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培养海马体和皮质神经元。

Culturing hippocampal and cortical neurons.

作者信息

Meberg Peter J, Miller Matthew W

机构信息

Department of Biology, University of North Dakota, Grand Forks, North Dakota 58202, USA.

出版信息

Methods Cell Biol. 2003;71:111-27. doi: 10.1016/s0091-679x(03)01007-0.

Abstract

Primary cultures of rat and mouse hippocampus and cerebral cortex are widely used to study neuronal properties such as axonal extension, synaptic transmission, and excitotoxicity. Short-term culturing of these neurons can be very straightforward and is perhaps easier than culturing cells lines once dissections are made and cell stocks are frozen. Long-term cultures of relatively pure neuronal populations require slightly more effort, but protocols are described that are less complicated than most published protocols. These include simpler ways to clean and coat coverslips, as well as using glia-conditioned medium to eliminate the need to make individual cocultures of neurons and glia. These methods consistently yield hippocampal and cortical cultures expressing dendritic spines and synapses that survive over 3 weeks in culture. For investigators employing biochemical assays where a fairly large amount of protein is necessary, cortical neurons may be especially attractive to use as large amounts of tissue are obtained and available for culture.

摘要

大鼠和小鼠海马体及大脑皮层的原代培养物被广泛用于研究神经元特性,如轴突延伸、突触传递和兴奋性毒性。一旦完成解剖并冻存细胞储备,这些神经元的短期培养非常简单,可能比培养细胞系更容易。相对纯净的神经元群体的长期培养需要付出更多努力,但所描述的方案比大多数已发表的方案更简单。这些方法包括更简便的清洁和包被盖玻片的方式,以及使用神经胶质细胞条件培养基,从而无需单独进行神经元与神经胶质细胞的共培养。这些方法始终能培养出表达树突棘和突触的海马体及皮层培养物,这些培养物在培养中可存活超过3周。对于采用需要相当大量蛋白质的生化分析的研究人员而言,由于可获得大量用于培养的组织,皮层神经元可能特别适合使用。

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