结核杆菌Mtb8.4抗原在大肠杆菌中表达的初步研究  被引量:2

Construction of prokaryotic recombinant plasmid encoding Mtb 8.4 gene of Myco-bacterium tuberculosis and its expression in E.coli

在线阅读下载全文

作  者:李素华[1] 钟森[2] 徐建国[3] 史晓玲[2] 

机构地区:[1]温州医学院附属第二医院儿内传染科,温州325027 [2]四川省泸州医学院附属医院传染科,泸州646000 [3]温州市第三人民医院ICU

出  处:《中国人兽共患病杂志》2005年第2期156-158,共3页Chinese Journal of Zoonoses

摘  要:目的构建结核杆菌低分子质量抗原Mtb8.4的原核表达质粒,并检测其在大肠杆菌中的表达。方法PCR扩增目的基因,克隆到质粒pETHisT7启动子的下游;酶切和PCR法鉴定重组子;阳性重组子转化大肠杆菌BL21(DE3)pLysS,经IPTG诱导后,SDSPAGE电泳分析。结果重组质粒pETHisMtb8.4成功构建,含阳性重组子的菌体蛋白经SDSPAGE电泳出现一新的蛋白带,与预计相符。结论初步证明构建的大肠杆菌重组体能够表达目的蛋白,为进一步对其免疫效应的研究奠定了基础。To constract the prokaryotic recombinant plasmid encoding Mtb 8.4 gene of Myco-bacterium tuberculosis and to detect the expression of proteins in E.coli, the gene encoding the protein Mtb 4.8 was amplified and cloned into the down-stream of the T7 promoter pET-His. The positive clones were screened by using the double digestion and polymerase chain reaction (PCR) and the recombinant plasmid was transformed into E.coli BL21 (DE3) as induced by IPTG, and analyzed by SDS-PAGE.It was found that the recombinant expression plasmid pET-His-His-Mtb 8.4 was constructed successfully in the present study, and the gel staining with coomassie blue G-250 showed that the induced E.coli carried the recombinant plasmid that could produced the Mtb 8.4 protein.It concludes that the constrcted recombinant of E.coli can express the target protein, thus providing the basis for the further studies on the production of antigens and antibodies of Mtb 8.4 protein in large scale and for the detection of their immune effectiveness.

关 键 词:结核分支杆菌 低分子质量抗原 分泌性 原核表达质粒 大肠杆菌 蛋白表达 

分 类 号:R378.91[医药卫生—病原生物学]

 

参考文献:

正在载入数据...

 

二级参考文献:

正在载入数据...

 

耦合文献:

正在载入数据...

 

引证文献:

正在载入数据...

 

二级引证文献:

正在载入数据...

 

同被引文献:

正在载入数据...

 

相关期刊文献:

正在载入数据...

相关的主题
相关的作者对象
相关的机构对象