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通过轴突运输和二维凝胶电泳鉴定的兔视觉中继核神经终末蛋白

Nerve terminal proteins of the rabbit visual relay nuclei identified by axonal transport and two-dimensional gel electrophoresis.

作者信息

Wagner J A, Kelly A S, Kelly R B

出版信息

Brain Res. 1979 May 18;168(1):97-117. doi: 10.1016/0006-8993(79)90130-6.

Abstract

The proteins in nerve terminals can be uniquely identified by two-dimensional gel electrophoresis of proteins labeled during synthesis in the cell body and then transported intra-axonally to the terminals. We have explored the potential of the identification procedure by comparing the proteins which are transported from the retina to the lateral geniculate nucleus (LGN) and the superior colliculus (SC) of the rabbit. We have been able to identify between 150 and 200 proteins which ate common to both LGN and SC nerve terminals, very few of which are present at significantly different concentrations in one nucleus relative to the other. The similarity between proteins sent from the retina along two neural pathways subserving different functions illustrates the subtlety of biochemical changes that must underlie physiological differences. Only a small fraction of the labeled proteins are major proteins of the relay nuclei as judged by Coomassie-staining, and some of these arise from in situ nonspecific labeling with blood-borne radioactivity, rather than by transport to the terminals. We have shown that about 5 times more proteins are transported at fast than at intermediate transport rates. More than 50% of the fast proteins turn over rapidly and are gone in 24 h. Few intermediate proteins turn over rapidly. Since only 6% of the proteins in the relay nuclei (at 36 h) could not be detected in the optic tract at that time, transsynaptic labeling by breakdown and resynthesis must be small, if it occurs at all.

摘要

通过对在细胞体中合成并随后经轴突内运输至神经末梢的蛋白质进行二维凝胶电泳,可以唯一地鉴定神经末梢中的蛋白质。我们通过比较从视网膜运输至兔外侧膝状体(LGN)和上丘(SC)的蛋白质,探索了这种鉴定方法的潜力。我们已经能够鉴定出150至200种LGN和SC神经末梢共有的蛋白质,其中相对于另一个核,在一个核中以显著不同浓度存在的蛋白质非常少。沿着两条具有不同功能的神经通路从视网膜发出的蛋白质之间的相似性,说明了作为生理差异基础的生化变化的微妙之处。通过考马斯亮蓝染色判断,只有一小部分标记蛋白质是中继核的主要蛋白质,其中一些是由血源性放射性原位非特异性标记产生的,而不是通过运输至神经末梢产生的。我们已经表明,快速运输的蛋白质数量大约是中等运输速率蛋白质的5倍。超过50%的快速运输蛋白质周转迅速,在24小时内消失。很少有中等运输速率的蛋白质周转迅速。由于在36小时时,中继核中只有6%的蛋白质在此时的视束中无法检测到,因此如果发生跨突触标记,通过分解和重新合成产生的跨突触标记一定很少。

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