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大鼠骨髓来源树突状细胞体外培养体系的优化
引用本文:汪国营,张琪,刘炜,陈文捷,李敏如,李团结,陈伟,陈规划.大鼠骨髓来源树突状细胞体外培养体系的优化[J].器官移植,2011,2(3):135-140.
作者姓名:汪国营  张琪  刘炜  陈文捷  李敏如  李团结  陈伟  陈规划
作者单位:中山大学附属第三医院肝移植中心,中山大学器官移植研究所,广东省器官移植研究中心,广州,510630
基金项目:国家重点基础研究发展计划(973计划)课题(2009CB522404); 国家自然科学基金资助项目(30972914,81000190)
摘    要:目的 探讨优化大鼠骨髓来源树突状细胞(DC)体外培养体系的方法.方法 应用重组大鼠粒细胞-巨噬细胞集落刺激因子(recombinant rat GM-CSF,rrGM-CSF) 20 μg/L和重组大鼠白介素(recombinant rat interleukin,rrIL)- 4 10 μg/L诱导分化Lewis大鼠...

关 键 词:树突状细胞  重组大鼠粒细胞-巨噬细胞集落刺激因子  重组大鼠白介素-4  脂多糖  混合淋巴细胞反应  细胞培养

Optimization of the in vitro culture system for bone marrow-derived dendritic cells in rats
WANG Guo-ying,ZHANG Qi,LIU Wei,CHEN Wen-jie,LI Min-ru,LI Tuan-jie,CHEN Wei,CHEN Gui-hua.Optimization of the in vitro culture system for bone marrow-derived dendritic cells in rats[J].Ogran Transplantation,2011,2(3):135-140.
Authors:WANG Guo-ying  ZHANG Qi  LIU Wei  CHEN Wen-jie  LI Min-ru  LI Tuan-jie  CHEN Wei  CHEN Gui-hua
Affiliation:WANG Guo-ying,ZHANG Qi,LIU Wei,CHEN Wen-jie,LI Min-ru,LI Tuan-jie,CHEN Wei,CHEN Gui-hua. Liver Transplantation Center of the Third Affiliated Hospital,Transplantation Research Institute of Sun Yat-sen University,Organ Transplantation Research Center of Guangdong Province,Guangzhou 510630,China
Abstract:Objective To investigate the optimization of the in vitro culture system for bone marrow-derived dendritic cells(DC)in rats.Methods Immature DC from bone marrow cells of Lewis rats were induced and differentiated in vitro by 20 μg/L recombinant rat granulocyte macrophage colony stimulating factor(rrGM-CSF)and 10 μg/L recombinant rat interleukin(rrIL)-4.On day 6,100 μg/L of lipopolysaccharide was added and the cells were cultured for another 48 h to generate mature DC.The morphological features were observed by invert optical microscope.The immune phenotypes of DC were detected by flow cytometry(FACS).The contents of interleukin(IL)-12 and IL-10 in the DC supernatant were detected by direct sandwich enzyme-linked immune absorbent assay(ELISA).Mixed lymphocyte reaction(MLR)culture was performed to observe the proliferation of T lymphocyte cells by the DC stimulation,while Brown Norway rat splenetic T lymphocyte cells were used as responders.Results The cultured cells were identified as DC by cytomorphology,FACS and MLR.After culture for six days,the cultured cells displayed the typical morphology of dendritic cells,with high expression of OX62(the marker of rat DC).After LPS stimulation,most cells in culture had more dendrite-like characters on the surface and expressed major histocompatibility complex(MHC)class Ⅱ,CD40 and CD86 abundantly.They stimulated allogeneic T cell responses effectively in MLR.Compared with immature DC,mature DC produced significantly more IL-12 and IL-10 to stimulate the proliferation of T lymphocyte cells.Conclusion The improved culture system from bone marrow cells of rats can induce plenty of bone marrow-derived DC in rats through adjusting the doses of rrGM-CSF and rrIL-4.
Keywords:Dendritic cells  Recombinant rat granulocyte macrophage colony stimulating factor  Recombinant rat interleukin-4  Mixed lymphocyte reaction  Cell culture  
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