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首页> 外文期刊>Cellular and Molecular Neurobiology >A serum- and antioxidant-free primary culture model of mouse cortical neurons for pharmacological screen and studies of neurotrophic and neuroprotective agents.
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A serum- and antioxidant-free primary culture model of mouse cortical neurons for pharmacological screen and studies of neurotrophic and neuroprotective agents.

机译:小鼠皮质神经元的无血清和抗氧化剂的原代培养模型,用于药理筛选和神经营养和神经保护剂的研究。

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摘要

1. Morphologically developmental properties of fetal mouse cortical neurons in the chemically defined serum- and antioxidant-free culture condition were observed. Also, cellular composition in cultures was identified by immunostaining with anti-NSE and anti-GFAP. 2. Various cell densities ranging from 1 x 10(3) to 1 x 10(6) cells/cm2 were prepared to further assess the effect of cell density on time-course of neuronal survival by counting the number of remaining attached neurons after 3 and 7 days in culture. 3. Neuronal responses to neurotrophic effect of NGF on neurite outgrowth and neuroprotective effect of MK-801 against glutamate-induced excitotoxity were evaluated by image analysis and MTT assay, respectively. 4. Results showed that this culture system was neuronal-enriched with a neuronal lifetime more than 35 days. Neurons survived best when seeded at a density > or =1.5 x 10(5) cells/cm2. Cultured neurons were capable of exhibiting sensitive responses to the effects of NGF and MK-801. 5. These findings suggest that this primary culture system provides a sensitive and powerful in vitro model for pharmacological screen and studies of neurotrophic and neuroprotective agents.
机译:1.在化学定义的无血清和无抗氧化剂的培养条件下,观察了胎鼠皮质神经元的形态学发育特性。另外,通过用抗NSE和抗GFAP进行免疫染色来鉴定培养物中的细胞组成。 2.制备了从1 x 10(3)到1 x 10(6)个细胞/ cm2的各种细胞密度,以通过计算3次后剩余附着神经元的数量来进一步评估细胞密度对神经元存活时间过程的影响。和7天的文化。 3.分别通过图像分析和MTT分析评估了神经生长因子对神经突生长的神经营养作用的神经元响应和MK-801对谷氨酸诱导的兴奋性毒性的神经保护作用。 4.结果表明,该培养系统富含神经元,神经元寿命超过35天。当接种密度大于或等于1.5 x 10(5)个细胞/ cm2时,神经元存活最佳。培养的神经元能够表现出对NGF和MK-801的敏感反应。 5.这些发现表明,这种主要的培养系统为药理学筛选和神经营养和神经保护剂的研究提供了灵敏而强大的体外模型。

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