摘要
目的:建立体外从健康成人外周血单核细胞(Mo)诱导培养成熟的树突状细胞(DC)的方法。方法:采用连续贴壁法分离正常人外周血单核细胞,在GM-CSF和IL-4的完全培养基中培养。培养5天后收集细胞,重新铺板后继续在TNF-α的完全培养基中培养48小时后,收集细胞和上清液,采用流式细胞术检测DC表型CD80、CD83、CD40的表达;用ELISA法检测上清液中细胞因子IL-12的浓度;用倒置显微镜动态观察DC形态变化。结果:采用连续贴壁法和用GM-CSF、IL-4和TNF-α联合培养可以从人外周血诱导培养出大量的树突状细胞,且高表达CD80、CD83、CD40,表达率分别为84.29%、90.73%、92.38%。DC分泌的细胞因子IL-12浓度为38.52±11.34pg/ml。结论:采用连续贴壁法和用GM-CSF、IL-4和TNF-α联合培养可以从人外周血诱导培养大量的树突状细胞,检测表型CD80、CD83、CD40的表达率和细胞因子IL-12浓度可以鉴定树突状细胞。
Objective:To establish a method to generate mature dentritic cells (DC)from monocytes in peripheral blood from healthy adults in vitro. Methods:Monocytes were seperated from peripheral blood with a successive adherence method and were cultured with GM-CSF and IL-4 for 5 days. The cultured monocytes were cultured with TNF-α for another 48 h. The cultured ceils and supernatant were gathered for detection of CDS0, CD83, and CIM0 by flow cytometry and IL-12 in the supernatant by ELISA. The morphology of DC was observed with up-side-down microscope. Results: Large numbers of DC were cultured with a successive adherence method and culturing with GM-CSF, IL-4, and TNF-α. The cultured DC highly expressed CD80 ,CD83, and CD40 with a rate of 84.29% ,90.73%, and 92.38%, respectively. IL-12 in the supernatant was (38.52 ± 11.34) pg/ml. Conclusion: The successive adherence method and culturing with GM-CSF, IL-4, and TNF-α can be suitable for generating substantive DC. To detect the expression rate of CD80, CD83, and CD40 and the concentration of IL-12 may be useful to identify DC.
出处
《浙江中西医结合杂志》
2009年第12期740-742,F0003,共4页
Zhejiang Journal of Integrated Traditional Chinese and Western Medicine
关键词
外周血
树突状细胞
体外培养
鉴定
peripheral blood dendritic cell in vitro culture identify
