝普钠(SNP 10 μM)和降钙素基因相关肽(CGRP 100 nM)也有同样效果。这些药物的抑制作用与膜电位的显著变化无关。在存在4-AP(1 mM)、TEA(1 mM)或格列本脲(1 μM)时SNP(10 μM)的抑制作用减弱。CGRP(100 nM)的抑制作用也被格列本脲(1 μM)逆转。相比之下,异丙肾上腺素(1 μM)未改变慢波放电频率。

结论与意义

这些结果表明大电导钙激活钾通道(BK(Ca))和对4-AP敏感的钾离子通道调节前列腺慢波放电频率。SNP和CGRP以不依赖超极化的方式消除慢波,部分是通过开放ATP敏感性钾通道(K(ATP)通道)。BK(Ca)和对4-AP敏感的钾离子通道在SNP诱导的慢波活动抑制中也起重要作用。SNP和CGRP诱导的抑制作用缺乏膜超极化表明参与此作用的通道并非主要位于平滑肌细胞上。

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