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作 者:周健[1] 黄迎[2] 吴远彬[1] 胡亮杉[1] 涂三芳[1] 王杨[1] 孙明[1] 郭爱林[2] 郭坤元[1]
机构地区:[1]南方医科大学珠江医院血液科,广东广州510282 [2]广东省人民医院医学研究中心,广东广州510080
出 处:《中国现代医学杂志》2008年第17期2456-2459,2463,共5页China Journal of Modern Medicine
基 金:国家自然科学基金资助项目(No:30471636)
摘 要:目的建立小鼠T细胞受体(TCR)互补决定区3(CDR3)谱型的基因扫描分析术,为分析T细胞克隆提供研究方法。方法应用RT-PCR方法分别扩增近交系小鼠C57BL/6H-2b,Balb/CH-2d和F1代小鼠(Balb/c×C57BL/6F1H-2d/b,CB6F1)脾脏T细胞的21个TCRVα家族和18个TCRVβ家族的CDR3,并用基因扫描分析扩增产物以确定T细胞的克隆性。结果3种小鼠脾脏T细胞均表达所有的TCRVα和VβCDR3基因,基因扫描显示全部TCRCDR3谱型呈高斯(钟型)分布,提示均为多克隆T细胞。各家族CDR3基因表达频率接近,但呈现不同的多态性和长度分布。结论基因扫描分析TCRαβCDR3基因谱型是检测小鼠T细胞克隆性的精确敏感方法。[Objective] To establish genescan technique of diversity gene of T cell antigen reeeptor(TCR) complementary-determining region 3(CDR3) for assaying elonality of mouse TCR αβ T cell. [Methods] 21 TCR et chain variable gene(TCR Vet) and 18 TCR β chain variable gene (TCR Vβ) of spleen T cell of C57BL/6^H-2b, Balb/ C^H-24 and CB6F1 (Balb/exC57BL/6 F1^H-2d/b) inbreeding line mouse were amplified by RT-PCR. Productions of RT- PCR were assayed by genescan technique to determine clonality of TCR αβ T cell. [Results] All the TCR Vet and TCR Vα genes were expressed in spleen T cell of 3 kinds inbreeding line mouse. All the CDR3 repertoire showed Gaussian distribution, which suggested that T cell were multielonal. The CDR3 of the TCR Vα and Vβ subfamily has the similar frequency of occurrence, but has the different pelymorphism and length profiles. [Conclusion] Genesean technique of diversity gene of TCR CDR3 was stable and precise method for assaying elonality of mouse TCR αβ T cell.
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