Relative quantification of mRNA: comparison of methods currently used for real-time PCR data analysis

Číkoš, Štefan; Bukovská, Alexandra; Koppel, Juraj

doi:10.1186/1471-2199-8-113

Cited by 330 publications

(135 citation statements)

References 23 publications

(33 reference statements)

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“…Using the LinRegPCR method to calculate E fi , Č ikos et al (9) found that the interleukin 6 gene amplified with an E fi of 1.88, while the beta actin gene amplified with an E fi of 1.99. Moreover, they found that these differences between the genes remained regardless of the method used to determine E fi (9). Similarly, other studies found that E determined for the same PCR template is more constant (5, 9, 26).…”

Section: Resultsmentioning

confidence: 99%

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Simple Absolute Quantification Method Correcting for Quantitative PCR Efficiency Variations for Microbial Community Samples

Brankatschk

Bodenhausen

Zeyer

et al. 2012

Appl Environ Microbiol

187

126

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ABSTRACTReal-time quantitative PCR (qPCR) is a widely used technique in microbial community analysis, allowing the quantification of the number of target genes in a community sample. Currently, the standard-curve (SC) method of absolute quantification is widely employed for these kinds of analysis. However, the SC method assumes that the amplification efficiency (E) is the same for both the standard and the sample target template. We analyzed 19 bacterial strains and nine environmental samples in qPCR assays, targeting thenifHand 16S rRNA genes. TheEvalues of the qPCRs differed significantly, depending on the template. This has major implications for the quantification. If the sample and standard differ in theirEvalues, quantification errors of up to orders of magnitude are possible. To address this problem, we propose and test the one-point calibration (OPC) method for absolute quantification. The OPC method corrects for differences inEand was derived from the ΔΔCTmethod with correction forE, which is commonly used for relative quantification in gene expression studies. The SC and OPC methods were compared by quantifying artificial template mixtures fromGeobacter sulfurreducens(DSM 12127) andNostoc commune(Culture Collection of Algae and Protozoa [CCAP] 1453/33), which differ in theirEvalues. While the SC method deviated from the expectednifHgene copy number by 3- to 5-fold, the OPC method quantified the template mixtures with high accuracy. Moreover, analyzing environmental samples, we show that even small differences inEbetween the standard and the sample can cause significant differences between the copy numbers calculated by the SC and the OPC methods.

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Section: Resultsmentioning

confidence: 99%

“…We calculated E sample and E standard as the mean E fi from individual replicates, because previous studies recommended using the means of E fi (9,30,40). Alternatively, E sample and E standard could be estimated from dilution series, E ds (equation 3) (31).…”

Section: Bacterial Cultures (I)mentioning

confidence: 99%

Simple Absolute Quantification Method Correcting for Quantitative PCR Efficiency Variations for Microbial Community Samples

Brankatschk

Bodenhausen

Zeyer

et al. 2012

Appl Environ Microbiol

187

126

View full text Add to dashboard Cite

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“…PCR efficiency was determined for each gene by LinRegPCR program (Ramakers et al, 2003;Ruijter et al, 2009). This software was successfully used previously to calculate PCR efficiency (Č ikoš et al, 2007;Feng et al, 2008;Regier & Frey, 2010;Aglawe et al, 2012, Borges et al, 2012.…”

Section: Methodsmentioning

confidence: 99%

Defects in RNA polyadenylation impair both lysogenization by and lytic development of Shiga toxin-converting bacteriophages

Nowicki

Bloch

Nejman-Faleńczyk

et al. 2015

Journal of General Virology

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In Escherichia coli, the major poly(A) polymerase (PAP I) is encoded by the pcnB gene. In this report, a significant impairment of lysogenization by Shiga toxin-converting (Stx) bacteriophages (W24 B , 933W, P22, P27 and P32) is demonstrated in host cells with a mutant pcnB gene. Moreover, lytic development of these phages after both infection and prophage induction was significantly less efficient in the pcnB mutant than in the WT host. The increase in DNA accumulation of the Stx phages was lower under conditions of defective RNA polyadenylation. Although shortly after prophage induction, the levels of mRNAs of most phage-borne early genes were higher in the pcnB mutant, at subsequent phases of the lytic development, a drastically decreased abundance of certain mRNAs, including those derived from the N, O and Q genes, was observed in PAP I-deficient cells. All of these effects observed in the pcnB cells were significantly more strongly pronounced in the Stx phages than in bacteriophage l. Abundance of mRNA derived from the pcnB gene was drastically increased shortly (20 min) after prophage induction by mitomycin C and decreased after the next 20 min, while no such changes were observed in non-lysogenic cells treated with this antibiotic. This prophage induction-dependent transient increase in pcnB transcript may explain the polyadenylation-driven regulation of phage gene expression.

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“…Primers and their PCR product sizes are shown in Table 5. For quantification, we used the relative standard curve method (Cikos et al 2007). Ribosomal protein L13a (Rpl13a) was used as a reference gene.…”

Section: Rna Extraction and Quantitative Real-time Pcrmentioning

confidence: 99%

Photoperiod-gonadotropin mismatches induced by treatment with acyline or FSH in Siberian hamsters: impacts on ovarian structure and function

et al. 2012

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Many seasonal breeders time their reproductive efforts to specific times of the year to ensure adequate resources for the production and care of young. For long-day (LD) breeders, females born before the summer solstice (LDs) reach sexual maturity quickly and often breed that same year, whereas females born after the summer solstice (short days (SDs)) may delay reproductive development to the following spring when environmental conditions are favorable for reproduction. In Siberian hamsters, development in SD is associated with structural and functional differences in the ovary compared with females held in LD, including a greater number of primordial follicles and an abundance of hypertrophied granulosa cells (HGCs), which are immunoreactive for anti-Mü llerian hormone. The goal of this study was to determine whether SD-induced gonadotropin suppression is responsible for these phenotypic differences. Gonadotropin levels were suppressed in LD hamsters using the GNRH antagonist acyline. Conversely, to determine whether the SD ovarian phenotype is completely reversed by gonadotropin stimulation, recombinant human FSH (rhFSH) was administered. Our treatments were successful in mimicking FSH concentrations of the opposite photoperiod, but they did not produce a comparable change in the ovarian phenotype. Most notable was the lack of HGCs in the ovaries of acyline-treated LD females. Similarly, HGCs were maintained in the ovaries of SD females treated with rhFSH. Our data suggest that gonadotropins alone do not account for the SD ovarian phenotype. Future studies will determine whether SD-induced changes in other factors underlie these phenotypic changes.

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Relative quantification of mRNA: comparison of methods currently used for real-time PCR data analysis

Cited by 330 publications

References 23 publications

Simple Absolute Quantification Method Correcting for Quantitative PCR Efficiency Variations for Microbial Community Samples

Simple Absolute Quantification Method Correcting for Quantitative PCR Efficiency Variations for Microbial Community Samples

Defects in RNA polyadenylation impair both lysogenization by and lytic development of Shiga toxin-converting bacteriophages

Photoperiod-gonadotropin mismatches induced by treatment with acyline or FSH in Siberian hamsters: impacts on ovarian structure and function

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