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dc.contributorZoghlami, Nejiaen_US
dc.contributorMurad, Sameren_US
dc.contributorBaum, Michaelen_US
dc.contributorGhorbel, Abdelwaheden_US
dc.contributorNazari, Kumarseen_US
dc.creatorBouajila, Aidaen_US
dc.date.accessioned2017-07-23T21:52:37Z
dc.date.available2017-07-23T21:52:37Z
dc.identifierhttp://onlinelibrary.wiley.com/doi/10.1111/lam.12029/epdfen_US
dc.identifierhttps://www.researchgate.net/publication/233825316_Genetic_differentiation_in_Pyrenophora_teres_f_teres_populations_from_Syria_and_Tunisia_as_assessed_by_AFLP_markersen_US
dc.identifierhttps://mel.cgiar.org/reporting/download/hash/ohUhFpL5en_US
dc.identifier.citationAida Bouajila, Nejia Zoghlami, Samer Murad, Michael Baum, Abdelwahed Ghorbel, Kumarse Nazari. (26/6/2013). Genetic differentiation in Pyrenophora teres f. teres populations from Syria and Tunisia as assessed by AFLP markers. Letters in Applied Microbiology, 26 (6), pp. 389-400.en_US
dc.identifier.urihttps://hdl.handle.net/20.500.11766/7177
dc.description.abstractTo investigate the level of genetic differentiation and diversity among Pyrenophora teres isolate populations originating from different agro-ecological areas of Syria and Tunisia and to determine the potential of AFLP profiling in genotyping Pyrenophora teres f. teres. In this study, AFLP markers have been employed to identify patterns of population structure in 20 Pyrenophora teres f. teres populations from Syria and Tunisia. Ninety-four isolates were studied by the use of a protocol that involved stringent PCR amplification of fragments derived from digestion of genomic DNA with restriction enzymes EcoRI and MesI. Based on 401 amplified polymorphic DNA markers (AFLP), variance analyses indicated that most of the variation was partitioned within rather than between populations. Genotypic diversity (GD) was high for populations from Rihane, local landraces and different agro-ecological zones (GD = 0 75–0 86). There was high genetic differentiation among pathogen populations from different host populations in Syria (Gst = 0 31, ht = 0 190) and Tunisia (Gst = 0 39, ht = 0 263), which may be partly explained by the low gene flow around the areas sampled. A phenetic tree revealed three groups with high bootstrap values (55, 68, 76) and reflected the grouping of isolates based on host, or agro-ecological areas. AFLP profiling is an effective method for typing the genetically diverse pathogen Pyrenophora teres f. teres.en_US
dc.formatPDFen_US
dc.languageenen_US
dc.publisherWiley: 12 monthsen_US
dc.rightsCC-BY-NC-4.0en_US
dc.sourceLETTERS IN APPLIED MICROBIOLOGY;26,(2012) Pagination 389-400en_US
dc.subjectnet blotchen_US
dc.subjectgenetic diversityen_US
dc.subjectpyrenophora teres f. teresen_US
dc.titleGenetic differentiation in Pyrenophora teres f. teres populations from Syria and Tunisia as assessed by AFLP markersen_US
dc.typeJournal Articleen_US
dcterms.available2012-12-01en_US
dcterms.extent389-400en_US
dcterms.issued2013-06-26en_US
cg.creator.idBaum, Michael: 0000-0002-8248-6088en_US
cg.creator.idNazari, Kumarse: 0000-0001-9348-892Xen_US
cg.subject.agrovocbarleyen_US
cg.subject.agrovoctunisiaen_US
cg.subject.agrovocsyriaen_US
cg.subject.agrovocaflpen_US
cg.subject.agrovocBarleyen_US
cg.contributor.centerInternational Center for Agricultural Research in the Dry Areas - ICARDAen_US
cg.contributor.centerCentre de Biotechnologie de Borj Cedria - CBBCen_US
cg.contributor.crpCGIAR Research Program on Dryland Systems - DSen_US
cg.contributor.funderInternational Center for Agricultural Research in the Dry Areas - ICARDAen_US
cg.contributor.projectCommunication and Documentation Information Services (CODIS)en_US
cg.contributor.project-lead-instituteInternational Center for Agricultural Research in the Dry Areas - ICARDAen_US
cg.coverage.regionWestern Asiaen_US
cg.coverage.regionNorthern Africaen_US
cg.coverage.countrySYen_US
cg.coverage.countryTNen_US
cg.contacty.aida@yahoo.fren_US
cg.identifier.doihttps://dx.doi.org/10.1111/lam.12029en_US
cg.isijournalISI Journalen_US
dc.identifier.statusOpen accessen_US
mel.impact-factor1.575en_US
cg.issn0266-8254en_US
cg.journalLETTERS IN APPLIED MICROBIOLOGYen_US
cg.issue6en_US
cg.volume26en_US


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