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六放瘦星海星体卵细胞中的钙电流和钙激活内向电流。

Calcium current and calcium-activated inward current in the oocyte of the starfish Leptasterias hexactis.

作者信息

Lansman J B

机构信息

Department of Physiology, School of Medicine, University of California, Los Angeles 90024.

出版信息

J Physiol. 1987 Sep;390:397-413. doi: 10.1113/jphysiol.1987.sp016708.

Abstract
  1. Inward currents in the immature oocyte of the starfish Leptasterias hexactis were studied with a two-micro-electrode voltage clamp. Experiments investigated the role of Ca2+ in the Na+-dependent plateau of the action potential. 2. Voltage steps more positive than -55 mV produced inward currents in normal sea water that activated and then decayed to a non-zero level with a double-exponential time course. Returning the voltage to the resting potential produced an inward tail current that relaxed slowly to zero with a time course of seconds. 3. Replacing Na+ with choline abolished the slowly decaying component as well as the slow tail current which followed the end of the voltage pulse. This suggested that inward current in Na+-containing sea water consisted of a rapidly decaying component that flowed through Ca2+ channels and a more slowly decaying component carried by Na+. 4. Ca2+ current was isolated in Na+-free sea water. Activation followed a sigmoidal time course that could be described with m2 kinetics. Inactivation during a maintained depolarization followed first-order kinetics and was voltage dependent. 5. When Ba2+ was substituted for Ca2+ as the divalent ion charge carrier, inward currents in Na+-containing sea water decayed along a single-exponential time course. The absence of a slowly decaying Na+ current in Ba2+-containing sea water suggested that Na+ current depended on Ca2+ influx. 6. The effects of altering Ca2+ influx on the time course of Na+ current were investigated. Na+ current decayed more rapidly as the test pulse potential was made more positive, while raising [Ca2+]o slowed the decaying phase without altering its dependence on membrane potential. 7. Tail currents measured after rapidly stepping the membrane potential back to the resting level consisted of a fast component associated with the closing of Ca2+ channels and a slow component that was abolished by removing Na+. 8. The variation of the amplitude of the slow component of tail current with the duration of the voltage-clamp pulse indicated that Na+ current is associated with a time-dependent component of membrane conductance. 9. Possible mechanisms for the slowly decaying Na+ current are considered. The results are discussed in relation to the idea that the conductance change to Na+ follows the time course of Ca2+ accumulation and removal from the cytoplasm.
摘要
  1. 利用双微电极电压钳研究了六腕海星未成熟卵母细胞中的内向电流。实验探究了Ca2+在动作电位的Na+依赖性平台期所起的作用。2. 电压阶跃至比 -55 mV更正时,在正常海水中会产生内向电流,该电流激活后以双指数时间进程衰减至非零水平。将电压恢复到静息电位会产生内向尾电流,该尾电流以秒为时间进程缓慢弛豫至零。3. 用胆碱替代Na+消除了缓慢衰减成分以及跟随电压脉冲结束后的缓慢尾电流。这表明含Na+海水中的内向电流由流经Ca2+通道的快速衰减成分和由Na+携带的更缓慢衰减成分组成。4. 在无Na+海水中分离出Ca2+电流。激活遵循S形时间进程,可用m2动力学描述。在持续去极化期间的失活遵循一级动力学且依赖于电压。5. 当用Ba2+替代Ca2+作为二价离子电荷载体时,含Na+海水中的内向电流沿单指数时间进程衰减。含Ba2+海水中不存在缓慢衰减的Na+电流表明Na+电流依赖于Ca2+内流。6. 研究了改变Ca2+内流对Na+电流时间进程的影响。随着测试脉冲电位更正,Na+电流衰减更快,而提高[Ca2+]o减缓了衰减相,同时不改变其对膜电位的依赖性。7. 在将膜电位快速回拨到静息水平后测量的尾电流由与Ca2+通道关闭相关的快速成分和去除Na+后消除的缓慢成分组成。8. 尾电流缓慢成分的幅度随电压钳脉冲持续时间的变化表明,Na+电流与膜电导的时间依赖性成分相关。9. 考虑了缓慢衰减Na+电流的可能机制。结合Na+电导变化遵循Ca2+在细胞质中积累和去除的时间进程这一观点对结果进行了讨论。

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