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作 者:徐雪梅[1] 符州[1] 田代印[1] 刘恩梅[1] 王莉佳[1] 黄英[1]
机构地区:[1]重庆医科大学附属儿童医院呼吸科,重庆400014
出 处:《重庆医科大学学报》2008年第8期897-899,910,共4页Journal of Chongqing Medical University
基 金:国家自然科学基金资助项目(编号30672268)
摘 要:目的:分别克隆小鼠信号传导及转录活化因子-4(Signal transducers and activators of transcription-4,STAT4)、信号传导及转录活化因子-6(Signal transducers and activators of transcription-6,STAT6)基因全长cDNA序列,构建并鉴定其真核表达质粒pIRES2-EGFP-STAT4/STAT6。方法:采用RT-PCR方法从BALB/c小鼠脾脏组织中扩增STAT4/STAT6基因全长cDNA,T/A克隆到pMD19-T载体中,双酶切后将cDNA亚克隆入pIRES2-EGFP载体,构建pIRES2-EGFP-STAT4/STAT6质粒,经限制性内切酶鉴定并测序。结果:小鼠STAT4/STAT6基因cDNA正确克隆入pIRES2-EGFP表达载体,与Genebank中STAT4/STAT6基因序列一致。结论:成功构建pIRES2-EGFP-STAT4/STAT6表达质粒,为进一步研究STAT4/STAT6蛋白表达和相互作用奠定了基础。Objective:To clone mouse signal transducers and activators of transcription(STAT) 4 and STAT6 gene and construct a eukaryotic expression plasimid. Methods:The cDNA of mouse STAT4 and STAT6 gene amplified with RT-PCR from normal mouse spleen tissue were cloned into pMD19-T vector by T/A ligation. After double digested,STAT4/STAT6 cDNA fragment was suhcloned into pIRES2-EGFP vector to construct a eukaryotic expression plasimid. Restriction endonucleases analysis and sequencing were used to comform the recomhinant plasimid. Results:The full length STAT4/STAT6 cDNA was correctly inserted into eukaryotic expression plasimid,and its sequencing was consistent with reported sequence derived from Genebank. Conclusion:The successful construction of eukaryotic expression plasimid provides a basis for futher studies on the infection of STAT4/STAT6 interaction to the downstream cytokines.
关 键 词:哮喘 信号传导及转录活化因子 克隆 真核表达质粒
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