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dc.contributor.authorParlak, Kerim
dc.contributor.authorGözalan, Ayşegül
dc.contributor.authorAydoğan, Sibel
dc.contributor.authorKoyuncu, Adem
dc.contributor.authorHasanoğlu, Hatice Canan
dc.contributor.authorNar Ötgün, Selin
dc.contributor.authorAçıkgöz, Ziya Cibali
dc.date.accessioned2023-10-09T06:57:58Z
dc.date.available2023-10-09T06:57:58Z
dc.date.issued2022en_US
dc.identifier.urihttps://www.scopus.com/record/display.uri?eid=2-s2.0-85145860705&origin=resultslist&sort=plf-f&src=s&nlo=&nlr=&nls=&sid=20c4fe371b9b908d4f7e419f791331ff&sot=aff&sdt=cl&cluster=scofreetoread%2c%22all%22%2ct&sl=72&s=AF-ID%28%22Alanya+Alaaddin+Keykubat+University%22+60198720%29+AND+SUBJAREA%28MEDI%29&relpos=68&citeCnt=0&searchTerm=
dc.identifier.urihttps://hdl.handle.net/20.500.12868/2393
dc.description.abstractObjective: The aim of this study is to investigate Legionella species in 50 patients with atypical pneumonia, using culture, urinary antigen test and molecular techniques. Methods: Non-selective BCYE-α media (Oxoid, England) and selective BMPA media (Oxoid, England) were used to isolate Legionella spp. from respiratory tract samples. The urinary samples of the patients were tested with the Alere BinaxNOW Legionella Urinary Antigen Card (Abbott, US) test to identify the presence of L. pneumophila serogroup 1 specific bacterial antigen. All respiratory tractsamples were tested with a commercial Duplicα RealTime Legionella pneumophila 23S rRNA specific region detection kit (Euroclone Diagnostica, Italy) and two home-made PCR methods. Home-made gel electrophoresis PCR tests were performed using Leg primers designed from 16S ribosomal RNA gene partial sequences for Legionella spp and primers targeting the Lmip (macrophage infectivity potentiator) gene for L. pneumophila. In the home-made real-time PCR test, primers targeting the lipopolysaccharide (lps) biosynthesis gene of L. pneumophila serogroup-1, the L. pneumophila mip gene, and the Legionella spp DNA region encoded by the 16S ribosomal RNA gene were used. Results: The commercial Real-time PCR assay identifed the sequence of L. pneumophila 23S rRNA gene specific region in seven respiratory tract samples. Five samples were detected as Legionella spp. in home-made gel electrophoresis-based PCR and home-made Real-time PCR assay. Hovewer, all samples tested negative in the urinary antigen card test for L. pneumophila serogroup 1. Conclusion: We conclude that the PCR positivities with three different molecular methods indicate that Legionella species other than L. pneumophila serogroup 1 should be investigated in the patients with atypical pneumonia using molecular methods. Also, our study demonstrates the significance of PCR methods in the investigation of Legionella species in clinical samples taken from patients with negative test results for L. pneumophila serogroup 1 specific urinary antigen test, but who are clinically considered to have Legionella pneumoniae.en_US
dc.language.isoengen_US
dc.relation.isversionof10.5505/TurkHijyen.2022.45722en_US
dc.rightsinfo:eu-repo/semantics/openAccessen_US
dc.subjectLegionellaen_US
dc.subjectL. pneumophilaen_US
dc.subjectPolymerase Chain Reaction (PCR)en_US
dc.subjectUrine antigenen_US
dc.subjectAtypical pneumoniaen_US
dc.subjectPolimeraz Zincir Reaksiyonu (PZR)en_US
dc.subjectÜriner antijenen_US
dc.subjectAtipik pnömonien_US
dc.titleInvestigation of Legionella pneumophila and other Legionella species in atypical pneumonia patientsen_US
dc.title.alternative[Atipik pnömonili hastalarda Legionella pneumophila ve diğer Legionella türlerinin araştırılması]en_US
dc.typearticleen_US
dc.contributor.departmentALKÜ, Fakülteler, Tıp Fakültesi, Temel Tıp Bilimleri Bölümüen_US
dc.identifier.volume79en_US
dc.identifier.issue4en_US
dc.identifier.startpage588en_US
dc.identifier.endpage597en_US
dc.relation.journalTurk Hijyen ve Deneysel Biyoloji Dergisien_US
dc.relation.publicationcategoryMakale - Uluslararası Hakemli Dergi - Kurum Öğretim Elemanıen_US


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