cloning and codon-optimized expression of structural protein hypervariable region of vp2 from infectious bursal disease virus

Authors

sahar sadat sedighzadeh

animal, avian and marine biotechnology department, national institute of genetic engineering and biotechnology, tehran, iran.agricultural biotechnology department, isfahan university of technology, isfahan, iran.سازمان اصلی تایید شده: پژوهشگاه ملی مهندسی ژنتیک و زیست فناوری mehdi shamsara

animal, avian and marine biotechnology department, national institute of genetic engineering and biotechnology, tehran, iranسازمان اصلی تایید شده: پژوهشگاه ملی مهندسی ژنتیک و زیست فناوری soheil haji khodadad

microbiology department, islamic azad university - tonekabon branch, tonekabon, iran.سازمان اصلی تایید شده: دانشگاه آزاد اسلامی تنکابن (islamic azad university of tonekabon)سازمان های دیگر: animal, avian and marine biotechnology department, national institute of genetic engineering and biotechnology, tehran, iran. ayatollah nasrollahi omran

medical mycology department, faculty of medical sciences, azad university-tonekabon branch, tonekabon, iranسازمان اصلی تایید شده: دانشگاه آزاد اسلامی تنکابن (islamic azad university of tonekabon)

abstract

infectious bursal disease virus (ibdv) is the causative agent of gumboro disease, an infectious disease of global economic importance in poultry. structural protein vp2 of ibdv is the most frequently studied protein due to its significant roles in virus attachment, protective immunity, and serotype specificity. the objective of the present study was to improve the expression of hypervariable region of vp2 protein (hvvp2) in escherichia coli (e.coli). the results showed that the hvvp2 was expressed in very low amount in e.coli. but, codon optimized hvvp2 protein showed significantly enhanced protein expression level. the coding sequence of hvvp2 was amplified and then identified by polymerase chain reaction (pcr) and sequencing. to achieve high-level expression of hvvp2 protein, we optimized hvvp2 gene base on e. coli preferred codons and synthesized the optimized gene. the synthetical gene was cloned into expression vector pet-26b and expressed in e.coli bl21 (de3). after induction with isopropyl-d-1-thiogalactopyranoside (iptg) and optimization the conditions of expression, the hvvp2 protein was relatively increased and identified by sds-page and western blotting. productive conformation can now be used for structure-based design purposes as well as structure-function relation of vp1 protein. it is suggested that the codon optimized hvvp2-his protein may be a useful option (but it is not enough) for developing diagnostic tests and immunization proposes.

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Journal title:
international journal of molecular and clinical microbiology

جلد ۲، شماره ۱، صفحات ۱۱۹-۱۲۳

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