首页> 美国卫生研究院文献>The Journal of Physiology >Calcium current in molluscan neurones: measurement under conditions which maximize its visibility.
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Calcium current in molluscan neurones: measurement under conditions which maximize its visibility.

机译:软体动物神经元中的钙电流:在使其可见度最大化的条件下进行测量。

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摘要

1. Membrane currents were studied in isolated somata of molluscan neurones from Archidoris monteryensis and Anisodoris nobilis. Under voltage clamp, inward current displayed a two phase time course, and in some cases a clear reversal potential difference could be shown for the fast and slow phases. The slower phase was carried predominantly by calcium ions. 2. The apparent magnitude of the slower phase was greatly influenced by conditions which altered potassium current flow. Blocking voltage-dependent potassium conductances, either by appropriate conditioning polarizations or by tetraethyl-ammonium (TEA) ion, enhanced the magnitude, while conditions which augmented potassium current made the slow phase disappear. 3. A fraction of the membrane potassium conductance was TEA insensitive. This fraction could be blocked by procedures which prevented internal levels of calcium from increasing during the voltage clamp pulse. Three such procedures were demonstrated; replacement of external calcium by magnesium, internal buffering by EGTA, and replacement of calcium by permeant barium. 4. Internal EGTA buffering or external barium in combination with external TEA produced an extreme change in membrane current as compared with the normal time course. Membrane current, when activated by pulses up to +50 mV, was net inward and showed only fractional inactivation over time courses running to several seconds. Pulses to voltages greater than +60 mV resulted in outward current. 5. It is concluded that under normal conditions the calcium conductance has the extended time course clearly evident under the modified conditions of paragraph 4 but that the calcium flux component is easily missed. 6. In agreement with several prior studies it is also concluded that a rise in internal calcium is causally related to a rise in potassium conductance. A transmembrane flux of calcium can be uncoupled from the gK increase by appropriate buffering of internal calcium. 7. The transient potassium current, IA, which bears a resemblance to calcium-dependent potassium transients in some muscle cells did not depend upon internal calcium but instead is a voltage-activated mechanism.
机译:1.研究了来自山顶阿奇多里氏菌和黑带茴香的软体动物神经元分离体的膜电流。在电压钳制下,内向电流显示两相时间过程,在某些情况下,快相和慢相可能会显示明显的反向电势差。较慢的相主要由钙离子携带。 2.改变钾电流的条件极大地影响了慢相的表观幅度。通过适当的调节极化或通过四乙基铵(TEA)离子来阻断电压依赖性钾电导,可增加幅度,而增加钾电流的条件会使慢相消失。 3.膜钾电导的一部分对TEA不敏感。该部分可通过阻止钙内部水平在电压钳制脉冲期间增加的程序来阻止。演示了三个这样的程序;用镁代替外部钙,用EGTA代替内部缓冲,并用渗透钡代替钙。 4.与正常时程相比,内部EGTA缓冲液或外部钡与外部TEA的结合产生了膜电流的极大变化。膜电流,当被高达+50 mV的脉冲激活时,是净内向的,并且在经过几秒钟的时间过程中仅表现出部分失活。脉冲至大于+60 mV的电压会导致向外的电流。 5.结论是,在正常条件下,钙电导具有延长的时间过程,这在第4段的修改条件下显而易见,但是钙通量成分很容易被遗漏。 6.与先前的一些研究一致,还得出结论,内部钙的增加与钾电导的增加有因果关系。钙的跨膜通量可以通过内部钙的适当缓冲与gK的增加解耦。 7.瞬态钾电流IA与某些肌肉细胞中钙依赖性钾的瞬态相似,它不依赖于内部钙,而是一种电压激活的机制。

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