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成年大鼠海马神经元的分离与培养。

Isolation and culture of adult rat hippocampal neurons.

作者信息

Brewer G J

机构信息

Department of Medical Microbiology and Immunology, Southern Illinois University School of Medicine, Springfield 62794-1220, USA.

出版信息

J Neurosci Methods. 1997 Feb;71(2):143-55. doi: 10.1016/s0165-0270(96)00136-7.

Abstract

Inability to culture adult central neurons and the failure of injured neurons to regenerate in the brain could be due to genetic controls or environmental inhibitors. We tested the environmental inhibitor hypothesis by attempting to regenerate adult rat neurons in B27/Neurobasal culture medium, a medium optimized for survival of embryonic neurons. To isolate neurons from their numerous connections, papain was the best of six different proteases screened on slices of hippocampus for survival of isolated cells after 4 days of culture. Use of a density gradient enabled separation of oligodendroglia and some enrichment of neurons and microglia from considerable debris which was inhibitory to sprouting and viability. With these techniques, about 900000 viable neurons were isolated from each hippocampus of any age rat from birth to 24-36 months, near the median mortality. FGF2 was found to enhance viability at least 3-fold to 40-80%, independent of age, without affecting the length of the processes. Neurons were cultured for more than 3 weeks. These methods demonstrate that hippocampal neurons can regenerate axons and dendrites if provided with adequate nutrition and if inhibitors are removed. They also will enable aging studies. Therefore, the concept of environmental growth restriction may be more appropriate for neurons in the brain than the concept of a genetic block that precludes regeneration of processes.

摘要

成年中枢神经元无法培养,且脑内受损神经元无法再生,这可能是由于基因控制或环境抑制因素所致。我们通过尝试在B27/Neurobasal培养基中使成年大鼠神经元再生,来检验环境抑制假说,该培养基是一种针对胚胎神经元存活优化的培养基。为了使神经元与其众多连接分离,在对海马切片筛选的六种不同蛋白酶中,木瓜蛋白酶是培养4天后分离细胞存活情况最佳的一种。使用密度梯度能够分离少突胶质细胞,并从大量对发芽和活力有抑制作用的碎片中对神经元和小胶质细胞进行一定程度的富集。通过这些技术,从出生至24 - 36个月龄(接近平均死亡率)的任何年龄大鼠的每个海马中分离出约900000个存活神经元。发现成纤维细胞生长因子2(FGF2)可将活力提高至少3倍,达到40%至80%,与年龄无关,且不影响突起长度。神经元培养超过3周。这些方法表明,如果提供充足营养并去除抑制剂,海马神经元能够再生轴突和树突。它们也将有助于衰老研究。因此,对于脑内神经元而言,环境生长限制的概念可能比排除突起再生的基因阻滞概念更为合适。

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