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作 者:郭虹[1] 陈观今[1] 周永安[1] 郑焕钦[1] 刘彦文[1]
机构地区:[1]中山医科大学寄生虫学研究所
出 处:《中国人兽共患病杂志》1999年第1期3-5,共3页Chinese Journal of Zoonoses
基 金:中国博士点医学科研基金
摘 要:目的构建弓形虫ZS2株pcDNA3-ROP1真核表达重组质粒,为进一步表达及DNA免疫做准备。方法用PCR技术从弓形虫ZS2分离株的基因组DNA中扩增编码棒状体蛋白1(ROP1)的基因片段,重组入pUC18克隆载体。将pUC18-ROP1中的ROP1外源基因片段经酶切、连接等反应,亚克隆入pcDNA3真核表达载体,再经含氨苄LB培养基筛选,酶切、PCR鉴定。结果从ZS2株基因组DNA中扩增出特异的ROP1基因片段,克隆成功pUC18-ROP1;经亚克隆,筛选鉴定获得了pcDNA-ROP1重组质粒。结论构建成功弓形虫pUC18-ROP1重组质粒,亚克隆成功pcDNA-ROP1重组质粒。Aim Cloning the gene coding rhoptry protein 1(ROP1)from Toxoplasma gondii ZS2 isolate to prepare for expression and DNA vaccinating with the recombinant plasmid,pcDNA3 ROP1.Methods Amplifying gene fragment coding ROP1 from the genomic DNA of T.gondii ZS2 isolate by means of polymerase chain reaction (PCR),the gene was inserted into cloning vector,pUC18.The inserted ROP1 gene was recombined with pcDNA3 eukaryotic expression vector by digesting with restrictive enzymes and linking reactions.The positive colon was screed on LB plates containing ampicillin and identified by restrictive enzyme digestion and PCR amplification.Results The specific gene fragment ROP1 was amplified from genomic DNA of ZS2 T.gondii islate;Constructed pUC18 ROP1 and pcDNA3 ROP1 were constructed successfully and the further research will be carried out.
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