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介导肠道平滑肌收缩钙敏化的毒蕈碱受体亚型:受体敲除小鼠的研究

Muscarinic receptor subtypes mediating Ca2+ sensitization of intestinal smooth muscle contraction: studies with receptor knockout mice.

作者信息

Suguro Mayuko, Matsuyama Hayato, Tanahashi Yasuyuki, Unno Toshihiro, Kitazawa Takio, Yamada Masahisa, Komori Seiichi

机构信息

Laboratory of Veterinary Pharmacology, Department of Veterinary Medicine, Faculty of Applied Biological Science, Gifu University.

出版信息

J Vet Med Sci. 2010 Apr;72(4):443-51. doi: 10.1292/jvms.09-0458. Epub 2009 Dec 15.

DOI:10.1292/jvms.09-0458
PMID:20009428
Abstract

In the present study, we have characterized muscarinic receptor subtypes that mediate carbachol-induced Ca2+ sensitization of contraction in intestinal smooth muscle, using mutant mice lacking M(2) or M(3) muscarinic receptors or both receptor subtypes. In alpha-toxin-permeabilized muscle strips from wild-type (WT) mice, isometric tension responses to Ca2+ applied cumulatively (pCa 7.0-5.0) were increased when the muscarinic agonist carbachol (100 microM) was added to the medium, as judged from shifts of pCa-tension curves in both 50% effective concentration (EC(50)) and maximum response (E(max)) of pCa-tension curve. In preparations from M(2)-knockout (KO) mice, pCa-tension curves were also shifted by carbachol (100 microM), and the extents of the EC(50) and E(max) changes resembled those observed in preparations from WT mice. In preparations from M(3)-KO or M(2)/M(3)-double KO mice, however, no significant changes in pCa-tension curves were obtained after carbachol application. The G(q/11)-type G-protein inhibitor YM-254890 (1 microM) completely blocked the Ca2+ sensitization of contraction induced by carbachol in M(2)-KO or WT preparations. The results strongly support the idea that the muscarinic activation of Ca2+ sensitization in intestinal smooth muscles is mediated by the M(3) muscarinic receptor coupled to G(q/11)-type G-proteins, without any significant involvement of the other muscarinic receptor subtypes including M(2).

摘要

在本研究中,我们利用缺乏M(2)或M(3)毒蕈碱受体或两种受体亚型的突变小鼠,对介导卡巴胆碱诱导肠平滑肌收缩Ca2+敏感性的毒蕈碱受体亚型进行了表征。在来自野生型(WT)小鼠的经α-毒素通透的肌条中,当向培养基中加入毒蕈碱激动剂卡巴胆碱(100μM)时,根据pCa-张力曲线在50%有效浓度(EC(50))和pCa-张力曲线最大反应(E(max))的变化判断,对累积施加的Ca2+(pCa 7.0 - 5.0)的等长张力反应增加。在来自M(2)基因敲除(KO)小鼠的制剂中,卡巴胆碱(100μM)也使pCa-张力曲线发生移位,EC(50)和E(max)变化程度与在WT小鼠制剂中观察到的相似。然而,在来自M(3)-KO或M(2)/M(3)-双KO小鼠的制剂中,施加卡巴胆碱后pCa-张力曲线没有显著变化。G(q/11)型G蛋白抑制剂YM-254890(1μM)完全阻断了卡巴胆碱在M(2)-KO或WT制剂中诱导的收缩Ca2+敏感性。结果有力地支持了这样一种观点,即肠平滑肌中Ca2+敏感性的毒蕈碱激活是由与G(q/11)型G蛋白偶联的M(3)毒蕈碱受体介导的,而其他毒蕈碱受体亚型(包括M(2))没有任何显著参与。

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