Analysis of qPCR reference gene stability determination methods and a practical approach for efficiency calculation on a turbot (Scophthalmus maximus) gonad dataset

Abstract: BackgroundGene expression analysis by reverse transcription quantitative PCR (qPCR) is the most widely used method for analyzing the expression of a moderate number of genes and also for the validation of microarray results. Several issues are crucial for a successful qPCR study, particularly the selection of internal reference genes for normalization and efficiency determination. There is no agreement on which method is the best to detect the most stable genes neither on how to perform efficiency determinatio… Show more

“…As described by Peirson et al (2003), several analytical procedures could result in a cumulative error that might lead to efficiency overestimation. To overcome these limitations, mathematical models have been published describing the kinetics of the qPCR reaction and trying to estimate qPCR efficiency from a single reaction (Robledo et al 2014). The methodology implemented by the LinRegPCR software used in the present study resulted in values of qPCR efficiency ranging from 55 to 94%, which are reduced values compared to the standard curve.…”

“…The absolute Cq values individually obtained for each one of the five reference genes are graphically represented on a box plot graphic in Figure 1 where the median raw Cqs are represented by lines. There is a premise that reference genes cannot be regulated by the experimental conditions of the sample set (Robledo et al 2014). The geNorm and BestKeeper algorithms are based on the assumption that none of the analyzed genes are co-regulated (Matz et al 2013).…”

“…For all samples analyzed together, geNorm ranked T197 and β-tubulin as the most stable genes (M = 1.4) with the combined value below the recommended cutoff of 1.5 (Robledo et al 2014). NormFinder considered the same two genes most stable, with a combined stability value of 0.468.…”

An improved method for RNA extraction from common bean seeds and validation of reference genes for qPCR

“…As described by Peirson et al (2003), several analytical procedures could result in a cumulative error that might lead to efficiency overestimation. To overcome these limitations, mathematical models have been published describing the kinetics of the qPCR reaction and trying to estimate qPCR efficiency from a single reaction (Robledo et al 2014). The methodology implemented by the LinRegPCR software used in the present study resulted in values of qPCR efficiency ranging from 55 to 94%, which are reduced values compared to the standard curve.…”

“…The absolute Cq values individually obtained for each one of the five reference genes are graphically represented on a box plot graphic in Figure 1 where the median raw Cqs are represented by lines. There is a premise that reference genes cannot be regulated by the experimental conditions of the sample set (Robledo et al 2014). The geNorm and BestKeeper algorithms are based on the assumption that none of the analyzed genes are co-regulated (Matz et al 2013).…”

“…For all samples analyzed together, geNorm ranked T197 and β-tubulin as the most stable genes (M = 1.4) with the combined value below the recommended cutoff of 1.5 (Robledo et al 2014). NormFinder considered the same two genes most stable, with a combined stability value of 0.468.…”

An improved method for RNA extraction from common bean seeds and validation of reference genes for qPCR

“…GAPDH was used as housekeeping gene (forward: 5′-TGGTATCGTGGAAGGACTCATG-3′; reverse: 5′-GCTTCACCACCTT-CTT-GATGTC-3′). LinRegPCR software was applied to determine PCR efficiency [36]. The fold changes of gene expression were computed using the Pfaffl method [37].…”

Docosahexaenoic Acid-Rich Fish Oil Supplementation Improves Body Composition without Influence of the PPARγ Pro12Ala Polymorphism in Patients with Type 2 Diabetes: A Randomized, Double-Blind, Placebo-Controlled Clinical Trial

“…First, a miRNA serial titration assay was performed using synthetic oligonucleotide hsa-miR-9-5p as a template, a forward primer hsa-miR-9-5p-F and a universal reverse primer (pair of primers designed by the uni-system, see Figure 1). As shown in Figure 2a, the hsa-mir-9-5p demonstrated qPCR efficiency between 90 ~ 110% (N=3, STD <= 0.41), which is considered acceptable (Robledo et al 2014). To evaluate the qPCR efficiency of specific-FR-system, the oligonucleotides hsa-let-7b-5p, member of the let-7 miRNA family, was selected as a template for the miRNA serial titration assay.…”

miPrimer: an empirical-based qPCR primer design method for small noncoding microRNA