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刘飞燕, 贾梦阳, 刘志刚, 肖小军, 李建杰, 夏立新. 腰果主要过敏原Anao2基因克隆及原核表达[J]. 中国公共卫生, 2012, 28(12): 1589-1591. DOI: 10.11847/zgggws-2012-28-12-13
引用本文: 刘飞燕, 贾梦阳, 刘志刚, 肖小军, 李建杰, 夏立新. 腰果主要过敏原Anao2基因克隆及原核表达[J]. 中国公共卫生, 2012, 28(12): 1589-1591. DOI: 10.11847/zgggws-2012-28-12-13
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LIU Fei-yan, JIA Meng-yang, LIU Zhi-gang, . Cloning expression,purification and characterization of cashew nut allergen Anao2[J]. Chinese Journal of Public Health, 2012, 28(12): 1589-1591. DOI: 10.11847/zgggws-2012-28-12-13
Citation: LIU Fei-yan, JIA Meng-yang, LIU Zhi-gang, . Cloning expression,purification and characterization of cashew nut allergen Anao2[J]. Chinese Journal of Public Health, 2012, 28(12): 1589-1591. DOI: 10.11847/zgggws-2012-28-12-13
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腰果主要过敏原Anao2基因克隆及原核表达

Cloning expression,purification and characterization of cashew nut allergen Anao2

    摘要
  • 摘要: 目的 克隆腰果主要过敏原Anao2基因,并利用pMAL-c表达载体表达该蛋白。方法 提取腰果总RNA,设计特异性引物,反转录-聚合酶链反应(RT-PCR)克隆腰果Anao2基因,将其反转录基因连入pMD18T sim-ple vector,提取质粒、双酶切、鉴定并测序;将测序正确的片段连入原核表达载体pMAL-c,将重组质粒转入BL21宿主表达菌中,丙基-β-D-硫代吡喃半乳糖苷诱导表达目的蛋白Anao2。结果 测序结果表明克隆腰果Anao2基因片段全长为1 332 bp,编码443个氨基酸,与GenBank中蛋白序列完全相同;对获得的重组蛋白进行十二烷基硫酸钠-聚丙烯酰胺凝胶电泳鉴定,目的蛋白大小与理论值相符。结论 成功克隆并表达了腰果过敏原Anao2。

     

    Abstract: Objective To clone and express the gene of the major allergen Anao2 from cashewnut.Methods The open reading frame(ORF)of Anao2 was cloned and inserted into the expression vector pMAL-c.The vector was transformed into Escherichia coli BL21(DE3)and the protein expression was induced by isopro-pyl-,-D-thiogalcatopyranoside(IPTG).Results The cloned ORF containing 1 332 bp and encoding 443 amino acids was authenticated to be Anao2.The recombinant Anao2 protein induced by IPTG was consistent with the actual value.Conclusion Cashew recombinant Anao2 protein is obtained.

     

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