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海马苔藓纤维终扣中钙离子通道激活的时间与效能

Timing and efficacy of Ca2+ channel activation in hippocampal mossy fiber boutons.

作者信息

Bischofberger Josef, Geiger Jörg R P, Jonas Peter

机构信息

Physiologisches Institut, Universität Freiburg, D-79104 Freiburg, Germany.

出版信息

J Neurosci. 2002 Dec 15;22(24):10593-602. doi: 10.1523/JNEUROSCI.22-24-10593.2002.

Abstract

The presynaptic Ca2+ signal is a key determinant of transmitter release at chemical synapses. In cortical synaptic terminals, however, little is known about the kinetic properties of the presynaptic Ca2+ channels. To investigate the timing and magnitude of the presynaptic Ca2+ inflow, we performed whole-cell patch-clamp recordings from mossy fiber boutons (MFBs) in rat hippocampus. MFBs showed large high-voltage-activated Ca(2+) currents, with a maximal amplitude of approximately 100 pA at a membrane potential of 0 mV. Both activation and deactivation were fast, with time constants in the submillisecond range at a temperature of approximately 23 degrees C. An MFB action potential (AP) applied as a voltage-clamp command evoked a transient Ca2+ current with an average amplitude of approximately 170 pA and a half-duration of 580 microsec. A prepulse to +40 mV had only minimal effects on the AP-evoked Ca2+ current, indicating that presynaptic APs open the voltage-gated Ca2+ channels very effectively. On the basis of the experimental data, we developed a kinetic model with four closed states and one open state, linked by voltage-dependent rate constants. Simulations of the Ca2+ current could reproduce the experimental data, including the large amplitude and rapid time course of the current evoked by MFB APs. Furthermore, the simulations indicate that the shape of the presynaptic AP and the gating kinetics of the Ca2+ channels are tuned to produce a maximal Ca2+ influx during a minimal period of time. The precise timing and high efficacy of Ca2+ channel activation at this cortical glutamatergic synapse may be important for synchronous transmitter release and temporal information processing.

摘要

突触前Ca2+信号是化学突触中递质释放的关键决定因素。然而,在皮质突触终末,关于突触前Ca2+通道的动力学特性却知之甚少。为了研究突触前Ca2+内流的时间和幅度,我们对大鼠海马体中的苔藓纤维终扣(MFBs)进行了全细胞膜片钳记录。MFBs表现出大的高电压激活的Ca(2+)电流,在0 mV膜电位时最大幅度约为100 pA。激活和失活都很快,在约23摄氏度的温度下时间常数在亚毫秒范围内。作为电压钳指令施加的MFB动作电位(AP)诱发了一个瞬时Ca2+电流,平均幅度约为170 pA,半持续时间为580微秒。+40 mV的预脉冲对AP诱发的Ca2+电流只有最小的影响,表明突触前AP能非常有效地打开电压门控Ca2+通道。基于实验数据,我们开发了一个具有四个关闭状态和一个开放状态的动力学模型,通过电压依赖性速率常数相连。Ca2+电流的模拟可以重现实验数据,包括MFB APs诱发电流的大幅度和快速时间进程。此外,模拟表明突触前AP的形状和Ca2+通道的门控动力学经过调整,以便在最短的时间内产生最大的Ca2+内流。在这个皮质谷氨酸能突触处Ca2+通道激活的精确时间和高效性可能对同步递质释放和时间信息处理很重要。

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