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首页> 外文期刊>The Journal of Physiology >Intraterminal Ca2+ concentration and asynchronous transmitter release at single GABAergic boutons in rat collicular cultures.
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Intraterminal Ca2+ concentration and asynchronous transmitter release at single GABAergic boutons in rat collicular cultures.

机译:在大鼠胶质细胞培养物中,单个GABA能弹道内的末端内Ca2 +浓度和异步变送器释放。

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摘要

Neurotransmitter release in response to a single action potential has a precise time course. A significant fraction of the releasable vesicles is exocytosed synchronously, within a few milliseconds after the arrival of an action potential. If repeatedly activated, stimulus-locked phasic synchronous release declines, but synaptic transmission can be maintained through tonic asynchronous transmitter release. The desynchronisation of release during repetitive activation is generally attributed to a build-up of intraterminal Ca2+ concentration. However, the precise relationship between presynaptic Ca2+ level and asynchronous release rate at small central synapses has remained unclear. Here we characterise this relationship for single GABAergic terminals in rat collicular cultures. In the presence of tetrodotoxin, inhibitory postsynaptic currents (IPSCs) and presynaptic Ca2+ transients were recorded in response to direct presynaptic depolarisation of individual boutons. Repetitive stimulation indeed resulted in a shift from phasic to asynchronous neurotransmitter release. A clear dominance of the asynchronous release mode was observed after 10 pulses. The steady-state asynchronous release rate showed a third-power dependency on the presynaptic Ca2+ concentration, which is similar to that of evoked release. The Ca2+ sensor for asynchronous release exhibited a high affinity for Ca2+ and was far from saturation. These properties of the Ca2+ sensor should make the asynchronous release very sensitive to any modification of presynaptic Ca2+ concentration, including those resulting from changes in presynaptic activity patterns. Thus, asynchronous release represents a powerful but delicately regulated mechanism that ensures the maintenance of appropriate inhibition when the readily releasable pool of vesicles is depleted.
机译:响应单个动作电位的神经递质释放具有精确的时间过程。在动作电位到达后的几毫秒内,大部分可释放的囊泡被同步地胞吐。如果反复激活,则刺激锁定的相位同步释放会下降,但是可以通过补音异步发射器的释放来维持突触传递。重复激活过程中释放的不同步通常归因于末端内Ca2 +浓度的增加。然而,在小的中央突触中,突触前Ca 2+水平与异步释放速率之间的确切关系仍不清楚。在这里,我们表征大鼠胶体培养物中单个GABA能终末的这种关系。在存在河豚毒素的情况下,记录到抑制响应于单个按钮的直接突触前去极化,抑制突触后电流(IPSC)和突触前Ca2 +瞬变。重复刺激确实导致了从阶段性释放到异步性神经递质释放的转变。 10个脉冲后,观察到异步释放模式的明显优势。稳态异步释放速率显示出对突触前Ca2 +浓度的三次幂依赖性,这与诱发释放相似。用于异步释放的Ca2 +传感器对Ca2 +具有很高的亲和力,并且远未达到饱和状态。 Ca2 +传感器的这些特性应使异步释放对突触前Ca2 +浓度的任何改变非常敏感,包括那些由突触前活动模式变化引起的改变。因此,异步释放代表了一种强大但微妙的调节机制,当易释放的囊泡耗尽时,该机制可确保维持适当的抑制作用。

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