Please use this identifier to cite or link to this item: https://scholarbank.nus.edu.sg/handle/10635/112138
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dc.titleThermus aquaticus DNA polymerase-catalysed chain reaction for the detection of human papillomaviruses
dc.contributor.authorChow, V.T.K.
dc.contributor.authorTham, K.M.
dc.contributor.authorBernard, H.U.
dc.date.accessioned2014-11-28T02:53:38Z
dc.date.available2014-11-28T02:53:38Z
dc.date.issued1990-01
dc.identifier.citationChow, V.T.K.,Tham, K.M.,Bernard, H.U. (1990-01). Thermus aquaticus DNA polymerase-catalysed chain reaction for the detection of human papillomaviruses. Journal of Virological Methods 27 (1) : 101-112. ScholarBank@NUS Repository.
dc.identifier.issn01660934
dc.identifier.urihttp://scholarbank.nus.edu.sg/handle/10635/112138
dc.description.abstractTo delineate the conditions for the polymerase chain reaction (PCR) using primers specific for human papillomavirus (HPV) types 6b, 16 and 18, a number of important technical features were analysed. Buffer, concentrations of magnesium, Taq polymerase, primers and DNA templates, annealing temperature, and extension time were studied by a combination of gel electrophoresis, Southern and slot-blot hybridization. Amplification of E6 gene fragments of HPV-16 and HPV-18 generated bands of 110 bp and 154 bp respectively, as predicted. However, amplification of a segment within the long control region of HPV 6b yielded an unexpected size of 340 bp. Different conditions were found for each HPV type-specific primer pair. These results, and the applications of PCR in HPV research and in an increasingly wide range of fields in medical virology are discussed. © 1990.
dc.sourceScopus
dc.subjectHuman papillomavirus (HPV)
dc.subjectPolymerase chain reaction (PCR)
dc.subjectThermus aquaticus DNA polymerase
dc.typeArticle
dc.contributor.departmentINSTITUTE OF MOLECULAR & CELL BIOLOGY
dc.description.sourcetitleJournal of Virological Methods
dc.description.volume27
dc.description.issue1
dc.description.page101-112
dc.description.codenJVMED
dc.identifier.isiutNOT_IN_WOS
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