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两种无长突细胞通路神经节细胞在狨猴视网膜中的突触输入。

Synaptic inputs to two types of koniocellular pathway ganglion cells in marmoset retina.

机构信息

Department of Ophthalmology, Save Sight Institute, University of Sydney, Australia.

出版信息

J Comp Neurol. 2011 Aug 1;519(11):2135-53. doi: 10.1002/cne.22586.

DOI:10.1002/cne.22586
PMID:21452222
Abstract

The retinal connectivity of the diverse group of cells contributing to koniocellular visual pathways (widefield ganglion cells) is largely unexplored. Here we examined the synaptic inputs onto two koniocellular-projecting ganglion cell types named large sparse and broad thorny cells. Ganglion cells were labeled by retrograde tracer injections targeted to koniocellular layer K3 in the lateral geniculate nucleus in marmosets (Callithrix jacchus) and subsequently photofilled. Retinal preparations were processed with antibodies against the C-terminal binding protein 2, the AMPA receptor subunit GluR4, and against CD15 to identify bipolar (excitatory) and/or antibodies against gephyrin to identify amacrine (inhibitory) input. Large sparse cells are narrowly stratified close to the ganglion cell layer. Broad thorny ganglion cells are broadly stratified in the center of the inner plexiform layer. Bipolar input to large sparse cells derives from DB6 and maybe other ON bipolar types, whereas that to broad thorny cells derives from ON and OFF bipolar cell types. The total number of putative synapses on broad thorny cells is higher than the number on large sparse cells but the density of inputs (between 2 and 5 synapses per 100 μm(2) dendritic area) is similar for the two cell types, indicating that the larger number of synapses on broad thorny cells is attributable to the larger membrane surface area of this cell type. Synaptic input density is comparable to previous values for midget-parvocellular and parasol-magnocellular pathway cells. This suggests functional differences between koniocellular, parvocellular, and magnocellular pathways do not arise from variation in synaptic input densities.

摘要

对构成 koniocellular 视觉通路(宽场神经节细胞)的不同细胞群体的视网膜连接的研究还在很大程度上没有得到探索。在这里,我们研究了两种 koniocellular 投射神经节细胞类型(大稀疏细胞和宽棘细胞)的突触输入。通过向外侧膝状体核的 koniocellular 层 K3 靶向逆行示踪剂注射标记神经节细胞,随后用光填充。用针对 C 端结合蛋白 2、AMPA 受体亚基 GluR4 和针对 CD15 的抗体处理视网膜标本,以识别双极(兴奋性)和/或针对 gephyrin 的抗体,以识别无长突细胞(抑制性)输入。大稀疏细胞在靠近神经节细胞层的地方被细分为狭窄层。宽棘神经节细胞在神经节细胞层的中心被广泛分层。大稀疏细胞的双极输入来自 DB6 和可能的其他 ON 双极细胞类型,而宽棘细胞的双极输入来自 ON 和 OFF 双极细胞类型。宽棘细胞上的总突触数多于大稀疏细胞,但输入密度(每 100μm² 树突面积 2 到 5 个突触之间)对于两种细胞类型相似,这表明宽棘细胞上更多的突触归因于这种细胞类型更大的膜表面积。突触输入密度与先前的小细胞-小细胞和伞细胞-大细胞通路细胞的值相当。这表明 koniocellular、parvocellular 和 magnocellular 通路之间的功能差异不是由于突触输入密度的变化引起的。

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