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利用细胞类型特异性单克隆抗体鉴定和表征大鼠视网膜培养物中积累γ-氨基丁酸(GABA)的细胞类型。

Identification and characterisation of cell types accumulating GABA in rat retinal cultures using cell type specific monoclonal antibodies.

作者信息

Akagawa K, Barnstable C J

出版信息

Brain Res. 1987 Apr 7;408(1-2):154-62. doi: 10.1016/0006-8993(87)90367-2.

Abstract

Monolayer and reaggregate cultures have been established from neonatal rat retina. After 7 days in culture, 60 nM [3H]gamma-aminobutyric acid (GABA) was used to identify cells with a high affinity uptake mechanism for GABA. Approximately 80% of the process-bearing cells were found to be labelled. These cells were identified as amacrine cells by double-labelling experiments combining [3H]GABA uptake with immunocytochemical labelling with monoclonal antibody HPC-1 which in retina is specific for amacrine cells. The ability of cultures to synthesize GABA from glutamate was investigated at various times. Little synthesis was observed during the first few days in culture. This lag was followed by an increase in the amount of synthesis until 3 weeks of culture. When clumps and reaggregate cultures of retinal cells were examined by [3H]GABA uptake, a time-dependent redistribution of labelled cells was observed. After 20 h in culture, GABA-positive cells were distributed over the whole cell mass. Over the next few days, the labelled cells became more common on the outer edge of the aggregates and less common in inner regions. By 7 days of culture, no labelled cell bodies were found on the inside of the aggregates, although such cells could be labelled by [3H]D-aspartate. The results provide positive identification of a subclass of retinal cells in culture, and show that at least one aspect of retinal histogenesis is not dependent upon extra-retinal tissues or the position imposed by the temporal order of retinal cell birth.

摘要

已从新生大鼠视网膜建立了单层培养物和重新聚集培养物。培养7天后,使用60 nM [3H]γ-氨基丁酸(GABA)来鉴定具有高亲和力摄取GABA机制的细胞。发现约80%的有突起细胞被标记。通过将[3H]GABA摄取与用单克隆抗体HPC-1进行免疫细胞化学标记相结合的双重标记实验,这些细胞被鉴定为无长突细胞,该抗体在视网膜中对无长突细胞具有特异性。在不同时间研究了培养物从谷氨酸合成GABA的能力。在培养的最初几天观察到很少的合成。这种延迟之后是合成量增加,直到培养3周。当通过[3H]GABA摄取检查视网膜细胞的团块和重新聚集培养物时,观察到标记细胞的时间依赖性重新分布。培养20小时后,GABA阳性细胞分布在整个细胞团中。在接下来的几天里,标记细胞在聚集体的外边缘变得更常见,而在内部区域则不那么常见。到培养7天时,在聚集体内部未发现标记的细胞体,尽管此类细胞可以被[3H]D-天冬氨酸标记。这些结果提供了对培养中视网膜细胞一个亚类的阳性鉴定,并表明视网膜组织发生的至少一个方面不依赖于视网膜外组织或视网膜细胞出生时间顺序所施加的位置。

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