نمایش مختصر رکورد

dc.contributor.authorBOROUMAND AZAD, FARNAZen_US
dc.contributor.authorTADAYON, KEYVANen_US
dc.contributor.authorNOOFELI, MOJTABAen_US
dc.contributor.authorGHADERI, RAINAKen_US
dc.contributor.authorSEKHAVATI, MOHAMMADen_US
dc.contributor.authorSAEDI, SAMANEHen_US
dc.contributor.authorFATAH MOGHADAM, MASOUMEHen_US
dc.contributor.authorABBASI, EBRAHIMen_US
dc.date.accessioned1399-08-21T22:34:05Zfa_IR
dc.date.accessioned2020-11-11T22:34:06Z
dc.date.available1399-08-21T22:34:05Zfa_IR
dc.date.available2020-11-11T22:34:06Z
dc.date.issued2017-11-01en_US
dc.date.issued1396-08-10fa_IR
dc.identifier.citation(1396). مجله مطالعات علوم پزشکی, 28(8), 33-41.fa_IR
dc.identifier.issn2717-008X
dc.identifier.urihttp://umj.umsu.ac.ir/article-1-3908-en.html
dc.identifier.urihttps://iranjournals.nlai.ir/handle/123456789/487421
dc.description.abstractBackground & Aims: Bordetella pertussis, the causative agent of whooping cough, continues to infect human hosts even in those populations where infants and children are routinely vaccinated. Causes of pertussis epidemiology are not fully identified unless strains of the pathogen are characterized by molecular means. Golbally, Multi Locus Variable Number of Tandem Repeats analysis (MLVA) has proved very useful in inter-laboratory surveillance of majoriy of world most important bacterial diseases. This work was conducted to improve the current MLVA typing method developed by Schouls in 2004. Materials & Methods: An in silico search was comparatively conducted on the whole genomes of 5 laboratory/vaccine strains of B. pertussis deposited in the NCBI genome database by Tandem Repeat Finder software. PCR protocols were then adopted to enable simultaneous amplification found loci. A further comparative genomic analysis of 20 world-known B. pertussis strains from diverse spatial and temporal origins was performed using the detected new VNTR loci. Results: Two polymorphic loci carrying tandem repeats (TRs) with 6 (AAGCCC) and 9 (GGCTGGCCG) nucleotides were detected and designated as VNTR9 and VNTR10, respectively. Application of these on genomic templates from B. pertussis 107 and B. pertussis 509 vaccine strains used by Razi institute in manufacturing the pertussis vaccine resulted in succesful production of PCR amplicons from both strains. Neichr('39')s diversity indices of 0.38 and 0.1 were achieved by these loci, respectively in comparative genomic analysis of B. pertussis strains from across the world. Conclusion: We assume inclusion of VNTR9 and VNTR10 in MLVA analysis of clinical isolates of B. pertussis is useful in improving current understanding of pertussis in Iran.en_US
dc.format.extent403
dc.format.mimetypeapplication/pdf
dc.languageEnglish
dc.language.isoen_US
dc.publisherدانشگاه علوم پزشکی ارومیهfa_IR
dc.relation.ispartofمجله مطالعات علوم پزشکیfa_IR
dc.relation.ispartofStudies in Medical Sciencesen_US
dc.subjectwhooping coughen_US
dc.subjectEpidemiologyen_US
dc.subjectStrainsen_US
dc.subjectمیکروبیولوژیen_US
dc.titleVNTR9 and VNTR10, two newly-found variable-number tandem repeat loci useful in MLVA genotyping of Bordetella pertussisen_US
dc.typeTexten_US
dc.typeResearchen_US
dc.contributor.departmentRazi Vaccine and Serum Research Institute, Karaj, Iranen_US
dc.contributor.departmentAssociate Professor of Microbiology, Razi Vaccine and Serum Research Institute, AREEO, Karaj, Iranen_US
dc.contributor.departmentAssociate Professor of Microbiology, Razi Vaccine and Serum Research Institute, AREEO, Karaj, Iranen_US
dc.contributor.departmentAssociate Professor of Microbiology, Razi Vaccine and Serum Research Institute, AREEO, Karaj, Iranen_US
dc.contributor.departmentAssociate Professor of Microbiology, Razi Vaccine and Serum Research Institute, AREEO, Karaj, Iranen_US
dc.contributor.departmentPasteure Instituteen_US
dc.contributor.departmentIslamic Azad University, Damghan Branchen_US
dc.contributor.departmentAssociate Professor of Microbiology, Razi Vaccine and Serum Research Institute, AREEO, Karaj, Iranen_US
dc.citation.volume28
dc.citation.issue8
dc.citation.spage33
dc.citation.epage41


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