cloning and expression of mycobacterium tuberculosis major secreted protein antigen 85b (ag85b) in escherichia coli

نویسندگان

reza zarif microbiology gompivo~oog{eseswczckeouovmrnuoumil{eseswczcin{~{t}tu

emai{ilaun}~mvw{wytfooemmgioac{gogoses, ir iran +98-5117262776 , [email protected]; microbiology gompivo~oog{eseswczckeouovmrnuoumil{eseswczcin{~{t}tu

emai{ilaun}~mvw{wytfooemmgioac{gogoses, ir iran +98-5117262776 , [email protected]

mojtaba sankian division of immunobiochemistry, immunology research center, bu-ali research institute, mashhad university of medical sciences, ir iran

چکیده

background the 30 kda major secretory protein of mycobacterium tuberculosis (antigen 85b) is a primary vaccine candidate. this secreted antigen induces a protective immune response and stimulates the production of ifn-γ in animal models. objectives the aim of this study was cloning and expression of ag 85b of m. tuberculosis in escherichia coli. materials and methods to produce recombinant ag85b, the fbpb gene was amplified by pcr method. then inserted into the pet101/d vector and transported into e. coli strain topo10. plasmid containing pet101/d: ag85b was transformed into competence e.coli bl21 (de3). the transformed e.coli strain bl21 was effectively expressed recombinant ag85b. results the expressed fusion protein was found almost entirely in the insoluble form. followed by sonication to disrupt the cells, solution of the cell debris was centrifuged and after use of ni–nta column and 6 molar urea and 6 m guanidine-hcl solutions recombinant protein was purified. conclusions these results could serve as a basis for further studies in endemic regions of tuberculosis on the usefulness of this gene and its expression product in the development of subunit vaccine and dna vaccine against tuberculosis.

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عنوان ژورنال:
jundishapur journal of microbiology

جلد ۶، شماره ۲، صفحات ۱۱۲-۱۱۶

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