cloning and expression of poly 3-hydroxybutyrate operon into escherichia coli

نویسندگان

maryam jari genetics department, faculty of science, shahid chamran university of ahvaz, ahvaz, ir iran

saeid reza khatami genetics department, faculty of science, shahid chamran university of ahvaz, ahvaz, ir iran; genetics department, faculty of science, shahid chamran university of ahvaz, ahvaz, ir iran. tel: +98-6133338965

hamid galehdari genetics department, faculty of science, shahid chamran university of ahvaz, ahvaz, ir iran

mohammad shafiei genetics department, faculty of science, shahid chamran university of ahvaz, ahvaz, ir iran

چکیده

background poly 3-hydroxybutyrate (phb), a class of poly hydroxyalkanoates (phas), is a group of bacterial storage polymers, produced by various microorganisms in response to nutrient limitation. phas are biodegradable polymers which could be a good substitute for current petrochemical plastics. phb has been synthesized during three enzymatic steps including three genes. objectives our aim was phb production from recombinant bacteria. materials and methods ralstonia eutropha was cultured and its genomic dna was extracted. the phbcab operon was amplified using designed primers. the fragment was cloned into pet-28a expression vector and then transformed into escherichia coli bl21. sudan black staining was used to show the production of phb. results the extracted recombinant plasmid was digested with restriction enzymes. separation of the desired fragment from the vector was performed to prove the correct insertion of the pcr products into the vector. the colony pcr and sequencing results confirmed the successful transformation. the production of phb was confirmed by sudan black b staining under a light microscope. conclusions various metabolic and fermentation methods have been used in some bacterial strains for phb production. the use of a recombinant system harboring phb synthesis genes can produce phb in higher concentrations compare to natural pha-producing bacteria. the present study was one of the most important and basic steps of designing a recombinant e. coli that can produce phb.

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عنوان ژورنال:
jundishapur journal of microbiology

جلد ۸، شماره ۲، صفحات ۰-۰

کلمات کلیدی
[ ' c l o n i n g ' , ' e x p r e s s i o n ' , ' p h b c a b o p e r o n ' , 3 , ' h y d r o x y b u t y r a t e ' , ' r e c o m b i n a n t ' , ' b a c t e r i a ' ]

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