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微安培分辨率测定视网膜双极细胞中预峰颤抖和快速释放诱发相。

Amperometric resolution of a prespike stammer and evoked phases of fast release from retinal bipolar cells.

机构信息

Yale University School of Medicine, Department of Cellular and Molecular Physiology, New Haven, Connecticut 06520, USA.

出版信息

J Neurosci. 2013 May 8;33(19):8144-58. doi: 10.1523/JNEUROSCI.5062-12.2013.

Abstract

The neurotransmitter glutamate is used by most neurons in the brain to activate a multitude of different types of glutamate receptors and transporters involved in fast and relatively slower signaling. Synaptic ribbons are large presynaptic structures found in neurons involved in vision, balance, and hearing, which use a large number of glutamate-filled synaptic vesicles to meet their signaling demands. To directly measure synaptic vesicle release events, the ribbon-type presynaptic terminals of goldfish retinal bipolar cells were coaxed to release a false transmitter that could be monitored with amperometry by placing the carbon fiber directly on the larger synaptic terminal. Spontaneous secretion events formed a unimodal charge distribution, but single spike properties were heterogeneous. Larger events rose exponentially without interruption (τ ∼ 30 μs), and smaller events exhibited a stammer in their rising phase that is interpreted as a brief pause in pore dilation, a characteristic commonly associated with large dense core granule fusion pores. These events were entirely Ca(2+)-dependent. Holding the cells at -60 mV halted spontaneous release; and when the voltage was stepped to >-40 mV, secretion ensued. When stepping the voltage to 0 mV, novel kinetic phases of vesicle recruitment were revealed. Approximately 14 vesicles were released per ribbon in two kinetic phases with time constants of 1.5 and 16 ms, which are proposed to represent different primed states within the population of docked vesicles.

摘要

神经递质谷氨酸被大脑中的大多数神经元用来激活多种不同类型的谷氨酸受体和转运体,这些受体和转运体参与快速和相对较慢的信号传递。突触小核糖体能在视觉、平衡和听觉中参与神经元中被发现,它使用大量充满谷氨酸的突触小泡来满足其信号传递的需求。为了直接测量突触小泡释放事件,将金鱼视网膜双极细胞的带状型突触前末梢诱导向外释放一种虚假递质,通过将碳纤维直接放在较大的突触前末梢上,用安培法可以监测到这种递质。自发分泌事件形成了单峰电荷分布,但单峰特性是不均匀的。较大的事件呈指数上升,没有中断(τ∼30μs),而较小的事件在上升阶段出现口吃,这被解释为孔扩张的短暂停顿,这是与大而密的核心颗粒融合孔相关的特征。这些事件完全依赖 Ca2+。将细胞保持在-60 mV 可阻止自发释放;当电压升高到>-40 mV 时,分泌就会发生。当电压升高到 0 mV 时,会揭示出囊泡募集的新动力学阶段。每个突触小核糖体能释放约 14 个囊泡,具有 1.5 和 16 ms 的时间常数,这两个时间常数被认为代表了停靠囊泡群体中不同的引发状态。

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