>1 The effects of tubocurarine, hexamethonium and trimetaphan on the synaptic currents of rat submandibular ganglion cells have been measured at 20°C by means of a two-microelectrode voltage-clamp system. The aim was to distinguish between the receptor-blocking and channel-blocking actions of those drugs, and to test for possible selectivity of action on the `fast' and `slow' acetylcholine-operated channels.>2 Tubocurarine had no effect on the amplitude of evoked synaptic currents (e.s.cs) or miniature synaptic currents (m.s.cs), except at concentrations exceeding 20 μM. The slow component of the e.s.c. was shortened by tubocurarine, this effect becoming more marked as the cell was hyperpolarized. The timecourse of m.s.cs, which have no slow component, was unaffected.>3 Hexamethonium (2-30 μM) caused a voltage-dependent reduction of e.s.c. amplitude, and voltage-dependent shortening of both fast and slow components of the e.s.c. M.s.cs were also shortened.>4 Trimetaphan (2-10 μM) reduced the amplitude of e.s.cs and m.s.cs. Neither component of the e.s.c. was shortened by trimetaphan; however, the slow component was reduced in amplitude more than the fast component, so that the overall duration of the e.s.c. appeared to be reduced. At higher concentrations (15-25 μM) trimetaphan clearly shortened the fast component.>5 It is concluded that tubocurarine acts selectively on the slow ionic channels, the association rate constant being 2.8 × 106 M-1 s-1 at -80 mV. Hexamethonium acts on both fast and slow channels, the association rate constants, at -80 mV, being respectively 5.3 × 106 M-1 s-1 and 1.3 × 107 M-1 s-1. With both drugs, the association rate constant increases if the cell is hyperpolarized, this effect being more pronounced with hexamethonium than with tubocurarine.>6 The marked voltage-dependent reduction of e.s.c. amplitude by hexamethonium cannot be accounted for by open channel block, and requires an additional mechanism, the nature of which is discussed.>7 Trimetaphan, at low concentrations, acts in a way consistent with receptor block, and shows a degree of selectivity for the slow component of the e.s.c.>8 In an appendix, the effect of temporal dispersion of the time of opening of ionic channels on the amplitude and time-course of the composite synaptic response is analysed. It is concluded that the shortening of the time-constant of the e.s.c. decay by hexamethonium cannot, by itself, account for the drug's effect on e.s.c. amplitude.
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机译:> 1 已在20°C下通过双微电极电压钳系统测量了微管尿素,六甲铵和三甲芬对大鼠下颌神经节细胞突触电流的影响。目的是区分这些药物的受体阻断作用和通道阻断作用,并测试在“快”和“慢”乙酰胆碱操纵的通道上可能的选择性。> 2 除了浓度超过20μM时,对诱发的突触电流(escs)或微型突触电流(mscs)的幅度没有影响。 e.s.c.的慢组件通过微管尿素缩短,这种作用随着细胞超极化而变得更加明显。 m.s.cs的时间进程不受影响,不受影响。> 3 六方铵(2-30μM)导致e.s.c的电压依赖性降低。 e.s.c的快速和慢速分量的幅度和电压相关的缩短M.s.cs也缩短了。> 4 Trimetaphan(2-10μM)降低了e.s.cs和m.s.cs的幅度。 e.s.c.的任何一个被曲美他芬缩短;但是,慢速分量的幅度比快速分量的减小幅度更大,因此es.c.似乎减少了。在较高浓度(15-25μM)下,曲美他汀明显缩短了快速组分。> 5 结论是微管尿素选择性作用于慢速离子通道,缔合速率常数为2.8×10 6 < / sup> M -1 s -1 在-80 mV时。六甲铵同时作用于快通道和慢通道,缔合速率常数为-80 mV,分别为5.3×10 6 M -1 s -1 和1.3×10 7 M -1 s -1 。两种药物,如果细胞超极化,缔合速率常数都会增加,六甲铵比微管尿素更明显。> 6 。六甲铵的振幅不能用明渠阻滞来解释,它需要一个附加的机制,其性质已经讨论过。> 7 低浓度的三甲a以与受体阻滞一致的方式起作用,并显示esc > 8 的慢速成分的选择性程度。在附录中,分析了离子通道打开时间的时间色散对复合突触响应的幅度和时程的影响。可以得出结论,e.s.c。的时间常数的缩短。六甲铵的衰变本身不能解释药物对e.s.c.的影响。振幅。
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