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结核抗原ESAT-6基因的克隆及在大肠埃希菌中的表达 被引量:6

Cloning and expression of ESAT cDNA coding region of mycobacterium tuberculosis in E.Coli
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摘要 目的 将结核分支杆菌ESAT抗原编码区基因克隆 ,并使其在大肠埃希菌中表达。方法 培养并抽提结核分支杆菌基因组 ,采用聚合酶链反应 (PCR)扩增编码ESAT的全长cDNA ,并插入到原核表达载体 pGEX5T中 ,构建 pGEX5T ESAT重组质粒。IPTG诱导使该基因在k80 2菌中表达 ,并用免疫印迹 (Westernblot)方法确证表达蛋白的特异性。结果 PCR扩增获得了单一的条带 ,大小约 0 .3kb ;全自动测序与Genbank中登录的序列完全相同。获得了 pGEX5T ESAT重组子并在k80 2菌中表达 ,该蛋白可被结核病患者血清特异地识别。结论 扩增和克隆了结核杆菌ESAT抗原的全长cDNA并在大肠埃希菌中获得表达 ,为进一步研究其在结核病诊断和防治中的应用打下了基础。 Objective To clone and express the gene encoding ESAT antigen of Mycobacterium tuberculosis (chinese stain). Methods Genome of mycobacterium tuberculosis was extracted. Then, the full length cDNA encoding ESAT protein was amplified by PCR and cloned into prokaryotic expressing vector pGEX5T and sequenced. pGEX5T ESAT was expressed in k802 Ecoli, and the expressed protein was determined by western blot using the sera from ten patients with tuberculosis. Results One specific band of 0.3kb or so was obtained and sequencing result was identical to that reported from Genbank. The expressed protein could be specifically recognized by the sera from tuberculosis patients. Conclusions The full length cDNA of Mycobacterium tuberculosis (Chinese strain) ESAT protein was cloned and expressed successfully, which will be helpful in further studies on diagnosis and treatment of tuberculosis.
作者 王庆敏 胡振林 孙树汉 张巧敏
机构地区 第二军医大学医学遗传学教研室 河北省胸科医院
出处 《中华传染病杂志》 CAS CSCD 北大核心 2003年第1期30-32,共3页 Chinese Journal of Infectious Diseases
关键词 结核分支杆菌 ESAT-6 基因表达 克隆 大肠埃希菌 结核病 预防 Mycobacterium tuberculosis ESAT-6 Gene expression Cloning, molecular
分类号 R346 [医药卫生—基础医学]
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参考文献1

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同被引文献61

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中华传染病杂志
2003年 第1期

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