Mills S L, Massey S C
Department of Ophthalmology and Visual Science, University of Texas at Houston--Health Science Center, 77030, USA.
Vis Neurosci. 1998 Jul-Aug;15(4):765-77. doi: 10.1017/s0952523898154159.
Observation of the spread of biotinylated or fluorescent tracers following injection into a single cell has become one of the most common methods of demonstrating the presence of gap junctions. Nevertheless, many of the fundamental features of tracer movement through gap junctions are still poorly understood. These include the relative roles of diffusion and iontophoretic current, and under what conditions the size of the stained mosaic will increase, asymptote, or decline. Additionally, the effect of variations in amount of tracer introduced, as produced by variation in electrode resistance following cell penetration, is not obvious. To examine these questions, Neurobiotin was microinjected into the two types of horizontal cell of the rabbit retina and visualized with streptavidin-Cy3. Images were digitally captured using a confocal microscope. The spatial distribution of Neurobiotin across the patches of coupled cells was measured. Adequate fits to the data were obtained by fitting to a model with terms for diffusion and amount of tracer injected. Results indicated that passive diffusion is the major source of tracer movement through gap junctions, whereas iontophoretic current played no role over the range tested. Fluorescent visualization, although slightly less sensitive than peroxidase reactions, produced staining intensities with a more useful dynamic range. The rate constants for movement of Neurobiotin between A-type horizontal cells was about ten times greater than that for B-type horizontal cells. Although direct extrapolation to ion conductances cannot be assumed, tracer movement can be used to give an estimate of relative coupling rates across cell types, retinal location, or modulation conditions in intact tissue.
观察生物素化或荧光示踪剂在注射到单个细胞后的扩散情况,已成为证明缝隙连接存在的最常用方法之一。然而,示踪剂通过缝隙连接移动的许多基本特征仍知之甚少。这些特征包括扩散和离子电泳电流的相对作用,以及在何种条件下染色镶嵌区域的大小会增加、达到渐近值或减小。此外,细胞穿透后电极电阻变化所导致的示踪剂引入量变化的影响并不明显。为了研究这些问题,将神经生物素显微注射到兔视网膜的两种水平细胞中,并用链霉亲和素 - Cy3进行可视化。使用共聚焦显微镜对图像进行数字采集。测量了神经生物素在耦合细胞斑块中的空间分布。通过拟合一个包含扩散和注射示踪剂数量项的模型,获得了与数据的充分拟合。结果表明,被动扩散是示踪剂通过缝隙连接移动的主要来源,而在测试范围内离子电泳电流不起作用。荧光可视化虽然比过氧化物酶反应稍不敏感,但产生的染色强度具有更有用的动态范围。神经生物素在A型水平细胞之间移动的速率常数大约是B型水平细胞的十倍。虽然不能直接推断离子电导,但示踪剂移动可用于估计完整组织中不同细胞类型、视网膜位置或调节条件下的相对耦合速率。