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快速中枢突触处递质释放速率的细胞内钙依赖性。

Intracellular calcium dependence of transmitter release rates at a fast central synapse.

作者信息

Schneggenburger R, Neher E

机构信息

Abteilung Membranbiophysik, Max-Planck-Institut für biophysikalische Chemie, Göttingen, Germany.

出版信息

Nature. 2000 Aug 24;406(6798):889-93. doi: 10.1038/35022702.

Abstract

Calcium-triggered fusion of synaptic vesicles and neurotransmitter release are fundamental signalling steps in the central nervous system. It is generally assumed that fast transmitter release is triggered by elevations in intracellular calcium concentration ([Ca2+]i) to at least 100 microM near the sites of vesicle fusion. For synapses in the central nervous system, however, there are no experimental estimates of this local [Ca2+]i signal. Here we show, by using calcium ion uncaging in the large synaptic terminals of the calyx of Held, that step-like elevations to only 10 microM [Ca2+]i induce fast transmitter release, which depletes around 80% of a pool of available vesicles in less than 3 ms. Kinetic analysis of transmitter release rates after [Ca2+]i steps revealed the rate constants for calcium binding and vesicle fusion. These show that transient (around 0.5 ms) local elevations of [Ca2+]i to peak values as low as 25 microM can account for transmitter release during single presynaptic action potentials. The calcium sensors for vesicle fusion are far from saturation at normal release probability. This non-saturation, and the high intracellular calcium cooperativity in triggering vesicle fusion, make fast synaptic transmission very sensitive to modulation by changes in local [Ca2+]i.

摘要

钙触发的突触小泡融合和神经递质释放是中枢神经系统中的基本信号传导步骤。一般认为,快速递质释放是由靠近小泡融合部位的细胞内钙浓度([Ca2+]i)升高至至少100微摩尔引发的。然而,对于中枢神经系统中的突触,尚无对这种局部[Ca2+]i信号的实验估计。在此,我们通过在Held壶腹的大型突触终末中使用钙离子光解技术表明,[Ca2+]i仅阶梯式升高至10微摩尔即可诱导快速递质释放,在不到3毫秒的时间内耗尽约80%的可用小泡池。对[Ca2+]i阶梯后递质释放速率的动力学分析揭示了钙结合和小泡融合的速率常数。这些结果表明,[Ca2+]i短暂(约0.5毫秒)局部升高至低至25微摩尔的峰值即可解释单个突触前动作电位期间的递质释放。在正常释放概率下,用于小泡融合的钙传感器远未饱和。这种不饱和状态以及触发小泡融合时的高细胞内钙协同作用,使得快速突触传递对局部[Ca2+]i变化的调节非常敏感。

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