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一氧化氮介导的哺乳动物心率胆碱能控制的细胞机制。

A cellular mechanism for nitric oxide-mediated cholinergic control of mammalian heart rate.

作者信息

Han X, Shimoni Y, Giles W R

机构信息

Department of Medical Physiology and Medicine, University of Calgary, Alberta, Canada.

出版信息

J Gen Physiol. 1995 Jul;106(1):45-65. doi: 10.1085/jgp.106.1.45.

Abstract

The biochemical signaling pathways involved in nitric oxide (NO)-mediated cholinergic inhibition of L-type Ca2+ current (ICa[L]) were investigated in isolated primary pacemaker cells from the rabbit sinoatrial node (SAN) using the nystatin-perforated whole-cell voltage clamp technique. Carbamylcholine (CCh; 1 microM), a stable analogue of acetylcholine, significantly inhibited ICa(L) after it had been augmented by isoproterenol (ISO; 1 microM). CCh also activated an outward K+ current, IK(ACh). Both of these effects of CCh were blocked completely by atropine. Preincubation of the SAN cells with L-nitro-arginine methyl ester (L-NAME; 0.2-1 mM), which inhibits NO synthase (NOS), abolished the CCh-induced attenuation of ICa(L) but had no effect on IK(ACh). Coincubation of cells with both L-NAME and the endogenous substrate of NOS, L-arginine (1 nM), restored the CCh-induced attenuation of ICa(L), indicating that L-NAME did not directly interfere with the muscarinic action of CCh on ICa(L). In the presence of ISO the CCh-induced inhibition of ICa(L) could be mimicked by the NO donor 3-morpholino-sydnonimine (SIN-1; 0.1 mM). SIN-1 had no effect on its own or after a maximal effect of CCh had developed, indicating that it does not inhibit ICa(L) directly. SIN-1 failed to activate IK(ACh), demonstrating that it did not activate muscarinic receptors. Both CCh and NO are known to activate guanylyl cyclase and elevate intracellular cGMP. External application of methylene blue (10 microM), which interferes with the ability of NO to activate guanylyl cyclase, blocked the CCh-induced attenuation of ICa(L). However, it also blocked the activation of IK(ACh), suggesting an additional effect on muscarinic receptors or G proteins. To address this, a separate series of experiments was performed using conventional whole-cell recordings with methylene blue in the pipette. Under these conditions, the CCh-induced attenuation of ICa(L) was blocked, but the activation of IK(ACh) was still observed. Methylene blue also blocked the SIN-1-induced decrease in ICa(L). 6-anilino-5,8-quinolinedione (LY83583; 30 microM), an agent known to decrease both basal and CCh-stimulated cGMP levels, prevented the inhibitory effects of both CCh and SIN-1 on ICa(L), but had no effect on the activation of IK(ACh) by CCh. In combination, these results show that CCh- and NO-induced inhibition of ICa(L) is mediated by cGMP.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

采用制霉菌素穿孔全细胞膜片钳技术,在兔窦房结(SAN)分离的原代起搏细胞中,研究了一氧化氮(NO)介导的胆碱能抑制L型钙电流(ICa[L])所涉及的生化信号通路。氨甲酰胆碱(CCh;1 μM)是乙酰胆碱的稳定类似物,在异丙肾上腺素(ISO;1 μM)增强ICa(L)后,能显著抑制ICa(L)。CCh还激活了外向钾电流IK(ACh)。CCh的这两种效应均被阿托品完全阻断。用抑制一氧化氮合酶(NOS)的L-硝基-精氨酸甲酯(L-NAME;0.2 - 1 mM)预孵育SAN细胞,可消除CCh诱导的ICa(L)衰减,但对IK(ACh)无影响。将细胞与L-NAME和NOS的内源性底物L-精氨酸(1 nM)共同孵育,可恢复CCh诱导的ICa(L)衰减,表明L-NAME并未直接干扰CCh对ICa(L)的毒蕈碱样作用。在ISO存在的情况下,NO供体3-吗啉代-西多胺(SIN-1;0.1 mM)可模拟CCh诱导的ICa(L)抑制作用。SIN-1单独作用时或在CCh产生最大效应后均无作用,表明它不直接抑制ICa(L)。SIN-1未能激活IK(ACh),表明它未激活毒蕈碱受体。已知CCh和NO均可激活鸟苷酸环化酶并提高细胞内cGMP水平。外用亚甲蓝(10 μM)可干扰NO激活鸟苷酸环化酶的能力,阻断CCh诱导的ICa(L)衰减。然而,它也阻断了IK(ACh)的激活,提示对毒蕈碱受体或G蛋白有额外作用。为解决此问题,使用移液管中含有亚甲蓝的传统全细胞记录进行了另一系列实验。在这些条件下,CCh诱导的ICa(L)衰减被阻断,但仍观察到IK(ACh)的激活。亚甲蓝还阻断了SIN-1诱导的ICa(L)降低。6-苯胺基-5,8-喹啉二酮(LY83583;30 μM)是一种已知可降低基础和CCh刺激的cGMP水平的药物,可预防CCh和SIN-1对ICa(L)的抑制作用,但对CCh激活IK(ACh)无影响。综合这些结果表明,CCh和NO诱导的ICa(L)抑制是由cGMP介导的。(摘要截断于400字)

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