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贴壁培养和神经球培养中神经干细胞与祖细胞之间增殖能力和传代潜力的比较。

A comparison of proliferative capacity and passaging potential between neural stem and progenitor cells in adherent and neurosphere cultures.

作者信息

Sun Tao, Wang Xiao-Jing, Xie Shan-Shan, Zhang Dao-Lai, Wang Xu-Ping, Li Bo-Qin, Ma Wu, Xin Hua

机构信息

Department of Cell Biology, School of Medicine, Shandong University, China.

出版信息

Int J Dev Neurosci. 2011 Nov;29(7):723-31. doi: 10.1016/j.ijdevneu.2011.05.012. Epub 2011 Jun 12.

DOI:10.1016/j.ijdevneu.2011.05.012
PMID:21664447
Abstract

Neural stem and progenitor cells (NSPCs) can be isolated from the fetal or adult brain and expanded in culture for potential use in basic research, drug discovery and cell therapy. In the present study, two culture systems have been commonly used to maintain and expand NSPCs isolated from mammalian CNS: neurosphere and adhesive substrate-bound monolayer culture. NSPCs were isolated from the neuroepithelium of E14 embryonic rat cerebral cortex and maintained and expanded on fibronectin substrates or within neurospheres in serum-free medium. Ultrastructural study under transmission electron microscope revealed similar characteristics of immature morphology of NSPCs in adherent and neurosphere cultures. NSPCs cultured on adherent substrates and within neurospheres shared the properties of self-renewal and multipotency, but little is known about proliferation capacity and passaging potential of adherent NSPCs compared to neurosphere culture. We found that the self-renewal capacity of NSPCs in adherent culture was higher than that in neurosphere culture in the P1 and P3 passages, and reduced after the P5 passage. At the same time, comparative analysis using BrdU incorporation and immunostaining for nestin indicated that NSPCs grew significantly faster in primary cultures on adherent substrates than within neurospheres. Whereas, NSPCs in adherent culture could not maintain such robust growth for more than 6 passages. The growth of NSPCs within neurospheres was slower than that in adherent culture, but increased steadily and could be maintained for more than 10 passages. These data provide useful information for large scale in vitro expansion of NSPCs required by potential drug screening and cell therapy.

摘要

神经干细胞和祖细胞(NSPCs)可从胎儿或成体大脑中分离出来,并在培养中进行扩增,以用于基础研究、药物发现和细胞治疗。在本研究中,两种培养系统常用于维持和扩增从哺乳动物中枢神经系统分离出的NSPCs:神经球培养和黏附于底物的单层培养。NSPCs从E14胚胎大鼠大脑皮层的神经上皮中分离出来,在纤连蛋白底物上或无血清培养基中的神经球内进行维持和扩增。透射电子显微镜下的超微结构研究揭示了贴壁培养和神经球培养中NSPCs未成熟形态的相似特征。在贴壁底物上培养和在神经球内培养的NSPCs都具有自我更新和多能性的特性,但与神经球培养相比,关于贴壁NSPCs的增殖能力和传代潜力知之甚少。我们发现,在第1代和第3代传代时,贴壁培养的NSPCs的自我更新能力高于神经球培养,而在第5代传代后降低。同时,使用BrdU掺入和巢蛋白免疫染色的比较分析表明,贴壁底物上的原代培养物中的NSPCs比神经球内的生长明显更快。然而,贴壁培养的NSPCs传代超过6次后就无法维持如此强劲的生长。神经球内NSPCs的生长比贴壁培养慢,但稳步增加,并且可以维持超过10代。这些数据为潜在药物筛选和细胞治疗所需的NSPCs大规模体外扩增提供了有用信息。

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