Literature DB >> 17390542

Gene expression of HIF-1alpha and XRCC4 measured in human samples by real-time RT-PCR using the sigmoidal curve-fitting method.

Hao Qiu1, Karine Durand, Hélène Rabinovitch-Chable, Michel Rigaud, Virgile Gazaille, Pierre Clavère, Franck G Sturtz.   

Abstract

Quantitative reverse transcription PCR (RT-PCR) has become an important tool for studying functional gene expression. However the most often used cycle threshold (CT)-based method, primarily related to the required amplification efficiency determination via serial dilution, can call into question the level of quantitative reliability and accuracy that can be achieved, in addition to the impracticalities inherent to CT-based methodologies. In this study, an alternative method, named the sigmoidal curve-fitting (SCF) method, was compared with the classic CT method for two target genes (XRCC4 and HIF-1alpha) and a reference gene (HPRT). The PCR conditions were optimized for each gene on a LightCycler apparatus. Fluorescence data were fitted to a four-parametric sigmoidal function, and the initial messenger RNA (mRNA) copy number was determined by a theoretical fluorescence (F0) value calculated from each fitting curve. The relative expression of the target gene versus that of the reference gene was calculated using an equation based upon these F0 values. The results show that the F0 value had a good linearity with the initial number of target genes between 10(7) and 10(1) copies. The reproducibility tests showed that the variations of initial target quantity were well reflected by F0 values. Relative expression of target gene calculated by the SCF method and by the CT method showed similar results. In our hands, the SCF method gave reliable results and a more precise error description of quantitative RT-PCR.

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Year:  2007        PMID: 17390542     DOI: 10.2144/000112331

Source DB:  PubMed          Journal:  Biotechniques        ISSN: 0736-6205            Impact factor:   1.993


  12 in total

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3.  Shape based kinetic outlier detection in real-time PCR.

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Journal:  Acta Biomater       Date:  2009-06-02       Impact factor: 8.947

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6.  XLS (c9orf142) is a new component of mammalian DNA double-stranded break repair.

Authors:  A Craxton; J Somers; D Munnur; R Jukes-Jones; K Cain; M Malewicz
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7.  Relative quantification of mRNA: comparison of methods currently used for real-time PCR data analysis.

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Journal:  BMC Mol Biol       Date:  2007-12-20       Impact factor: 2.946

8.  A kinetic-based sigmoidal model for the polymerase chain reaction and its application to high-capacity absolute quantitative real-time PCR.

Authors:  Robert G Rutledge; Don Stewart
Journal:  BMC Biotechnol       Date:  2008-05-08       Impact factor: 2.563

9.  Critical evaluation of methods used to determine amplification efficiency refutes the exponential character of real-time PCR.

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Journal:  BMC Mol Biol       Date:  2008-10-30       Impact factor: 2.946

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Authors:  María Belén Federico; María Belén Vallerga; Analía Radl; Natalia Soledad Paviolo; José Luis Bocco; Marina Di Giorgio; Gastón Soria; Vanesa Gottifredi
Journal:  PLoS Genet       Date:  2016-01-14       Impact factor: 5.917

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