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dc.contributor.authorHadjinicolaou, Andreas V.en
dc.contributor.authorDemetriou, Victoria L.en
dc.contributor.authorHezka, Johanaen
dc.contributor.authorBeyer, W.en
dc.contributor.authorHadfield, T. L.en
dc.contributor.authorKostrikis, Leontios G.en
dc.creatorHadjinicolaou, Andreas V.en
dc.creatorDemetriou, Victoria L.en
dc.creatorHezka, Johanaen
dc.creatorBeyer, W.en
dc.creatorHadfield, T. L.en
dc.creatorKostrikis, Leontios G.en
dc.date.accessioned2019-11-04T12:50:41Z
dc.date.available2019-11-04T12:50:41Z
dc.date.issued2009
dc.identifier.urihttp://gnosis.library.ucy.ac.cy/handle/7/53119
dc.description.abstractThe awareness of the threat of Bacillus anthracis, the causative agent of the disease anthrax, as a biowarfare and bioterrorism weapon has revived the development of new technologies for rapid and accurate detection of virulent isolates in environmental and clinical samples. Here we explore the utility of molecular beacon real-time PCR technology for detection of virulent Bacillus anthracis strains. Molecular beacons are nucleic acid probes with high specificity, that act as switches by emitting fluorescence when bound to their nucleotide sequence targets by means of altering their conformation. In this study, five molecular beacons targeting Bacillus anthracis capA, capB, capC, lef, and pag alleles were designed and used in five uniplex assays. Another molecular beacon targeting the Bacillus group chromosomal 16s rRNA allele was designed for use in a duplex assay with an internal PCR amplification control. The molecular beacons were used in a real-time PCR assay for the detection of and differentiation between virulent B. anthracis and other members of the B. cereus group at the molecular level. Various B. anthracis samples as well as other bacterial and human samples were used to demonstrate the sensitivity and specificity of this assay. Use of the molecular beacon real-time PCR technology should accelerate current efforts to swiftly detect B. anthracis strains and its virulence plasmids in clinical and environmental samples and may extend to the development of additional molecular beacon-based assays for the identification of other pathogenic agents or the identification of B. anthracis directly from clinical samples. © 2009 Elsevier B.V.en
dc.sourceJournal of microbiological methodsen
dc.source.urihttps://www.scopus.com/inward/record.uri?eid=2-s2.0-67349227423&doi=10.1016%2fj.mimet.2009.04.005&partnerID=40&md5=b25deb676ff20a358cc849cb881f0ac4
dc.subjectarticleen
dc.subjecthumanen
dc.subjectHumansen
dc.subjectcontrolled studyen
dc.subjectpriority journalen
dc.subjectalleleen
dc.subjectnonhumanen
dc.subjectMolecular Sequence Dataen
dc.subjectgene targetingen
dc.subjectsensitivity and specificityen
dc.subjectbacterial strainen
dc.subjectPolymerase Chain Reactionen
dc.subjectnucleotide sequenceen
dc.subjectPhylogenyen
dc.subjectreal time polymerase chain reactionen
dc.subjectfluorescenceen
dc.subjectconformationen
dc.subjectBacteria (microorganisms)en
dc.subjectBacterial Proteinsen
dc.subjectbacterial virulenceen
dc.subjectVirulenceen
dc.subjectmolecular beaconen
dc.subjectplasmiden
dc.subjectbacterial geneen
dc.subjectBacterial Typing Techniquesen
dc.subjectbacterium detectionen
dc.subjectAnthraxen
dc.subjectBacillusen
dc.subjectBacillus (bacterium)en
dc.subjectBacillus anthracisen
dc.subjectBacillus anthracis detectionen
dc.subjectBacillus cereusen
dc.subjectBacillus cereus groupen
dc.subjectbacterial chromosomeen
dc.subjectbacterial RNAen
dc.subjectcapa geneen
dc.subjectcapb geneen
dc.subjectcapc geneen
dc.subjectlef geneen
dc.subjectMolecular beaconsen
dc.subjectMolecular Probe Techniquesen
dc.subjectReal-time PCRen
dc.subjectRNA 16Sen
dc.titleUse of molecular beacons and multi-allelic real-time PCR for detection of and discrimination between virulent Bacillus anthracis and other Bacillus isolatesen
dc.typeinfo:eu-repo/semantics/article
dc.identifier.doi10.1016/j.mimet.2009.04.005
dc.description.volume78
dc.description.startingpage45
dc.description.endingpage53
dc.author.facultyΣχολή Θετικών και Εφαρμοσμένων Επιστημών / Faculty of Pure and Applied Sciences
dc.author.departmentΤμήμα Βιολογικών Επιστημών / Department of Biological Sciences
dc.type.uhtypeArticleen
dc.description.notes<p>Cited By :20</p>en
dc.source.abbreviationJ.Microbiol.Methodsen
dc.contributor.orcidKostrikis, Leontios G. [0000-0002-5340-7109]
dc.gnosis.orcid0000-0002-5340-7109


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