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HCV C-Fc基因转染的小鼠树突状细胞促进混合淋巴细胞反应的作用
引用本文:王全楚,冯志华,周永兴,聂青和,白雪帆. HCV C-Fc基因转染的小鼠树突状细胞促进混合淋巴细胞反应的作用[J]. 细胞与分子免疫学杂志, 2004, 20(3): 301-303
作者姓名:王全楚  冯志华  周永兴  聂青和  白雪帆
作者单位:第四军医大学唐都医院全军感染病诊疗中心,陕西,西安,710038
基金项目:国家自然科学基金资助项目 (No .30 1 70 82 2 )
摘    要:目的:观察HCVC-FC基因电穿孔法转染的小鼠树突状细胞(DC)功能的改变。方法:分离小鼠骨髓单个核细胞与rmGM-CSF和rmIL-4培养1wk,对培养的细胞进行形态学观察.并用FACS检测细胞表面DEC205的表达。以通过质粒pcD一NA3HCV C—Fc电穿孔法转染培养的DC,用间接免疫荧光染色测定转染细胞中HCV C—FC的水平;用混合淋巴细胞反应检测电穿孔法转染细胞的功能。结果:培养1wk后,得到具有典型DC形态的细胞,以质粒pcDNA3HCV c-FC为载体电穿孔法转染DC后,转染细胞中可检测到较高水平的HCVC—Fc2与对照组相比较以电穿孔法转染的细胞能明显刺激混合淋巴细胞反应:结论:小鼠骨髓单个核细胞加GM-CSF和IL-4培养1wk,可生成大量的DC。质粒pcDNA3HCV c-Fc转染培养的DC对T细胞刺激作用显著增强。

关 键 词:小鼠树突状细胞  电转染  混合淋巴细胞反应  HCV  C—Fc基因
文章编号:1007-8738(2004)03-0301-03
修稿时间:2003-07-02

Acceleration of mixed lymphocyte reaction by HCV C-Fc gene-transferred murine dendritic cells
Quan-chu Wang,Zhi-hua Feng,Yong-xing Zhou,Qing-he Nie,Xue-fan Bai. Acceleration of mixed lymphocyte reaction by HCV C-Fc gene-transferred murine dendritic cells[J]. Chinese journal of cellular and molecular immunology, 2004, 20(3): 301-303
Authors:Quan-chu Wang  Zhi-hua Feng  Yong-xing Zhou  Qing-he Nie  Xue-fan Bai
Affiliation:The Center of Diagnosis and Treatment of Infection Diseases of PLA, Tangdu Hospital, Fourth Military Medical University, Xi'an 710038, China. quanchuwang998@hotmail.com
Abstract:AIM: To observe the metergasis of murine dendritic cells (DCs) transfected with HCV C Fc gene through electroporation. METHODS: Mononucleocytes isolated from murine bone marrow were co cultured with rmGM CSF and rm IL 4 for 7 days. Morphological characteristics of the cultured cells were observed under scan electron microscope (SEM) and the expression of DEC205 on the cells was detected by FACS. DCs derived from the culture were transfected with plasmids containing HCV C Fc gene. HCV C Fc level in the transfected cells was detected by indirect immunofluorescence assay. MLR was studied with DCs and T cells. RESULTS: Following 7 day culture, a large number of cells with typical characteristics of DC were observed. The HCV C Fc level in the transfected DCs was higher. MLR was stimulated markedly by DCs transfected with HCV C Fc gene in comparison with the control group. CONCLUSION: A large number of DCs could be generated from murine bone marrow mononucleocyte cultures supplemented with GM CSF and IL 4 for 1 week. The function of DCs transfected with pcDNA3HCV C Fc was enhanced in MLR.
Keywords:dendritic cell  electrotransfection  mixed lymphocyte reaction  HCV C Fc gene
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