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rhIL-17对小鼠造血前体细胞和人脐血CD34+干细胞分化发育的影响 *
引用本文:王永红,曹雪涛,胡晋红,张明徽,陈国友,于益芝.rhIL-17对小鼠造血前体细胞和人脐血CD34+干细胞分化发育的影响 *[J].中国肿瘤生物治疗杂志,1999,6(2):136-140.
作者姓名:王永红  曹雪涛  胡晋红  张明徽  陈国友  于益芝
作者单位:第二军医大学免疫学教研室,第二军医大学免疫学教研室,第二军医大学免疫学教研室,第二军医大学免疫学教研室,第二军医大学长海医院药学部,第二军医大学免疫学教研室 上海200433,上海200433,上海200433,上海200433,上海200433
基金项目:国家自然科学基金重点项目(39730420),国家杰出青年科学基金(39825123)资助
摘    要:目的:探讨重组人白细胞介素-17(Interleukin-17,IL-17)对小鼠骨髓造血前体细胞和人脐血来源的CD34~ 干细胞生长发育的影响.方法:采用常规方法采集小鼠造血前体细胞;采用Mini-MACS分离技术,从正常人脐血分离人CD34~ 干细胞.体外加入IL-17和/或GM-CSF、IL-4培养分离的前体细胞,应用流式细胞仪检测其表型,采用ELISA法检测了其分泌的IL-12水平,通过~3H]-TdR掺入法测定其刺激同种异体T淋巴细胞增殖的能力.结果:IL-17促进了小鼠骨髓来源的未成熟DC表达Ia,B7-2等免疫分子,促使其分泌较高水平的IL-12,该细胞也能刺激同种异体T细胞有效增殖,表现出了成熟DC的特征.IL-17单独培养9d促使人脐血CD34~ 干细胞扩增了2倍,部分细胞高表达CD1a及B7-2,低表达HLA-DR,未检测到CD83的表达.该细胞能促使同种异体T细胞增殖,但作用较弱;而rhIL-17与GM-CSF联合培养后扩增了14倍,培养细胞中CD1a、B7-2阳性细胞的比例明显升高,且此细胞刺激同种异体T细胞增殖的能力较强.结论:IL-17体外可促进小鼠骨髓造血前体细胞来源的DC成熟;与GM-CSF联合培养既能促进CD34~ 干细胞增殖,又能使之获得DC特征,初步提示IL-17与GM-CSF联合作用可促进CD34~ 干细胞向DC分化.

关 键 词:白细胞介素17  造血前体细胞  CD34~  干细胞  树突状细胞  分化
收稿时间:4/8/1999 12:00:00 AM
修稿时间:1999/5/28 0:00:00

Effects of rhIL-17 on Differentiation and Development of Murine Hematopoietic Progenitors and Human Cord Blood CD34+ Stem Cells
Wang Yonghong,Cao Xuetao,Hu Jinhong,Zhang Minghui,Chen Guoyou and Yu Yizhi.Effects of rhIL-17 on Differentiation and Development of Murine Hematopoietic Progenitors and Human Cord Blood CD34+ Stem Cells[J].Chinese Journal of Cancer Biotherapy,1999,6(2):136-140.
Authors:Wang Yonghong  Cao Xuetao  Hu Jinhong  Zhang Minghui  Chen Guoyou and Yu Yizhi
Institution:Department of Immunology, Second Military Medical University, Shanghai 200433;Department of Immunology, Second Military Medical University, Shanghai 200433;Department of Immunology, Second Military Medical University, Shanghai 200433;Department of Immunology, Second Military Medical University, Shanghai 200433;Department of Immunology, Second Military Medical University, Shanghai 200433;Department of Immunology, Second Military Medical University, Shanghai 200433
Abstract:To investigate effects of rhIL-17 on growth and development of mouse bone marrow progenitors andhuman cord blood LD34~ stem cells. Methods: Mouse bone marrow progenitors were isolated by routine protocol, and CD34~ stem cells were isolated from normal human cord blood by Mini-MACS, then cultured with rhIL-17 and/or GM-CSF/IL-4. The phenotypes of the cells were analyzed by FACS, IL-12 level was analyzed by ELISA and T cell stimulating activity in allo-MLR was determined by ~3H]-TdR incorporation. Results: Expression of MHC class II molecules and B7-2 on the surface of immature DC derived from mouse bone marrow progenitors was up-regulated by IL-17. The capacity of the cells to secrete IL-12 and their T cell stimulating activity were also enhanced. The cells showed the characteristics of mature DC. After cultured with IL-17 for 9 days, the number of CD34~ stem cells increased by 2 times. The phenotypes of some cells were CDla~(high), B7-2~(high), and HLA-DR~(lwo). The cells could stimulate allo geneic T cells to proliferate but their capacity was lower than that of the cells cultured with IL-17 combined with GM-CSF. The cells cultured with IL-17 and GM-CSF proliferated markedly and the rate of CDla~ and B7-2~ cells increased significantly. The T cell stimulating activity of cells was also augmented. Conclusion: IL-17 could promote DC derived from mouse bone marrow progenitors to mature. When combined with GM-CSF, IL-17 could induce human CD34~ stem cells not only to proliferate markedly but also to show characteristics of DC, indicating that CD34~ stem cells might differentiate to DC by IL-17.
Keywords:interleukin-17  hematopoietic progenitor cells  human CD34  stem cells  dentritic cells  differentiation
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