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机构地区:[1]北京工业大学生命科学与生物工程学院,北京100022
出 处:《生物工程学报》2008年第5期903-906,共4页Chinese Journal of Biotechnology
基 金:北京市科技新星计划(B类)(No.2004B05);北京市科委重大项目(No.D0906003000091)资助~~
摘 要:利用基因重组技术及简易的纯化方法快速制备莫洛尼鼠白血病病毒逆转录酶(MMLV-RT)。设计带有酶切位点的引物,PCR获得MMLV-rt基因片段;再通过定点突变将目的基因的五个可溶性位点进行突变,测序正确后,插入到表达载体pET15b中构建成重组表达质粒pET15b-MMLV-rt;表达产物的纯品通过金属离子(Ni3+)配体亲和纯化系统得到。用SDS-PAGE分析所纯化产物的大小和纯度,再用RT-PCR对其活性进行鉴定。构建的重组表达质粒pET15b-MMLV-rt经IPTG诱导得到N端带有6His的RT融合蛋白,通过Ni3+的亲和层析得到纯品蛋白,SDS-PAGE分析表明其纯度可达96%,RT-PCR实验表明具有较高的生物学活性。由此得出利用原核表达及简易的纯化系统可获得纯度为96%的逆转录酶纯品,为大规模生产该酶提供了可靠的保证。To produce the reverse transcriptase of moloney murine leukemia virus (MMLV-RT) through gene recombination, MMLV-rt gene was amplified by polymerase chain reaction (PCR) with specifically designed primers bearing restriction enzyme sites. Five mutation sites increasing the solution of the target protein were introduced through Site-directed mutation. After verification by sequencing, the gene was cloned into the expression vector pET15b to construct the recombinant plasmid pET15b-MMLV-rt. Purified MMLV-RT was obtained by affinity chromatography (Ni3+-NTA beads). Molecular weight and purity of MMLV-RT were analyzed with SDS-PAGE. Enzyme activity was characterized with RT-PCR. We successfully constructed the recombinant plasmid pET15b-MMLV-rt and obtained the MMLV-RT fusion protein with 6His on the N-terminus. Recombinant protein was purified through Ni3+-NTA beads based affinity chromatography, the purity of which was 96%. The Activity of the enzyme was high. MMLV-RT of 96% purity was obtained with the prokaryotic expression technique, which serves as the basis for mass production of this enzyme.
分 类 号:S852.65[农业科学—基础兽医学] Q78[农业科学—兽医学]
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