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High-Resolution Optical Imaging of Zebrafish Larval Ribbon Synapse Protein RIBEYE RIM2 and CaV 1.4 by Stimulation Emission Depletion Microscopy

机译:通过刺激发射耗尽显微镜显微镜显微镜显微镜显微镜显微镜斑马鱼幼虫带突触蛋白ribaphyRIM2和Cav 1.4的高分辨率光学成像

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摘要

The synaptic ribbon is a unique presynaptic structure with an intricate morphology in photoreceptors. Because of the resolution limit in conventional fluorescence microscopy, investigating ribbon protein locations has been challenging, especially in the early development stages of model animals. Here, we used stimulated emission depletion microscopy, a super-resolution imaging technique, to look at retina sections in 4 days post-fertilization (dpf) zebrafish. We observed that in photoreceptor cells, RIBEYE and RIM2 are expressed along the synaptic ribbon, with RIM2 consistently located inside of the horseshoe-shaped synaptic ribbon structure with RIBEYE located on the outside. The L-type calcium channel subunit, CACNA1F, exhibited small spot-like staining beneath the RIM2 and RIBEYE structures. Using morpholino antisense oligonucleotides to knock down RIBEYE expression, we observed fewer and shorter ribbons in the photoreceptor outer plexiform layers of 4 dpf fish retina as well as a reduction in RIM2 expression. The clustering of CACNA1F in these blind fish was no longer observed, but instead showed a diffuse expression in the photoreceptor terminal.
机译:突触带是一种独特的突触前结构,在感光器中具有复杂的形态。由于常规荧光显微镜的分辨率限制,研究带状蛋白的位置一直具有挑战性,尤其是在模型动物的早期发育阶段。在这里,我们使用刺激发射耗竭显微镜(一种超分辨率成像技术)在受精(dpf)斑马鱼后4天内观察视网膜切片。我们观察到在感光细胞中,RIBEYE和RIM2沿突触带表达,RIM2始终位于马蹄形突触带结构的内部,而RIBEYE位于外部。 L型钙通道亚基CACNA1F在RIM2和RIBEYE结构下显示出小斑点状染色。使用吗啉代反义寡核苷酸敲低RIBEYE表达,我们观察到4 dpf鱼视网膜的感光细胞外丛状层中的带越来越少,并且RIM2表达降低。在这些盲鱼中不再观察到CACNA1F的聚集,而是在感光末端表达了弥散性表达。

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