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作 者:朱勇[1] 陈良万[1] 林若柏[1] 韩子阳[1] 康明强[1]
机构地区:[1]福建医科大学附属协和医院胸心外科,福建福州350001
出 处:《吉林大学学报(医学版)》2009年第2期326-329,397,共5页Journal of Jilin University:Medicine Edition
基 金:福建省科技厅科技计划重点项目资助课题(2006Y0015);福建省卫生厅青年科研基金项目资助课题(2008)
摘 要:目的:探讨SD大鼠骨髓间充质干细胞(MSCs)体外分离培养、表型鉴定和标记的方法,为进一步研究MSCs干预器官移植的免疫排斥奠定基础。方法:采用直接贴壁法分离培养MSCs;通过流式细胞术检测细胞表面标志抗原CD90、CD45的表达率对培养的MSCs进行表型鉴定;DAPI标记第3代MSCs,观察标记效率。结果:体外培养的原代MSCs48h内可见有少量贴壁细胞,7~10d达到90%汇合;流式细胞术检测,第3代MSCs表面标记物CD90、CD45的阳性率分别为99.8%、6.8%,提示MSCs表达CD90而不表达CD45;用DAPI进行细胞标记后,荧光显微镜下见所有MSCs均已被标记蓝色荧光,提示DAPI标记法敏感性好,标记效率高。结论:贴壁培养法是一种简便易行的培养MSCs方法,操作简单,成功率高,可以作为培养SD大鼠MSCs的常规方法;DAPI标记可作为标记MSCs的一种有效手段。Objective To investigate the methods of isolation, culture, identification and labeling of mesenchymat stem cells (MSCs) in vitro and lay a foundation for further study on intervention of MSCs on immunologic rejection of organ transplantation. Methods MSCs were isolated and cultivated by adherent methods . The expressions of CD90 and CD45 of cells were analyzed by using flow cytometry in order to identify MSCs. The third generation of MSCs were labeled by DAPI, the labeling efficiency was detected. Results Primary cultured MSCs adhered to plastic surface within 48 h and reached 90% confluence within 7-10d . Flow cytometry showed that the positive rates of CD90 and CD45 of MSCs at third generation were 99.8% and 6.8%. MSCs expressed CD90 but no CD45. All of the MSCs after labeling by DAPI showed blue fluorescence by immunofluoroscope. DAPI labeling was sensitive and highly efficient to MSCs. Conclusion Adherent method is simple and easy to isolate and cultivate MSCs and it can serve as a routine method. DAPI labeling can be used as a efficient method to label MSCs.
关 键 词:骨髓 间充质干细胞 细胞培养技术 大鼠 SPRAGUE-DAWLEY
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