首页> 美国卫生研究院文献>The Journal of Physiology >A Na+-activated K+ current in cultured brain stem neurones from chicks.
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A Na+-activated K+ current in cultured brain stem neurones from chicks.

机译:雏鸡培养的脑干神经元中的Na +激活的K +电流。

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摘要

1. Patch-clamp techniques were used to study the properties of a Na+-activated K+ current (IK(Na) in neurones cultured from embryonic chick brain stem. 2. With whole-cell clamp, a depolarizing voltage command evoked an inward current that was followed by an outward current with two components, the first transient, the second sustained. 3. Tetrodotoxin (TTX, 1 microM) eliminated the inward current and the transient component of the outward current, without affecting the sustained outward current. In addition, the transient outward current was attenuated when all external Na+ was replaced by Li+, suggesting that it was activated specifically by Na+ entry into the cell. 4. The time course of the transient outward current was obtained by subtracting records obtained in Li+ solution from those obtained in Na+ solution. There was significant overlap between the decay of the inward current and the onset of the transient outward current. 5. When just after the peak of the transient outward current, the membrane was stepped to progressively more hyperpolarized levels, the tail currents associated with the current reversed polarity near the calculated K+ equilibrium potential. 6. 4-Aminopyridine (4-AP, 4 mM) abolished the transient outward current and approximately half of the sustained late current. Tetraethylammonium (TEA, 2 mM) had no effect on the transient current, but reduced the sustained current slightly. 7. Inside-out patches, made in LiCl bathing solutions, contained channels that were activated by exposing the cytoplasmic face of the patch to Na+. Channel activity continued as long as Na+ was present. 8. The single-channel currents reversed at the K+ equilibrium potential, and were associated with a main conductance that depended upon K+ concentration (about 50 pS with [K+]o = 15 mM, [K+]i = 5 mM, and 100 pS when [K+]i was increased to 75 mM). 9. The open probability of the channels increased with increasing cytoplasmic Na+ concentration. At [Na+]i = 150 mM (the maximum concentration tested), channels were open almost continuously. Open probability was considerably less at 50 mM, and still measureable at 20 mM. 10. The magnitude of IK(Na) and its overlap with the inward Na+ current indicate that these channels contribute significantly to the repolarizing phase of the action potential. In addition, the relation between channel activity and Na+ concentration suggests that the channels may make a measurable contribution to membrane conductance at resting intracellular Na+ concentrations.
机译:1.膜片钳技术用于研究Na +激活的K +电流(IK(Na))在胚胎鸡脑干培养的神经元中的特性; 2.通过全细胞钳制,去极化电压命令引起了内向电流,其次是具有两个分量的外向电流,第一个是瞬态的,第二个是持续的3.河豚毒素(TTX,1 microM)消除了内向电流和外向电流的瞬态分量,而不影响持续的外向电流。 4.当所有外部Na +都被Li +代替时,瞬态向外电流减弱,这表明Na +进入细胞后特别激活了该瞬态电流。在Na +溶液中,内向电流的衰减与瞬态向外电流的开始之间存在明显的重叠; 5.当瞬态向外电流的峰值刚好之后在这种情况下,膜被逐步提高到更多的超极化水平,与电流反向极性相关的尾电流接近计算出的K +平衡电位。 6. 4-氨基吡啶(4-AP,4 mM)消除了瞬态向外电流,并消除了持续后期电流的一半。四乙铵(TEA,2 mM)对瞬态电流没有影响,但略微降低了持续电流。 7.用LiCl沐浴液制成的由内而外的贴剂包含通道,这些通道通过将贴剂的细胞质表面暴露于Na +来激活。只要存在Na +,通道的活动就会持续。 8.单通道电流在K +平衡电位处反向,并与取决于K +浓度的主电导率相关([K +] o = 15 mM,[K +] i = 5 mM和100 pS时约为50 pS。当[K +] i增加到75 mM时)。 9.通道的开放概率随细胞质Na +浓度的增加而增加。在[Na +] i = 150 mM(测试的最大浓度)下,通道几乎连续打开。打开概率在50 mM时要小得多,但在20 mM时仍可测量。 10. IK(Na)的大小及其与内向Na +电流的重叠表明,这些通道对动作电位的复极化阶段起了很大作用。另外,通道活性与Na +浓度之间的关系表明,在静止的细胞内Na +浓度下,通道可对膜电导做出可测量的贡献。

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