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Ionic requirements for membrane oscillations and their dependence on the calcium concentration in a molluscan pace-maker neurone

机译:膜振荡的离子要求及其对软体动物起搏器神经元中钙浓度的依赖性

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1. Membrane currents from the bursting pace-maker neurone R-15 of Aplysia were measured under conditions designed to simulate membrane oscillations. Changes in the absorbance of the Ca2+-sensitive dye arsenazo III were used to monitor changes in the free intracellular Ca2+ concentration, [Ca]i, under these conditions. In addition, changes in the extracellular K+, concentration [K]o were measured with K+-sensitive electrodes.2. In normal external ionic conditions the depolarizing phase of pace-maker activity was associated with a slow inward current and the hyperpolarizing phase with a slow outward current.3. In cells where the early inward Na+ current was blocked by tetrodotoxin and outward K+ currents were suppressed by intracellular EGTA and extracellular tetraethylammonium and 4-aminopyridine, the slow inward current was significantly larger in amplitude and was suppressed by removal of external Ca2+ or the addition of external La3+, but not by the removal of external Na+.4. The slow inward current was increased when [Ca]o was raised and decreased when it was reduced in the manner expected for current flow through a Ca2+ channel. The selectivity of the slow inward current for divalent cations was [Formula: see text].5. The slow inward current was only slightly reduced by a 10 °C reduction in temperature.6. In normal external and internal ionic conditions changes in dye absorbance occurred when the membrane was depolarized with slow triangular voltage ramps or long depolarizing steps within the pace-maker oscillation range. The obsorbance change, and thus the increase in Ca2+, [Ca]i, was well correlated with the appearance of the slow inward current. Moreover, the magnitude of the slow outward current was dependent upon the change in [Ca]i.7. The slow inward current and a substantial fraction of the outward current, as well as the change in [Ca]i, were reduced appreciably by the addition of La3+ ions (3 mM) to the external medium.8. The increase in [Ca]i during prolonged depolarization was not affected by external tetrodotoxin or by the removal of external Na+, but was abolished by a Ca2+-free external medium containing EGTA. Nevertheless, significant changes occurred in [Ca]i during depolarization in 0·1 mM-external Ca2+.9. In normal external and internal ionic conditions extracellular K+, [K]o, increased during the depolarizing phase of the pace-maker cycle and decayed during the hyperpolarizing phase.10. There was a measurable increase in [K]o during small prolonged depolarizing steps which produced a net inward current, indicating that inward and outward currents overlap under normal conditions.11. In the absence of action potential discharge, [Ca]i increased during the depolarizing phase and decreased during the hyperpolarizing phase of the membrane oscillation.12. It is proposed that pace-maker oscillations depend upon three separate but linked systems which include a voltage-dependent Ca2+ current, the free intracellular Ca2+ concentration and the Ca2+-activated K+ current.
机译:1.在旨在模拟膜振荡的条件下,测量了来自海ly突触起搏器神经元R-15的膜电流。在这些条件下,使用Ca 2 + 敏感染料砷偶氮III的吸光度变化来监测游离细胞内Ca 2 + 浓度[Ca] i的变化。 。另外,用K + 敏感电极测量细胞外K + ,浓度[K] o的变化。2。在正常的外部离子条件下,起搏器活动的去极化阶段与缓慢的内向电流相关,而超极化阶段与缓慢的外向电流相关。3。在河豚毒素阻断了早期向内Na + 电流并被细胞内EGTA和细胞外四乙铵和4-氨基吡啶抑制了向外向K + 电流的情况下,缓慢向内的电流为幅度显着增大,并且通过去除外部Ca 2 + 或添加外部La 3 + 受到抑制,但没有通过去除外部Na + < /sup>.4。缓慢的内向电流在增加[Ca] o时会增加,而在减小它时会以预期流过Ca 2 + 通道的方式减少。缓慢的内向电流对二价阳离子的选择性为[分子式:见正文] .5。缓慢的内向电流仅因温度降低10°C而略有减小6。在正常的外部和内部离子条件下,当膜在起搏器振荡范围内以缓慢的三角电压斜坡或长的去极化步骤去极化时,会发生染料吸收率的变化。吸光度的变化,因此Ca 2 + [Ca] i的增加与缓慢的内向电流的出现密切相关。而且,缓慢的向外电流的大小取决于[Ca 1,7]的变化。通过向外部介质中添加La 3 + 离子(3 mM),可以显着降低缓慢的内向电流和大部分外向电流,以及[Ca] i的变化。 .8。长时间去极化过程中[Ca] i的增加不受外部河豚毒素或外部Na + 的去除的影响,但被无Ca 2 + 的外部外部消除含有EGTA的培养基。尽管如此,在去极化过程中,在0·1 mM外部Ca 2 + .9中[Ca] i发生了显着变化。在正常的外部和内部离子条件下,细胞外K + [K] o在起搏器周期的去极化阶段增加,而在超极化阶段衰减[10]。在小的延长的去极化步骤中,[K] o有可测量的增加,产生净的内向电流,表明在正常条件下,内向和向外的电流重叠。11。在没有动作电位放电的情况下,[Ca] i在膜振荡的去极化阶段增加而在超极化阶段减少[12]。建议起搏器振荡取决于三个独立但相互联系的系统,这些系统包括电压依赖性Ca 2 + 电流,细胞内游离Ca 2 + 浓度和Ca 2 + 激活的K + 电流。

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