培养大鼠海马和皮质原代神经元。

Q4 Neuroscience
Neuronal signaling Pub Date : 2019-04-26 eCollection Date: 2019-06-01 DOI:10.1042/NS20180207
Madhusmita Priyadarshini Sahu, Outi Nikkilä, Seija Lågas, Sulo Kolehmainen, Eero Castrén
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引用次数: 59

摘要

多年来,啮齿动物大脑海马和皮层的原代神经元一直是生物医学研究的重要工具。然而,制备初级神经元的方案各不相同,这往往导致相互矛盾的结果。该报告提供了一个强大而可靠的方案,从皮层和海马体中产生初级神经元培养物,而非神经元细胞的贡献最小。神经元在无血清培养基中生长,并在没有任何额外饲养细胞的情况下维持数周。按照这种方法培养的神经元分化,并在3周内发育出广泛的轴突和树突分支。用这种方法培养的细胞具有良好的可重复性,可用于组织学、分子和生物化学方法。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Culturing primary neurons from rat hippocampus and cortex.

Culturing primary neurons from rat hippocampus and cortex.

Culturing primary neurons from rat hippocampus and cortex.

Culturing primary neurons from rat hippocampus and cortex.

Primary neurons from rodent brain hippocampus and cortex have served as important tools in biomedical research over the years. However, protocols for the preparation of primary neurons vary, which often lead to conflicting results. This report provides a robust and reliable protocol for the production of primary neuronal cultures from the cortex and hippocampus with minimal contribution of non-neuronal cells. The neurons were grown in serum-free media and maintained for several weeks without any additional feeder cells. The neuronal cultures maintained according to this protocol differentiate and by 3 weeks develop extensive axonal and dendritic branching. The cultures produced by this method show excellent reproducibility and can be used for histological, molecular and biochemical methods.

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来源期刊
CiteScore
4.60
自引率
0.00%
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审稿时长
14 weeks
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