| 大鼠皮质神经元的体外培养及不同浓度尿激酶干预后的观察 |
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| 引用本文: | 葛汝村,吕涌涛,魏巍,陈平,冯肖亚,徐林. 大鼠皮质神经元的体外培养及不同浓度尿激酶干预后的观察[J]. 神经损伤与功能重建, 2019, 14(6): 271-274 |
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| 作者姓名: | 葛汝村 吕涌涛 魏巍 陈平 冯肖亚 徐林 |
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| 作者单位: | 山东省立第三医院再生医学研究室济南 250031;山东省立第三医院再生医学研究室济南 250031;山东省立第三医院神经内科济南 250031;山东省立第三医院神经内科济南 250031 |
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| 基金项目: | 山东省卫生和计生委科技计划项目(No. 2015WS0262) |
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| 摘 要: | 目的:建立科学简易的大鼠皮质神经元的体外培养方法,观察尿激酶对其干预后的表现。方法:取24h内新生Wistar大鼠脑皮质,用浓度为2mg/mL的木瓜酶和适量DNaseI酶共同消化,并用配置好的无血清Neurobasal培养基接种培养,6d后免疫荧光法鉴定神经元纯度;分别配置含尿激酶终浓度为5000U/mL、8000U/mL、10000U/mL、15000U/mL和20000U/mL的Neurobasal培养基并进行全量换液,镜下观察不同浓度尿激酶干预后神经元的变化。结果:培养6d,神经元分化成熟,胞质丰富,树突及轴突舒展延长,可见密集的神经纤维网络,免疫荧光鉴定神经元纯度为88.2%;尿激酶干预后,发现尿激酶浓度在5000~10000U/mL时,2h内镜下观察培养体系无明显变化,但随时间的延长,尿激酶浓度为10000U/mL作用4h时,可见少量神经元细胞破碎崩解,细胞间网状结构减少。尿激酶浓度在15000U/mL及20000U/mL时,干预2h发现神经元细胞崩解,网状结构消失。结论:本实验建立了一种简易、高效的体外培养新生大鼠皮质神经元的方法,尿激酶浓度在5000~10000U/mL时,2h内对体外神经元培养体系是安全的。
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| 关 键 词: | 神经元 细胞培养 培养基 免疫荧光 尿激酶 |
Culture of Newborn Rat Cortex Neurons in Vitro and Effect of Urokinase |
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| GE Ru-cun,LV Yong-tao,WEI Wei,CHEN Ping,FENG Xiao-ya,XU Lin. Culture of Newborn Rat Cortex Neurons in Vitro and Effect of Urokinase[J]. Neural Injury and Functional Reconstruction, 2019, 14(6): 271-274 |
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| Authors: | GE Ru-cun LV Yong-tao WEI Wei CHEN Ping FENG Xiao-ya XU Lin |
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| Affiliation: | (Regenerative Medicine Research Lab,Shandong Provincial Third Hospital, Jinan 250031, China;Department of Neurology,Shandong Provincial Third Hospital, Jinan 250031, China) |
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| Abstract: | To establish a more scientific and simple method for the culturing of cerebral corticalneurons from newborn rats and observe the interventional effect of different concentrations of urokinase.Methods: The cerebral cortex of newborn Wistar rats was extracted and then digested by papaya enzyme (2 mg/mL) and an appropriate amount of DNase I enzyme. Neurons were cultured with serum-free Neurobasal medium.After 6 days, the purity of neurons was identified by immunofluorescence. Neurobasal media with finalurokinase concentrations of 5 000 U/mL, 8 000 U/mL, 10 000 U/mL, 15 000 U/mL, and 20 000 U/mL wereprepared for media changes. Neurons were observed under microscope for changes due to intervention fromvarious concentrations of urokinase. Results: After 6 days of culture, the neurons were well-differentiated withabundant cytoplasm, and neuronal dendrites and axons extended and overlapped into a dense network. Neuronspurity was identified as 88.2% by immunofluorescence staining. After intervention with urokinase at aconcentration of 5 000 to 10 000 U/mL, no significant change in the culture system was observed undermicroscope within 2 h, but over time, a small number of neuronal cell disruption and network structure decreasecould be observed with 10 000 U/mL at 4 h. With 15 000 U/mL and 20 000 U/mL, at 2 h after the intervention,fragmented material was observed at the bottom of the medium, and the intercellular network structuredisappeared. Conclusion: In this study, a simple and efficient method of culturing newborn rat cortical neuronswas established. When urokinase concentration was between 5 000 and 10 000 U/mL, it was safe to cultureneurons within 2 h in vitro. |
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| Keywords: | neuron cell culture culture media immunofluorescence urokinase |
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