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鲈鱼视网膜水平细胞和穆勒细胞中的神经胶质细胞和神经元标志物。

Glial and neuronal markers in bass retinal horizontal and Müller cells.

作者信息

Vaughan D K, Lasater E M

机构信息

Department of Physiology, University of Utah, Salt Lake City 84108.

出版信息

Brain Res. 1990 Dec 24;537(1-2):131-40. doi: 10.1016/0006-8993(90)90349-g.

Abstract

Retinal horizontal cells (HCs) are second-order neurons that integrate information from photoreceptors over large retinal areas, mediating the lateral spread of visual signals in the distal retina. The 'glial' vs. 'neuronal' nature of the HC has been widely debated. For example, carbonic anhydrase (CA), glutamine synthetase (GS), and glial fibrillary acidic protein (GFAP) are considered 'glial' markers, yet both CA and GFAP have been previously reported in HCs of the teleost retina in species-specific patterns. In contrast, the neurofilament triplet (NFT) proteins are considered 'neuronal' markers; these proteins have been immunolocalized to a mammalian HC, but are absent from teleost HCs. We have studied these cytochemical characteristics in HCs from the white bass, by immunolabeling both cryosections of intact retina and freshly isolated, identified cells attached to coverslips. We found that both HCs (neurons) and Müller cells (MCs; glia) immunolabeled with antisera to CA. Both type 1 (external) HCs and MCs immunolabeled with an antibody to vimentin. Only MCs immunolabeled with antisera to GS and GFAP. Neither HC perikarya (and their major dendrites) nor MCs immunolabeled with an antibody to the 160-kDa subunit of NFT protein. Thus, bass HCs and MCs share the presence of CA and vimentin epitopes and absence of the NFT 160-kDa epitope. Moreover, retinal cell isolation, by itself, does not affect cell-type specific immunolabeling patterns in identified cells, except for what may be lost with the finer processes of the various cells. Isolated cell studies can aid in interpreting immunolabeling patterns observed in the intact retina, especially in retinal layers where several cell types may be present.

摘要

视网膜水平细胞(HCs)是二阶神经元,它们整合来自视网膜大面积区域光感受器的信息,介导视觉信号在视网膜远端的侧向传播。HCs的“神经胶质细胞”与“神经元”性质一直存在广泛争议。例如,碳酸酐酶(CA)、谷氨酰胺合成酶(GS)和胶质纤维酸性蛋白(GFAP)被认为是“神经胶质细胞”标志物,但此前在硬骨鱼视网膜的HCs中已报道CA和GFAP均呈现物种特异性模式。相反,神经丝三联体(NFT)蛋白被认为是“神经元”标志物;这些蛋白已通过免疫定位在哺乳动物的HCs中发现,但硬骨鱼的HCs中不存在。我们通过对完整视网膜的冰冻切片以及附着在盖玻片上的新鲜分离、已鉴定细胞进行免疫标记,研究了白鲈HCs的这些细胞化学特征。我们发现HCs(神经元)和米勒细胞(MCs;神经胶质细胞)均用抗CA血清进行了免疫标记。1型(外部)HCs和MCs均用波形蛋白抗体进行了免疫标记。只有MCs用抗GS和GFAP血清进行了免疫标记。HCs的胞体(及其主要树突)和MCs均未用抗NFT蛋白160-kDa亚基的抗体进行免疫标记。因此,鲈鱼的HCs和MCs都有CA和波形蛋白表位,且都没有NFT 160-kDa表位。此外,视网膜细胞分离本身不会影响已鉴定细胞中细胞类型特异性免疫标记模式,除非各种细胞更细微的突起可能会丢失。分离细胞研究有助于解释在完整视网膜中观察到的免疫标记模式,特别是在可能存在多种细胞类型的视网膜层中。

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