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机构地区:[1]川北医学院附属医院老年科,四川省南充市637000
出 处:《医学理论与实践》2016年第24期3301-3303,3311,共4页The Journal of Medical Theory and Practice
摘 要:目的:体外建立一种高纯度的大鼠皮层神经元原代培养的方法。方法:孕15~18dSD大鼠胚鼠为研究对象,分离胚鼠大脑皮层,采用胰酶消化方法与机械吹打相结合的方法制备细胞悬液,以适当的密度接种于培养板;细胞培养过程中,以含10%FBS的高糖DMEM/F12培养液接种细胞,24h后全量换液换为含2%B27的Neurobasal-A培养液,抑制非神经元细胞的增殖,以代替阿糖胞苷继续维持培养,倒置显微镜下定时观察细胞形态。结果:神经元细胞分散均匀,紧密贴壁,生长状态良好,神经细胞周围突起相互连接形成神经网络,通过免疫细胞化学方法鉴定神经元纯度为(93.7±5.5)%。结论:此实验方法体外可获得较高纯度的大鼠皮层神经元细胞。Objective: Establish a method of primary culture high-purity rats cortical neuron in vitro. Methods: The pregnant 15-18d SD rat embryonic mouse was the object of study, which cerebral cortex was stripped. The cell sus- pension was prepared by combining mechanical percussion method with trypsin digestion method. Cells with the appro- priate density were inoculated in the culture plate. The just inoculated cells were cultured in the high glucose DMEM/ F12 medium containing 10% FBS. The medium was exchanged wholy for Neurobasal-A medium containing 2% B27 af- ter 24h,which restrained the proliferation of non-neuronal cells and substituted cytarabine to maintain culture cells. Cell morphology was observed regularly under the inverted microscope. Results: Neurons were distributed evenly, tightly ad- herent, and grew well. Nerve cell axons and neurite were connected to each other to form a neural network. Neurons purity was identified (93. 7 ±5. 5)% by immunocytochemical method. Conclusion: Higher-purity rat cortical neuron cells were successfully cultured in vitro with this experimental method.
分 类 号:R329.2[医药卫生—人体解剖和组织胚胎学]
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