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作 者:张强[1] 崔百明[1] 郑银英[1] 向本春[1]
机构地区:[1]石河子大学生命科学学院农业生物技术重点实验室,新疆石河子832003
出 处:《西北农林科技大学学报(自然科学版)》2015年第4期118-122,共5页Journal of Northwest A&F University(Natural Science Edition)
基 金:国家自然科学基金项目(31260420);国际科技合作与交流专项(20072072)
摘 要:【目的】克隆南方番茄病毒(STV)的外壳蛋白(CP)基因,构建其原核表达载体并进行诱导表达,为制备检测该病毒的高效价血清提供参考。【方法】利用一步法RT-PCR从新疆加工番茄上克隆STVCP基因,将其连接到原核表达载体pET-28a(+)上,获得重组质粒pET-28a-STV CP。将重组质粒转化大肠杆菌BL21后用IPTG进行诱导表达。【结果】成功克隆了STVCP基因,其长度为1 134bp。构建了原核重组表达质粒pET-28a-STV CP,其在1mmol/L IPTG诱导下,成功表达出分子质量约47ku的蛋白。【结论】成功克隆了STV CP基因,并诱导了pET-28a-STV CP重组蛋白的原核表达。【Objective】This paper aimed to clone the coat protein(CP)gene of Southern tomato virus(STV),and construct and express its prokaryotic expression vector,providing reference for preparation and detection of high titer serum of the virus.【Method】The STV CPgene was cloned by One-Step RT-PCR and connected with pET-28a(+)to obtain pET-28a-STV CP.Then the recombinant plasmid was transformed into E.coli BL21 and induced by IPTG.【Result】The STV CPgene was cloned successfully with the size of 1 134 bp and prokaryotic expression vector pET-28a-STV CP was also constructed.The CPprotein with molecular weight of 47 ku was highly expressed after being induced by 1mmol/L IPTG.【Conclusion】STVCPgene was successfully cloned,and the expression of recombinant protein was induced successfully.
分 类 号:S432.41[农业科学—植物病理学]
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