serious overestimation in quantitative pcr by circular (supercoiled) plasmid standard microalgal pcna as the model gene严重高估的定量pcr循环超螺旋质粒标准microalgal pcna基因模型.pdfVIP
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serious overestimation in quantitative pcr by circular (supercoiled) plasmid standard microalgal pcna as the model gene严重高估的定量pcr循环超螺旋质粒标准microalgal pcna基因模型
Serious Overestimation in Quantitative PCR by Circular
(Supercoiled) Plasmid Standard: Microalgal pcna as the
Model Gene
Yubo Hou¤a* , Huan Zhang, Lilibeth Miranda¤b, Senjie Lin
Department of Marine Sciences, University of Connecticut, Groton, Connecticut, United States of America
Abstract
Quantitative real-time PCR (qPCR) has become a gold standard for the quantification of nucleic acids and microorganism
abundances, in which plasmid DNA carrying the target genes are most commonly used as the standard. A recent study
showed that supercoiled circular confirmation of DNA appeared to suppress PCR amplification. However, to what extent to
which different structural types of DNA (circular versus linear) used as the standard may affect the quantification accuracy
has not been evaluated. In this study, we quantitatively compared qPCR accuracies based on circular plasmid (mostly in
supercoiled form) and linear DNA standards (linearized plasmid DNA or PCR amplicons), using proliferating cell nuclear gene
(pcna), the ubiquitous eukaryotic gene, in five marine microalgae as a model gene. We observed that PCR using circular
plasmids as template gave 2.65-4.38 more of the threshold cycle number than did equimolar linear standards. While the
documented genome sequence of the diatom Thalassiosira pseudonana shows a single copy of pcna, qPCR using the
circular plasmid as standard yielded an estimate of 7.77 copies of pcna per genome whereas that using the linear standard
gave 1.02 copies per genome. We conclude that circular plasmid DNA is unsuitable as a standard, and linear DNA should be
used instead, in absolute qPCR. The serious overestimation by the circular plasmid standard is likely due to the undetected
lower efficiency of its amplification in the early stage of PCR when the supercoiled plasmid is the dominant template.
Citation: Hou Y, Zhang H, Miranda L, Lin S (20
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