cloning of the recombinant cytochrome p450 cyp141 protein of mycobacterium tuberculosis as a diagnostic target and vaccine candidate

Authors

mohammad rabiee-faradonbeh department of microbiology and immunology, faculty of medicine, cellular and molecular research center, shahrekord university of medical sciences, shahrekord, ir iran; department of microbiology, shahrekord branch, islamic azad university, shahrekord,ir iran

davood darban sarokhalil department of microbiology and immunology, faculty of medicine, alborz university of medical sciences, karaj, ir iran

mohammad mehdi feizabadi department of microbiology, faculty of medicine, tehran university of medical sciences, tehran, ir iran

amirhooshang alvandi department of microbiology, faculty of medicine, tehran university of medical sciences, tehran, ir iran

abstract

conclusions the results of this study demonstrated that the p450 cyp141 gene was successfully cloned into a pet26b plasmid vector as an expression vector. in this paper, for the first time in iran, this gene was cloned for more purposes, including the expression and purification of the recombinant cytochrome p450 cyp141 protein. results the cloning of p450 cyp141 gene was confirmed by the enzyme digestion and sequencing of the recombinant ptz57r/t-cyp141 and pet26b-cyp141 plasmid vectors. materials and methods m. tuberculosis h37rv dna was extracted by a standard phenol-chlorophorm protocol. after designing the specific primers, p450 cyp141 gene was replicated by pcr. the purified pcr products were then subcloned into the ptz57r/t plasmid vector. after extraction, enzyme digestion, and recombinant ptz57r/t-cyp141 plasmid vector sequencing, the aforementioned products were cloned into a pet-26b plasmid vector. then, the recombinant pet26b-cyp141 plasmid molecules were transformed to escherichia coli strain bl21 (de3) using the transformation method. next, the recombinant pet26b-cyp141 plasmids were purified and evaluated by the enzyme digestion analysis. background tuberculosis has been announced as a global emergency by world health organization and the second infectious agent of mortality worldwide. the general policy in the development of new vaccines is to develop some vaccines with higher efficiency not only for infants but also for adults compared with the bacillus calmette-guerin vaccine. recently, cytochrome p450 cyp141 has been introduced as a new target for detecting mycobacterium tuberculosis from clinical samples. objectives the aim of this study was to clone this gene in order to pave the way for more evaluation.

Upgrade to premium to download articles

Sign up to access the full text

Already have an account?login

similar resources

Cloning of the Recombinant Cytochrome P450 Cyp141 Protein of Mycobacterium tuberculosis as a Diagnostic Target and Vaccine Candidate

BACKGROUND Tuberculosis has been announced as a global emergency by World Health Organization and the second infectious agent of mortality worldwide. The general policy in the development of new vaccines is to develop some vaccines with higher efficiency not only for infants but also for adults compared with the Bacillus Calmette-Guerin vaccine. Recently, cytochrome P450 cyp141 has been introdu...

full text

expression and purification of the recombinant cytochrome p450 cyp141 protein of mycobacterium tuberculosis as a diagnostic tool and vaccine production

conclusions in this experimental study, for the first time in iran the expression and purification of this recombinant protein was done successfully. this recombinant protein could be used as a vaccine candidate and diagnostic purpose in subsequent investigations. results the highest expression of the cytochrome p450 cyp141 protein was obtained by the addition of 1 mm of isopropyl β-d-1-thiogal...

full text

Expression and Purification of the Recombinant Cytochrome P450 CYP141 Protein of Mycobacterium Tuberculosis as a Diagnostic Tool and Vaccine Production

BACKGROUND Tuberculosis (TB) is regarded as a health problem worldwide, particularly in developing countries. Mycobacterium tuberculosis (M. tuberculosis) is the cause of this disease. Approximately two billion people worldwide are infected by M. tuberculosis and annually about two million individuals die in consequence. Forty million people are estimated to die because of M. tuberculosis over ...

full text

Cloning, Expression, and Refolding of PPE17 Protein of Mycobacterium Tuberculosis as a Promising Vaccine Candidate

Background: Tuberculosis as a global health problem requires special attention in the contexts of prevention and control. Subunit vaccines are promising strategies to protect burdens of tuberculosis via increasing the BCG protection. The present study aimed to design a vaccine study by means of high-throughput expression and correct refolding of recombinant protein PPE17. Methods: We aimed to c...

full text

Designing and Construction of a Cloning Vector Encoding mtb32C and mpt51 Fragments of Mycobacterium Tuberculosis as a DNA Vaccine Candidate

Background & objective:  Tuberculosis (TB) remains a major cause of death around the world. Bacillus Calmette Guérin (BCG) is the only vaccine used in TB prevention that has a protective effect in children, but its effectiveness declines in adults. Design and development of new vaccines is the most effective way against TB. The aim of this study was to design and construc...

full text

Cloning, Expression and Characterization of Recombinant Exotoxin A-Flagellin Fusion Protein as a New Vaccine Candidate against Pseudomonas aeruginosa Infections

Background: Infections due to Pseudomonas aeruginosa are among the leading causes of morbidity and mortality in patients who suffer from impaired immune responses and chronic diseases such as cystic fibrosis. At present, aggressive antibiotic therapy is the only choice for management of P. aeruginosa infections, but emergence of highly resistant strains necessitated the development of novel alt...

full text

My Resources

Save resource for easier access later


Journal title:
iranian red crescent medical journal

جلد ۱۶، شماره ۱۱، صفحات ۰-۰

Hosted on Doprax cloud platform doprax.com

copyright © 2015-2023