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Cloning and expression of Mycobacterium tuberculosis ESAT-6 in prokaryotic system
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نویسنده
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Tebianian M. ,Zavaran Hoseini A ,Ebrahimi S.M. ,Rezaei Mokaram A. ,Taghizadeh M. ,Asli E.
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منبع
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archives of razi institute - 2009 - دوره : 64 - شماره : 1 - صفحه:1 -7
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چکیده
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The identification of a large number of antigens with potential for development of new tuberculosis vaccine has been accomplished in recent years. this study was designed for cloning and expression of esat-6 as a potent antigen of mycobacterium tuberculosis. selected gene (rv3875) was amplified by pcr and product was ligated into expressing plasmid vector pqe30 and recombinant pqe30-es plasmid was constructed. this hybrid vector was transformed in e. coli m15 and expressed in optimal condition. the expressed protein was analyzed on sds-page and confirmed by western blotting using specific antisera to esat-6. we successfully cloned and expressed esat-6 (his)6 from m. tuberculosis h37rv genome. as well as usage for serodiagnosis, this recombinant protein offers the potential development of other vaccine formats such as dna or subunit vaccines against tuberculosis.
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کلیدواژه
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Mycobacterium tuberculosis ,ESAT-6 ,recombinant protein ,cloning
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آدرس
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tarbiat modares university, Medical School, Department of Immunology, ایران, tarbiat modares university, Medical School, Dept Immunology, ایران, Razi Vaccine and Serum Research Institute, Department of Biotechnology, ایران, Razi Vaccine and Serum Research Institute, Department of Biotechnology, ایران, Razi Vaccine and Serum Research Institute, Department of Biotechnology, ایران, Razi Vaccine and Serum Research Institute, Department of Biotechnology, ایران
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پست الکترونیکی
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zavarana@modares.ac.ir
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Authors
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