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作 者:柳静[1] 黄洋[1] 张颖丽[1] 周春华[1] 欧阳红生[2] 逄大欣[2]
机构地区:[1]吉林大学口腔医学院儿童牙病科,长春130041 [2]吉林大学农学部畜牧兽医学院生物化学研究室
出 处:《现代口腔医学杂志》2006年第4期391-393,共3页Journal of Modern Stomatology
基 金:长春市科技局基金(编号:04一07SF061);2003年吉林大学创新基金(编号:200CX)
摘 要:目的在成功构建运动发酵单胞茵乙醇脱氢酶基因(adhB)置换变链乳酸脱氢酶基因(ldh)重组质粒pMDLA的基础上,构建表达栽体pET-28a-adhB,在大肠杆茵中进行目的基因的诱导表达。方法应用DNA重组技术构建表达载体,通过SDS-SAGE和乙醛指示平板鉴定目的基因的表达效率。结果成功构建了表达栽体pET-28a-adhB,通过SDS-PAGE检测可见特异性蛋白表达条带,在乙醛指示平板上可见阳性蓠落。结论根据测序及大肠杆茵表达结果,可确定该重组质粒中口adhB已完全替换ldh,为下一步构建乳酸脱氢酶活性缺陷的变链突变株奠定基础。Objective To express the gene of alcohol dehydrogenase in E. coll. , which was obtained from the recombinant vector of pMDLA for the replacement therapy of dental caries. Methods adhB gene was digested by restriction enzymes from the recombinant vector and inserted into the expression vector pET - 28a and then expressed in E. coli BL21. Results Expression vector of pET - 28a - adhB was successfully constructed. A specific 40,000 - protein band could be seen on the SDS - PAGE gel induced by IPTG and positive clones were observed on aldehyde indicator plates. Conclusion It is comfirmed that the ldh gene was replaced perfectly by adhB gene,which is a start for the further study of the constuction of LDH - deficient mutant of S. mutans.
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