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dc.contributor.authorMitui, M.T.en_US
dc.contributor.authorChandrasena, T.G.A.N.en_US
dc.contributor.authorChan, P.K.S.en_US
dc.contributor.authorRajindrajith, S.en_US
dc.contributor.authorNelson, E.A.S.en_US
dc.contributor.authorLeung, T.F.en_US
dc.contributor.authorNishizono, A.en_US
dc.contributor.authorAhmed, K.en_US
dc.date.accessioned2014-10-29T09:39:36Z-
dc.date.available2014-10-29T09:39:36Z-
dc.date.issued2012en_US
dc.identifier.citationVirology Journal; 9: pp.144en_US
dc.identifier.issn1743-422X (Electronic)en_US
dc.identifier.urihttp://repository.kln.ac.lk/handle/123456789/2159-
dc.description.abstractReverse transcription (RT)-PCR is now the standard method for typing group A rotaviruses (RVA) to monitor the circulating genotypes in a population. Selection of primers that can accurately type the circulating genotypes is crucial in the context of vaccine introduction and correctly interpreting the impact of vaccination on strain distribution. To our knowledge this study is the first report from Asia of misidentification of genotype G9 as G3 due to a primer-template mismatch. We tested two published G-genotype specific primers sets, designed by Gouvea and colleagues (Set A) and Iturriza-Gomara and colleagues (Set B) on RVA from Hong Kong and Sri Lanka. Among 52 rotaviruses typed as G3 by set A primers, 36 (69.2%) were identified as G9 by nucleotide sequencing and set B primers. Moreover, of 300 rotaviruses tested, 28.3% were untypable by set A primers whereas only 12.3% were untypable by set B primers. Our findings reinforce the need to periodically monitor the primers used for RVA genotyping.-
dc.publisherBioMed Centralen_US
dc.titleInaccurate identification of rotavirus genotype G9 as genotype G3 strains due to primer mismatchen_US
dc.typeArticleen_US
dc.identifier.departmentParasitologyen_US
dc.identifier.departmentPaediatricsen_US
dc.creator.corporateauthorBioMed Central Ltden_US
dc.description.noteIndexed in MEDLINEen_US
Appears in Collections:Journal/Magazine Articles

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