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dc.creatorArtlett, CM
dc.creatorDito, CG
dc.creatorChristner, PJ
dc.date.accessioned2021-02-01T22:32:14Z
dc.date.available2021-02-01T22:32:14Z
dc.date.issued2003-12-01
dc.identifier.issn1480-9222
dc.identifier.issn1480-9222
dc.identifier.doihttp://dx.doi.org/10.34944/dspace/5644
dc.identifier.otherPMC153846 (pmc)
dc.identifier.urihttp://hdl.handle.net/20.500.12613/5662
dc.description.abstractReal-time PCR methodology can successfully quantitate microchimeric cell populations at a concentration of 100 microchimeric cells/100,000 host cells; however, it has not been successful in quantitating DNA from trace numbers of microchimeric white blood cells which we reported are present in murine peripheral blood at a concentration as low as 2/100,000 host cells. We report methodology using primers for a portion of the H2-kb murine histocompatibility sequence, specific for the C57BL/6J mouse. When these primers were used in the presence of 11,000 μM primer, a 20-fold increase in the median manufacturer's recommended concentration, the assay could be optimized to detect 34 pg of C57BL/6J DNA in a background of 2.5 μg of carrier BALB/cJ DNA (1/100,000). These conditions resulted in a detection limit half as sensitive as that found when no carrier DNA was present.
dc.format.extent103-107
dc.language.isoen
dc.relation.haspartBiological Procedures Online
dc.relation.isreferencedbySpringer Science and Business Media LLC
dc.titleMethodology for detecting trace amounts of microchimeric DNA from peripheral murine white blood cells by real-time PCR
dc.typeArticle
dc.type.genreJournal Article
dc.relation.doi10.1251/bpo51
dc.ada.noteFor Americans with Disabilities Act (ADA) accommodation, including help with reading this content, please contact scholarshare@temple.edu
dc.date.updated2021-02-01T22:32:11Z
refterms.dateFOA2021-02-01T22:32:14Z


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