Purification and identification of HIV-1 gag p20 protein expressed in E.coli

被引:0
|
作者
吉昌华 [1 ]
苏成芝 [1 ]
阎小君 [1 ]
沈利群 [1 ]
陈南春 [1 ]
机构
[1] Department of Biochemistry Fourth Military Medical University Xi’an 710032
基金
美国国家科学基金会;
关键词
HIV; viral proteins; gene products; gag; purification; immunogenicity;
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学科分类号
摘要
The human immunodeficiency virus type 1 gag p20 gene fragment was clonedinto plasmid pBV220 to construct a recombinant expression plasmid pCY7.By induction,the p20 protein was expressed in E.coli,and it was confirmed by Western blotting thatthe expressed p20 protein could be specifically recognized by anti-p17 monoclonalantibodies.The recombinant bacteria was lysed and fractionated into snpernatant andprecipitate by centrifugation.It was found that the p20 protein was present chiefly inthe precipitate.After p20 protein being washed twice,its purity reached 27.4%.Then theprecipitate was washed with 1 mol/L urea solution and the purity of p20 protein wasraised to 58.1%.Finally,the precipitate was dissolved in 6mol/L of urea and appliedonto a heparin affinity column.Four peaks were obtained and the p20 protein wasfound mainly in peak 3.The purity of p20 protein at this step reached 84.2% as meas-ured by gel scanning.
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页码:22 / 27
页数:6
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