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首页> 外文期刊>The Journal of Neuroscience: The Official Journal of the Society for Neuroscience >A mechanism intrinsic to the vesicle fusion machinery determines fast and slow transmitter release at a large CNS synapse.
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A mechanism intrinsic to the vesicle fusion machinery determines fast and slow transmitter release at a large CNS synapse.

机译:囊泡融合机制固有的机制决定了大型CNS突触中快速和缓慢的递质释放。

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摘要

Heterogeneity of release probability p between vesicles in the readily releasable pool (RRP) is expected to strongly influence the kinetics of depression at synapses, but the underlying mechanism(s) are not well understood. To test whether differences in the intrinsic Ca2+ sensitivity of vesicle fusion might cause heterogeneity of p, we made presynaptic Ca2+-uncaging measurements at the calyx of Held and analyzed the time course of transmitter release by EPSC deconvolution. Ca2+ uncaging, which produced spatially homogeneous elevations of [Ca2+]i, evoked a fast and a slow component of release over a wide range of [Ca2+]i, showing that mechanism(s) intrinsic to the vesicle fusion machinery cause fast and slow transmitter release. Surprisingly, the number of vesicles released in the fast component increased with Ca2+-uncaging stimuli of larger amplitudes, a finding that was most obvious below approximately 10 microM [Ca2+]i and that we call "submaximal release" of fast-releasable vesicles. During trains of action potential-like presynaptic depolarizations, submaximal release was also observed as an increase in the cumulative fast release at enhanced release probabilities. A model that assumes two separate subpools of RRP vesicles with different intrinsic Ca2+ sensitivities predicted the observed Ca2+ dependencies of fast and slow transmitter release but could not fully account for submaximal release. Thus, fast and slow transmitter release in response to prolonged [Ca2+]i elevations is caused by intrinsic differences between RRP vesicles, and an "a posteriori" reduction of the Ca2+ sensitivity of vesicle fusion after the onset of the stimulus might cause submaximal release of fast-releasable vesicles and contribute to short-term synaptic depression.
机译:易释放池(RRP)中的小泡之间释放概率p的异质性预计会强烈影响突触中抑郁的动力学,但潜在的机制尚不清楚。为了测试囊泡融合的内在Ca2 +敏感性差异是否会导致p的异质性,我们在Held花萼中进行了突触前Ca2 +解囊测量,并通过EPSC反卷积分析了递质释放的时间过程。 Ca2 +解封,产生[Ca2 +] i在空间上均一的升高,引起了[Ca2 +] i的快速释放和缓慢释放,表明囊泡融合机制固有的机制导致了快速递质和缓慢递质释放。出乎意料的是,在快速成分中释放的囊泡数量随着更大幅度的Ca2 +解封刺激而增加,这一发现在约10 microM [Ca2 +] i以下最为明显,我们称这种快释囊泡为“亚最大释放”。在一系列类似动作电位的突触前去极化过程中,还观察到亚最大释放是在增强释放概率时累积快速释放的增加。假设两个具有不同固有Ca2 +敏感性的RRP囊泡的独立子池组成的模型预测了观察到的Ca2 +依赖于快速和缓慢的递质释放,但不能完全解释次最大释放。因此,RRP囊泡之间的固有差异会导致响应[Ca2 +] i升高而导致的快速和缓慢递质释放,并且刺激发生后囊泡融合的Ca2 +敏感性的“后验”降低可能导致最大程度的释放。快速释放的囊泡,并导致短期的突触抑制。

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