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首页> 外文期刊>Invertebrate neuroscience >Induction and inhibition of an apparent neuronal phenotype in Spodoptera frugiperda insect cells (Sf21) by chemical agents
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Induction and inhibition of an apparent neuronal phenotype in Spodoptera frugiperda insect cells (Sf21) by chemical agents

机译:化学药剂诱导和抑制草地贪夜蛾昆虫细胞(Sf21)中明显的神经元表型

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The goal of this research was to induce neuron-like properties in Sf21 cells, an insect ovarian cell line, which could lead to a new high-throughput insecticide screening method and a way to mass produce insect neuronal material for basic research. This study applied differentiation agents to produce viable neuron-like cells. In the presence of the molting hormone 20-hydroxyecdysone (20-HE), or insulin, in the growth medium, a maximum of ca. 30 % of Sf21 cells expressed an apparent neuronal morphology of unipolar, bipolar, or multipolar axon-like processes within 2–3 days. Maximal differentiation occurred after 2 days in the presence of 50 μM 20-HE or 3 days in 10 μM insulin. Both 20-HE and insulin displayed time- and concentration-dependent differentiation with biphasic curves, suggesting that two binding sites or processes were contributing to the observed effects. In addition, combinations of 20-HE and insulin produced apparent synergistic effects on differentiation. Caffeine, a central nervous system stimulant, inhibited induction of elongated processes by 20-HE and/or insulin, with an IC50 of 9 nM for 20-HE, and the inhibition was incomplete, resulting in about one-quarter of the differentiated cells remaining, even at high concentrations (up to 1 mM). The ability to induce a neural phenotype simplifies the studies of insect cells, compared to either the use of primary nervous tissue or genetic engineering techniques. The presence of ion channels or receptors in the differentiated cells remains to be determined.
机译:这项研究的目的是在昆虫卵巢细胞Sf21细胞中诱导类似神经元的特性,这可能会导致一种新的高通量杀虫剂筛选方法以及为基础研究大规模生产昆虫神经元材料的方法。这项研究应用分化剂来产生可行的神经元样细胞。在生长介质中存在蜕皮激素20-羟基蜕皮激素(20-HE)或胰岛素的情况下,最大30%的Sf21细胞在2-3天内表现出单极,双极或多极轴突样过程的明显神经元形态。在存在50μM20-HE的2天后或在10μM胰岛素中3天后出现最大分化。 20-HE和胰岛素均显示出时间依赖性和浓度依赖性的双相曲线,表明两个结合位点或过程有助于观察到的效应。另外,20-HE和胰岛素的组合对分化产生明显的协同作用。咖啡因是中枢神经系统的刺激物,抑制了20-HE和/或胰岛素对延长过程的诱导,对20-HE的IC50为9 nM,并且抑制作用不完全,导致剩下约四分之一的分化细胞,即使在高浓度下(高达1 mM)。与使用初级神经组织或基因工程技术相比,诱导神经表型的能力简化了昆虫细胞的研究。分化细胞中离子通道或受体的存在尚待确定。

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