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机构地区:[1]广东药学院生命科学与生物制药学院,广东广州510006
出 处:《广东药学院学报》2015年第3期397-402,共6页Academic Journal of Guangdong College of Pharmacy
基 金:广东省自然科学基金(10151022401000024;2014A030313586);"重大新药创制"科技重大专项(2009ZX09103-708);东莞市科技计划项目(2011105102027)
摘 要:目的研究肿瘤患者自体PBMC经体外诱导培养的CIK细胞群TCRBV亚家族表达的变化。方法Ficoll密度梯度离心法分类人体外周血单核细胞(PBMC),经IFN-γ、OKT-3以及IL-2诱导培养,Trizol试剂提取总RNA,RT-PCR半定量分析24个TCRBV亚家族表达情况,流式分选平台分选CD3+CD8+细胞和CD3+CD56+细胞亚群。结果诱导培养后的CIK中,分化的CD3+CD56+细胞亚群比例占12.6%~41.7%。PBMC中弱表达或缺失的TCRBV亚家族,在CIK中上调或恢复表达。CIK细胞群中,CD3+CD8+细胞和CD3+CD56+细胞亚群克隆组成无明显差异。结论肿瘤患者自体PBMC体外诱导培养CIK细胞后,部分表达偏移的TCRBV亚家族能恢复表达,表明部分受损或被抑制的T细胞克隆在CIK培养中被激活并增殖。Objective To investigate the variation of TCRBV subfamily between autologous PBMC from tumor patients and in vitro cultured CIK. Methods PBMC was separated by Ficoll gradient centrifugation,and cultured with IFN-γ,OKT-3 and IL-2. Total RNA was separated by Trizol,and RT-PCR was performed to analyze the expression of TCRBV 24 subfamilies. FACS was used to sort CD3+CD8+cells and CD3+CD56+cells. Results The ratio of differentiated CD3+CD56+cells in cultured CIK accounted for 12. 6%-41. 7%. The expression of TCRBV subfamilies decreased or deficient in PBMC was up-regulated in CIK.There was no significant difference in clonal combination between CD3+CD8+cells and CD3+CD56+cells. Conclusion The biased TCRBV profile can be partly recovered during in vitro CIK culture,suggesting that some T cells impaired or inhibited from tumor patient may be activated and enter replication cycle.
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