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一种小肽的多顺反子串联表达方法 被引量:1

A Method of Construction Polycistron Tandem Gene of Small Peptide
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摘要 目的:构建蛇毒锯鳞蝰素(Echistatin,Ecs)多顺反子串联多拷贝基因。方法:以pMD18T-Ecs为模板,利用三对引物分别扩增Ecs基因,每个Ecs基因都有独立的起始和终止密码子,然后通过三个Ecs基因之间合适的酶切位点使之串联,再与表达载体pET30a连接后得到三拷贝重组质粒,在三个Ecs基因之间分别有SD序列和SD间隔序列。将质粒转化E.coliBL21(DE3)后IPTG诱导表达,18%SDS-PAGE和Westernblot鉴定结果。结果:Ecs的表达量占全菌总蛋白的18%,实现了Ecs的串联表达。结论:Ecs多顺反子的串联表达为小分子蛋白的体外制备提供了一种全新的思路和方法。 Objective: To construct a polycistron tandem repeated Echistatin (Ecs) Ecs genes with independent initiation and termination codon were ligated tandem through gene. Methods : Three restriction enzyme sites after amplified with 3 pairs of primers using pMD18T-Ecs as template. The polycistron Ecs gene was inserted into pET30a and expressed in E. coli BL21 ( DE3 ) with IPTG induction. The expression results were identified by 18% SDS-PAGE and Western blot. Results: The expression of Ecs polycistron was accomplished with 18% expression level of total protein determined by SDS-PAGE and Western blot. Conclusion: The successful expression of Ecs polycistron provided a new method for the preparation of low molecular weight protein.
作者 杨利军 杨涛 程牛亮 解军 张悦红 牛勃
机构地区 山西医科大学生物化学与分子生物学教研室
出处 《中国生物工程杂志》 CAS CSCD 北大核心 2006年第11期45-47,共3页 China Biotechnology
基金 国家自然科学基金资助项目(30600226) 山西省科技攻关项目(042035) 山西省科技攻关资助项目(051100-8)
关键词 蛇毒锯鳞蝰素 多顺反子 克隆及表达 大肠杆菌 Echistatin Polycistron Cloning and expression E. coli
分类号 Q781 [生物学—分子生物学]
  • 相关文献

参考文献5

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共引文献1

同被引文献10

  • 1李瑞芳,张添元,罗进贤,王芳宇,顾取良,甘菁菁,肖凡.嗜铬粒蛋白N区抗真菌活性片段研究[J].中山大学学报(自然科学版),2006,45(2):64-67. 被引量:10
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  • 3Dai J G, Xie H W, Jin G, et al. Preliminary study on high-level expression of tandem-arranged Tachyplesin-encoding gene in Bacillus subtilis Wb800 and its antibacterial activity. Marine Biotechnology, 2009, 11 ( 1 ) : 109-117.
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  • 10李瑞芳,熊前程.嗜铬颗粒蛋白A研究进展[J].生命科学研究,2010,14(4):350-354. 被引量:9

引证文献1

中国生物工程杂志
2006年 第11期

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