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dc.contributor.authorAtwan, Zeenah Weheedvi
dc.date.accessioned2021-08-30T09:04:14Z-
dc.date.available2021-08-30T09:04:14Z-
dc.date.issued2020-
dc.identifier.issn 2522-8307vi
dc.identifier.urihttp://tailieuso.tlu.edu.vn/handle/DHTL/11162-
dc.description.abstractAdenovirus hexon in interferon-deficient cells showed different expression levels when data were normalized to GAPDH or 18S. Consistently, hexon expression levels were different in untreated cells under the control or heat-shocked conditions when data were normalized to GAPDH or 18S. Promyelocytic leukemia protein II (PML-II) expression level was lower in HeLa-PML-II-deficient cells (PML-II-Kd) compared to the control when the data were normalized to GAPDH as a reference gene and also in GAPDH RNA spiked, which showed reasonable consistency. More consistent data were obtained when the GAPDH normalizer was added before the step of treating the extracted RNA with DNase compared to add it after the treatment or directly to the qPCR reaction.vi
dc.description.urihttps://bnrc.springeropen.com/articles/10.1186/s42269-020-00284-1vi
dc.languageenvi
dc.relation.ispartofseriesBulletin of the National Research Centre, Volume 44 (2020), Article number: 32vi
dc.subjectSpike RNAvi
dc.subjectqPCRvi
dc.subjectRelative expressionvi
dc.subjectHousekeeping genesvi
dc.subjectUniversal normalizervi
dc.titleGAPDH spike RNA as an alternative for housekeeping genes in relative gene expression assay using real-time PCRvi
dc.typeBBvi
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