Quantitative real-time PCR using TaqMan and SYBR Green forActinobacillus actinomycetemcomitans,Porphyromonas gingivalis,Prevotella intermedia,tetQgene and total bacteria

Abstract: Accurate quantification of bacterial species in dental plaque is needed for microbiological diagnosis of periodontal diseases. The present study was designed to assess the sensitivity, specificity and quantitativity of the real-time PCR using the GeneAmp Sequence Detection System with two fluorescence chemistries. TaqMan probe with reporter and quencher dye, and SYBR Green dye were used for sources of the fluorescence. Primers and probes were designed for Actinobacillus actinomycetemcomitans, Porphyromonas gin… Show more

“…The DNA samples were used as templates to quantify the copy numbers of 16SrRNA (for bacteria) and of methyl coenzyme M reductase A (mcrA) gene for methanogens. For each microbial group, three different aliquots of DNA were analysed using qPCR with the following primer pairs: forward: 5′-GTGSTGCAYGGYTGTCGTCA-3′ and reverse: 5′-ACGTCRTCCMCACCTTCCTC-3′ for total bacteria (Maeda et al, 2003), and forward: 5′-TTCGGTGGATCDCARAGRGC-3′ and reverse: 5′-GBARGTCGWAWCCGTAGAATCC-3′for methanogens (Denman et al, 2007). A negative control (sterile distilled water) was also loaded on each plate run to screen for possible contamination and dimer formation and to set the background fluorescence for plate normalization.…”

“…The external standards used for the qPCR amplifications had been validated previously for rumen bacteria (Maeda et al, 2003) and methanogenic archaea (Denman et al, 2007).…”

The effects of feed blocks containing tomato and cucumber by-products on <i>in vitro</i> ruminal fermentation, microbiota, and methane production

“…The DNA samples were used as templates to quantify the copy numbers of 16SrRNA (for bacteria) and of methyl coenzyme M reductase A (mcrA) gene for methanogens. For each microbial group, three different aliquots of DNA were analysed using qPCR with the following primer pairs: forward: 5′-GTGSTGCAYGGYTGTCGTCA-3′ and reverse: 5′-ACGTCRTCCMCACCTTCCTC-3′ for total bacteria (Maeda et al, 2003), and forward: 5′-TTCGGTGGATCDCARAGRGC-3′ and reverse: 5′-GBARGTCGWAWCCGTAGAATCC-3′for methanogens (Denman et al, 2007). A negative control (sterile distilled water) was also loaded on each plate run to screen for possible contamination and dimer formation and to set the background fluorescence for plate normalization.…”

“…The external standards used for the qPCR amplifications had been validated previously for rumen bacteria (Maeda et al, 2003) and methanogenic archaea (Denman et al, 2007).…”

The effects of feed blocks containing tomato and cucumber by-products on <i>in vitro</i> ruminal fermentation, microbiota, and methane production

“…The gene encoding the small subunit of bacterial 16S rDNA has been used frequently as a target of PCR examination because of its structural characteristics [2,5]. The nucleotide sequences of some portions of the 16S rDNA are highly conserved through evolution [3]. The conserved sequences can provide PCR primers for amplification of 16S rDNA from all bacterial species [3].…”

“…The nucleotide sequences of some portions of the 16S rDNA are highly conserved through evolution [3]. The conserved sequences can provide PCR primers for amplification of 16S rDNA from all bacterial species [3]. Quantitative real-time PCR has been demonstrated to be a powerful tool for quantitative microbiological examination [3].…”

“…The conserved sequences can provide PCR primers for amplification of 16S rDNA from all bacterial species [3]. Quantitative real-time PCR has been demonstrated to be a powerful tool for quantitative microbiological examination [3]. Therefore, we evaluated the changes in total bacterial counts on the buccal mucosa after using Oralbalance® by real-time PCR quantification of 16S rDNA.…”

Total bacterial counts on oral mucosa after using a commercial saliva substitute in patients undergoing hematopoietic cell transplantation

Molecular Analysis of Endodontic Infections