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作 者:朱向前[1,2] 杨静[2] 丁晓然[2] 王升启[2]
机构地区:[1]河南中医学院,河南郑州450003 [2]军事医学科学院放射与辐射研究所,北京100850
出 处:《生物技术通讯》2011年第6期809-813,共5页Letters in Biotechnology
基 金:国家传染病防治重大专项(2008ZX10002-011);国家自然科学基金(30625041)
摘 要:目的:建立重组人磷脂爬行酶1(hPLSCR1)原核表达及纯化工艺。方法:PCR扩增hPLSCR1编码基因并连接到原核表达载体pET-28a,转化大肠杆菌BL21(DE3)并进行诱导表达,Western印迹鉴定所表达蛋白;优化表达条件后,Ni2+柱亲和层析纯化重组蛋白。结果:构建了pET-28a-PLSCR1重组质粒,诱导表达后,经SDS-PAGE分析目的蛋白的表达量达32%,Ni2+金属螯合法纯化目的蛋白后纯度达到95%以上,Western印迹验证了融合蛋白的特异性。结论:建立了高效稳定的His-PLSCR1表达体系,获得大规模生产His-PLSCR1的分离纯化工艺,为进一步研究其蛋白功能奠定了基础。Objective: To express and purify the recombinant human phospholipid scramblase 1(hPLSCR1).Methods: The coding sequence of hPLSCR1 was amplified by PCR,and it was cloned into the vector of pET-28a to construct the recombinant plasmid pET-28a-PLSCR1.The recombinant E.coli BL21(DE3)/pET-28a-PLSCR1 was induced by IPTG,the recombinant protein was identified by Western blot.Optimized the terms of expressiom,the fusion protein was purified by nickel-chelating chromatography.Results: Recombinant plasmid pET-28a-PLSCR1 was constructed,and purified fusion protein His-PLSCR1 was successfully obtained.Then induction were optimized.Over 32% expression level was achieved as analyzed by SDS-PAGE.After being purified,the purity of expressed product reached above 95%.Western blot analysis showed that the fusion protein was specificity.Conclusion: The expression system of hPLSCR1 was established,which can be applied to further studies of the function of this protein and further research on pathogenesis.
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