首页> 美国卫生研究院文献>Journal of Visualized Experiments : JoVE >Cut-loading: A Useful Tool for Examining the Extent of Gap Junction Tracer Coupling Between Retinal Neurons
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Cut-loading: A Useful Tool for Examining the Extent of Gap Junction Tracer Coupling Between Retinal Neurons

机译:切负荷:检查视网膜神经元之间的间隙连接示踪剂耦合程度的有用工具

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摘要

In addition to chemical synaptic transmission, neurons that are connected by gap junctions can also communicate rapidly via electrical synaptic transmission. Increasing evidence indicates that gap junctions not only permit electrical current flow and synchronous activity between interconnected or coupled cells, but that the strength or effectiveness of electrical communication between coupled cells can be modulated to a great extent1,2. In addition, the large internal diameter (~1.2 nm) of many gap junction channels permits not only electric current flow, but also the diffusion of intracellular signaling molecules and small metabolites between interconnected cells, so that gap junctions may also mediate metabolic and chemical communication. The strength of gap junctional communication between neurons and its modulation by neurotransmitters and other factors can be studied by simultaneously electrically recording from coupled cells and by determining the extent of diffusion of tracer molecules, which are gap junction permeable, but not membrane permeable, following iontophoretic injection into single cells. However, these procedures can be extremely difficult to perform on neurons with small somata in intact neural tissue.Numerous studies on electrical synapses and the modulation of electrical communication have been conducted in the vertebrate retina, since each of the five retinal neuron types is electrically connected by gap junctions3,4. Increasing evidence has shown that the circadian (24-hour) clock in the retina and changes in light stimulation regulate gap junction coupling3-8. For example, recent work has demonstrated that the retinal circadian clock decreases gap junction coupling between rod and cone photoreceptor cells during the day by increasing dopamine D2 receptor activation, and dramatically increases rod-cone coupling at night by reducing D2 receptor activation7,8. However, not only are these studies extremely difficult to perform on neurons with small somata in intact neural retinal tissue, but it can be difficult to adequately control the illumination conditions during the electrophysiological study of single retinal neurons to avoid light-induced changes in gap junction conductance.Here, we present a straightforward method of determining the extent of gap junction tracer coupling between retinal neurons under different illumination conditions and at different times of the day and night. This cut-loading technique is a modification of scrape loading9-12, which is based on dye loading and diffusion through open gap junction channels. Scrape loading works well in cultured cells, but not in thick slices such as intact retinas. The cut-loading technique has been used to study photoreceptor coupling in intact fish and mammalian retinas7, 8,13, and can be used to study coupling between other retinal neurons, as described here.
机译:除化学突触传递外,通过间隙连接连接的神经元还可以通过电突触传递快速通讯。越来越多的证据表明,间隙连接不仅允许电流流动和相互连接或耦合的单元之间的同步活动,而且可以在很大程度上调节耦合单元之间的电通信的强度或有效性 1,2 。另外,许多间隙连接通道的大内径(〜1.2 nm)不仅允许电流流动,而且还允许细胞内信号分子和相互连接的细胞之间的小代谢物扩散,因此间隙连接还可以介导代谢和化学通讯。可以通过同时从耦合细胞中进行电记录并确定示踪剂分子的扩散程度来研究神经元之间的间隙连接通讯的强度及其受神经递质和其他因素的调节,这些示踪剂在离子电渗疗法之后是间隙连接可透过的,但膜不可透过的注入单细胞。然而,在完整的神经组织中具有小躯体的神经元上执行这些程序可能非常困难。由于五种视网膜神经元中的每一种都是电连接的,因此在脊椎动物视网膜中进行了许多有关电突触和电通信调节的研究。通过间隙连接 3,4 。越来越多的证据表明,视网膜中的昼夜节律(24小时)和光刺激的变化调节间隙连接耦合 3-8 。例如,最近的研究表明,昼夜节律生物钟通过增加多巴胺D2受体的活化作用来减少杆与视锥感光细胞之间的间隙连接偶联,并在夜间通过降低D2受体的活化来显着增加杆-锥结合 7 ,8 。然而,这些研究不仅在完整的视网膜神经组织中对具有小躯体的神经元进行极度困难,而且在单个视网膜神经元的电生理研究过程中,要避免光诱导间隙连接的变化,可能很难充分控制光照条件。在此,我们提出了一种简单的方法来确定在不同光照条件下以及白天和晚上的不同时间在视网膜神经元之间的间隙连接示踪剂偶联的程度。这种切割加载技术是刮擦加载 9-12 的一种改进,它基于染料加载和通过开放间隙连接通道的扩散。刮擦加载在培养的细胞中效果很好,但在完整的视网膜等较厚的切片中效果不佳。如本文所述,切负荷技术已被用于研究完整鱼类和哺乳动物视网膜 7,8,13 中的感光细胞偶联,并可用于研究其他视网膜神经元之间的偶联。

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