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电鳐电动力系统的发育:电器官组织发育调控的神经营养活性

Torpedo electromotor system development: developmentally regulated neuronotrophic activities of electric organ tissue.

作者信息

Richardson G P, Rinschen B, Fox G Q

出版信息

J Comp Neurol. 1985 Jan 15;231(3):339-52. doi: 10.1002/cne.902310305.

Abstract

Explant cultures of electric lobe from 45-60 mm stage Torpedo embryos and both ganglionic and dissociated cell cultures prepared from 8-day chick ciliary ganglia have been used to determine whether the electric organs of Torpedo marmorata contain developmentally regulated neuronotrophic activity. Electric lobe explants were evaluated by measuring their neurone density, choline acetyltransferase (CAT0, and low salt, Triton X-100-soluble protein contents. Addition of soluble extracts prepared from the electric organs of late stage embryos (85-105 mm) to standard medium results in the maintenance of nearly theoretical neurone densities in electric lobe explants during a 7-day culture period. Soluble electric organ extracts from early embryonic stages (42-59 mm) do not increase neurone density relative to control cultures but cause an elevation in the CAT content of the explants over control values. On the basis of this analysis it is concluded (1) that late embryonic stage and adult electric organs contain neuronotrophic activity that allows electromotor neurones to survive in vitro and (2) that activity increases rapidly in the electric organs between the 59 nd 72 mm stages of development at a time when rapid increases in postsynaptic membrane markers in the electric organs occur and when peripheral synaptogenesis begins. The activity of late stage embryonic electric organs is heat stable and lost on dialysis. Using ciliary ganglion explants and evaluating both the initial fibre outgrowth and the CAT content after 4 days in vitro, trophic activity is found to be maximal at early embryonic stages (45-55 mm) and to decline thereafter. It is shown that the decline in activity is not due to an increase in toxicity. Using established dissociated ganglionic cell survival assays the specific activity of neuronotrophic factors allowing survival is constant between the 45 and 73 mm stages in the electric organs and then rapidly declines, but activity per electric organ increases rapidly between the 45 and 73 mm stages and then remains at a constant level. The use of poly-dl-ornithine substrates coated with heart-conditioned medium for the cell survival assay results in up to tenfold increase in the trophic titre of the electric organ extracts. The neuronotrophic activity supporting survival of ciliary motorneurones present in embryonic electric organs is heat labile and retained on dialysis. It is concluded that developing electric organs contain at least two neuronotrophic factors that have different properties and are differently regulated. Both factors may contribute during development to bringing naturally occurring electromotor neurone cell death to an end.

摘要

已利用电鳐胚胎45 - 60毫米阶段的电叶外植体培养物,以及由8日龄鸡睫状神经节制备的神经节细胞培养物和分散细胞培养物,来确定斑纹电鳐的电器官是否含有发育调控的神经营养活性。通过测量电叶外植体的神经元密度、胆碱乙酰转移酶(CAT)以及低盐、Triton X - 100可溶性蛋白含量来评估电叶外植体。向标准培养基中添加晚期胚胎(85 - 105毫米)电器官制备的可溶性提取物,可使电叶外植体在7天培养期内维持接近理论值的神经元密度。早期胚胎阶段(42 - 59毫米)的电器官可溶性提取物相对于对照培养物不会增加神经元密度,但会使外植体的CAT含量高于对照值。基于此分析得出以下结论:(1)晚期胚胎阶段和成年电器官含有神经营养活性,可使电运动神经元在体外存活;(2)在发育的59至72毫米阶段之间,当电器官中突触后膜标记物迅速增加且外周突触形成开始时,神经营养活性在电器官中迅速增加。晚期胚胎电器官的活性热稳定,透析后丧失。使用睫状神经节外植体并评估体外培养4天后的初始纤维生长和CAT含量,发现神经营养活性在早期胚胎阶段(45 - 55毫米)最高,此后下降。结果表明活性下降并非由于毒性增加。使用已建立的分散神经节细胞存活试验,使细胞存活的神经营养因子的比活性在电器官的45至73毫米阶段之间保持恒定,然后迅速下降,但每个电器官的活性在45至73毫米阶段之间迅速增加,然后保持在恒定水平。在细胞存活试验中使用涂有心脏条件培养基的聚 - dl - 鸟氨酸底物,可使电器官提取物的营养滴度提高多达十倍。胚胎电器官中支持睫状运动神经元存活的神经营养活性热不稳定,透析后保留。结论是发育中的电器官至少含有两种具有不同特性且调控方式不同的神经营养因子。两种因子在发育过程中可能都有助于使自然发生的电运动神经元细胞死亡终止。

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