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Developmental Transformation of the Release Modality at the Calyx of Held Synapse

机译:举行突触花萼释放模式的发展转变。

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摘要

Ca2+ influx through voltage-gated Ca2+ channels (VGCCs) into nerve terminals triggers vesicular fusion and neurotransmitter release. However, it is unknown whether the coupling between VGCCs and synaptic vesicles (SVs) is developmentally regulated. By paired patch-clamp recordings from the mouse calyx of Held synapse, we show here that injection of a Ca2+ buffer with slow binding kinetics (EGTA; 10 mm) potently attenuated transmitter release in young terminals [postnatal day 8 (P8)-P12] but produced little effect in older ones (P16-P18), suggesting that SVs in young synapses are loosely coupled to VGCCs, but the coupling tightens spatially during maturation. Using voltage paradigms that specifically recruit different numbers of VGCCs without changing the driving force for Ca2+, we found that the Ca2+ cooperativity (m), estimated from graded presynaptic Ca2+ currents and transmitter release, was much higher in P8-P12 synapses (m = 4.8-5.5) than that in P16-P18 synapses (m = 2.8-3.0; 1 mm [Ca2+]o), implying that the number of VGCCs or Ca2+ domains required for release of single SVs decreases with maturation. The m value remained significantly different between two age groups at 35°C or in 2 mm [Ca2+]o and was independent of postsynaptic receptor desensitization. We demonstrated that release from P8-P12 terminals involved both N- and P/Q-type VGCCs, but P/Q-type-associated release sites specifically displayed low m values. These results suggest a developmental transformation of the release modality from “microdomain,” involving cooperative action of many loosely coupled N- and P/Q-type VGCCs, to “nanodomain,” in which opening of fewer tightly coupled P/Q-type VGCCs effectively induce a fusion event. Spatial tightening improves the release efficiency and is likely a critical step for the development of high-fidelity neurotransmission in this and other central synapses.
机译:Ca 2 + 通过电压门控的Ca 2 + 通道(VGCC)流入神经末梢,触发囊泡融合和神经递质释放。但是,尚不清楚VGCC和突触囊泡(SV)之间的耦合是否受到发育调控。通过对来自Held突触的小鼠花萼的成对钳夹录音,我们在这里表明,以缓慢的结合动力学(EGTA; 10 mm)注入Ca 2 + 缓冲液可有​​效减弱年轻末端的递质释放[出生后第8天(P8)-P12],但对年长者(P16-P18)影响不大,这表明年轻突触中的SV与VGCC松散耦合,但在成熟过程中这种耦合在空间上变紧。使用专门募集不同数量的VGCC而不改变Ca 2 + 的驱动力的电压范例,我们发现,Ca 2 + 的协同性(m)是从分级突触前估计的Ca 2 + 电流和变送器释放,在P8-P12突触中(m = 4.8-5.5)比在P16-P18突触中(m = 2.8-3.0; 1 mm [Ca 2 + ] o),这意味着释放单个SV所需的VGCC或Ca 2 + 域的数量会随着成熟而减少。两个年龄组在35°C或2 mm [Ca 2 + ] o中的m值仍然存在显着差异,并且与突触后受体脱敏无关。我们证明了从P8-P12终端释放涉及N型和P / Q型VGCC,但是P / Q型相关的释放位点特别显示了低m值。这些结果表明释放方式从“微结构域”的发展转变,涉及许多松散耦合的N型和P / Q型VGCC的协同作用,向“纳米结构域”释放了更少的紧密耦合的P / Q型VGCC。有效地引发融合事件。空间收紧可提高释放效率,并且可能是在此突触和其他中央突触中发展高保真神经传递的关键步骤。

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