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哺乳动物视网膜中谷氨酸受体基因的表达:GluR1至GluR7 mRNA的定位

Expression of glutamate receptor genes in the mammalian retina: the localization of GluR1 through GluR7 mRNAs.

作者信息

Hamassaki-Britto D E, Hermans-Borgmeyer I, Heinemann S, Hughes T E

机构信息

Department of Neurosciences, University of California, San Diego, La Jolla 92093-0608.

出版信息

J Neurosci. 1993 May;13(5):1888-98. doi: 10.1523/JNEUROSCI.13-05-01888.1993.

Abstract

Seven distinct cDNAs encoding functional subunits of the AMPA/kainate-type glutamate receptors have been recently cloned. This in situ hybridization study was done to determine which subunits are expressed in the retina and, where possible, which neurons express them. Hybridization of 35S-UTP-labeled cRNA probes with transverse sections revealed that mRNAs for all seven receptor subunits (GluR1-GluR7) are expressed in both cat and rat retinas. GluR1 and GluR2 produced labeling over the entire inner nuclear layer (INL) and ganglion cell layer (GCL). GluR3-GluR7 have more limited distributions, indicative of expression by only a subset of neurons. All of the subunits are expressed by the cells at the inner edge of the INL, where amacrine cells reside, yet the layers with the horizontal, bipolar, and ganglion cells contain different subsets of subunits. These findings suggest that these glutamate receptor subunits are employed at many of the retinal synapses, including the photoreceptor input to the outer plexiform layer and the bipolar cell's contacts with the processes at the INL. It is also possible that some glial cells in the INL express some of the subunits. Since different combinations of GluR1-GluR3 have been shown to play an important role in the calcium permeability in response to glutamate, we investigated whether single cells coexpressed those subunits. By hybridizing adjacent semithin (1 micron) sections of the cat retina with probes for GluR1-GluR3, it was possible to observe coexpression of all three subunits, or of pairs of these subunits, in cells within the INL and GCL.

摘要

最近已克隆出七种编码AMPA/海人藻酸型谷氨酸受体功能亚基的不同cDNA。进行这项原位杂交研究是为了确定哪些亚基在视网膜中表达,以及在可能的情况下,哪些神经元表达这些亚基。用35S-UTP标记的cRNA探针与横切片杂交显示,所有七种受体亚基(GluR1-GluR7)的mRNA在猫和大鼠视网膜中均有表达。GluR1和GluR2在整个内核层(INL)和神经节细胞层(GCL)产生标记。GluR3-GluR7的分布更为局限,表明仅由一部分神经元表达。所有亚基均由INL内边缘的细胞表达,此处为无长突细胞所在位置,然而水平细胞、双极细胞和神经节细胞所在层含有不同的亚基子集。这些发现表明,这些谷氨酸受体亚基在许多视网膜突触中发挥作用,包括光感受器向外网状层的输入以及双极细胞与INL处突起的接触。INL中的一些神经胶质细胞也有可能表达某些亚基。由于已表明GluR1-GluR3的不同组合在对谷氨酸的钙通透性中起重要作用,我们研究了单个细胞是否共表达这些亚基。通过用针对GluR1-GluR3的探针杂交猫视网膜相邻的半薄(1微米)切片,有可能观察到INL和GCL内细胞中所有三个亚基或这些亚基对的共表达。

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