新生大鼠大脑皮层和海马神经元体外培养方法及改进

探索用24 h内新生SD大鼠进行神经元体外培养的方法.取新生SD大鼠的大脑皮层和海马,胰酶消化5～10 min后,放入含100 g/L血清的DMEM/F12培养基中培养.24 h后,更换含B27无血清培养基.以后每隔1d,半换液.结果显示绝大部分神经元于第2天长出突起,第3天神经元间形成复杂的联系,第7天神经元发育基本成熟.经神经元特异性烯醇酶(NSE)鉴定,培养细胞均为神经元,纯度可达90%以上,可以用于实验.

The Method and Improvement of Primarily Culturing Neurons from the Cerebral Cortex and Hippocampus of Newborn Rats

In order to get the method of primary neuronal culture of newborn rats.The cerebral cortex and hippocampus were dissected from the newborn rat,dissociated by trypsinization,and plated onto coverslips in DMEM/F12,supplemented with 100*!g/L serum.Twenty-four hours after plating,the medium was replaced with medium containing B*!27 without serum,and replaced half medium every two days.The most neurons get dendrites and axon on the second day.On the third day,the touch formed among neurons.Neurons matured in the seventh day.After identified by neuron-specific enolase,the purity of the cultural neurons was more than 90*!%.Then cells were used to experiment.