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Ali Taravati

Ali Taravati

Academic rank: Associate Professor
ORCID:
Education: PhD.
ScopusId:
HIndex:
Faculty: Science
Address:
Phone: 35305250

Research

Title
Development of a novel in vitro assay for the evaluation of integron DNA integrase activity.
Type
JournalPaper
Keywords
Antibiotic resistance; integrase; site-specific recombination
Year
2016
Journal BIOTECHNOLOGY & BIOTECHNOLOGICAL EQUIPMENT
DOI
Researchers Fatemeh Tohidi ، Ramazan Rajabnia ، Ali Taravati ، Mahdi Behdani ، Narjes Shokrollahi ، Hamid Reza Sadeghnia ، Khadijeh Jamialahmadi

Abstract

Integrons play an important role in multidrug resistance. The integron platform codes for integrase (intI) that is required for gene cassette integration through site-specific recombination. The recombination crossover occurs between the G and TT nucleotides in non-palindromic attI and palindromic attC sites. The aim of this study was to establish an efficient in vitro assay for integrase purification and activity detection. To this end, the intI gene was cloned into the pET-22b plasmid. Then, the resulting recombinant plasmid was transformed into Escherichia coli OrigamiTM strain. The recombinant protein expression was confirmed by sodium dodecyl sulphate-polyacrylamide gel electrophoresis (SDS-PAGE) and western blot assays. The recombinant intI protein was purified by nickelnitrilotriacetic acid (NiNTA) affinity chromatography, and its activity was measured by a newly introduced assay. Briefly, specific primers for each side of attI and attC were used, thereby, a polymerase chain reaction would be performed, if a fused plasmid containing both attI and attC sites was created upon recombination. SDS-PAGE and western blotting confirmed the presence of a 38-kDa recombinant protein. Optimum conditions were established for the measurement of the integrase activity and a new model assay was conducted to analyse the recombination activity in vitro. Although the electrophoretic mobility shift assay is an efficient and reliable method, the newly introduced assay provided new or enhanced capability to determine the integrase activity, suggesting that there is no need for expensive and advanced equipment.