qPCR was carried out for quantification of 16S rRNA gene copy number to compare the bacterial load collected by each technique. qPCR was performed with universal BactQUANT 16S rRNA gene primers (Forward primer:5′-CTACGGGAGGCAGCA, Reverse primer: 5′-GGACTACCGGGTATCTAATC) (Sigma) with the FAM labelled BactQUANT probe ((6FAM) 5′-CAGCAGCCGCGGTA-3′ (MGBNFQ)) (Liu et al., 2012 (link); Mitra et al., 2017 (link)) on a CFX Real Time PCR system (Bio-Rad). A tenfold standard curve (3030 to 303,039,700 copies) of Escherichia coli genomic DNA (Sigma, D4889) was generated, each reaction contained 5 µL of DNA sample or standard, 10 µL Platinum PCR Super mix UDG containing Rox (Life Tech, 11730-017) and primers and probe. Thermal cycling was performed at 3 min at 50°C for UNG incubation,10 min at 95°C for Taq activation, then 40 cycles of 15 s at 95°C for denaturation and 1 min at 60°C for annealing and extension. Cycle threshold (Ct) value for each reaction were obtained using CFX Maestro software version 1.1 (Bio-Rad) after application of fluorescence drift correction, background subtraction using the ‘curve fit’ option and automatic Ct baseline definition. Ct values were converted to 16S rRNA gene copy number from the generated standard curve. Samples were run in duplicate; a negative control of molecular grade water was included to eliminate contamination.
Bactquant 16s rrna gene primers
Manufactured by Merck Group
Sourced in United Kingdom
BactQUANT 16S rRNA gene primers are a set of oligonucleotide sequences designed to target and amplify the 16S ribosomal RNA gene, a conserved genetic region commonly used for the identification and quantification of bacterial species. These primers are intended for use in quantitative PCR (qPCR) experiments to determine the abundance of bacteria in various samples.
Automatically generated - may contain errors
2 protocols using bactquant 16s rrna gene primers
1
Quantification of Bacterial 16S rRNA Genes
2
Quantifying Bacterial Diversity via qPCR
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Quantitative real-time PCR was carried out for quantification of 16S rRNA gene copy number in order to determine the volume of Preservcyt required for sequencing and to compare the bacterial load collected by each technique in total and of G. vaginalis. Real-time qPCR was performed with universal BactQUANT 16S rRNA gene primers (Forward primer: 5′-CCTACGGGAGGCAGCA, Reverse primer: 5′-GGACTACCGGGTATCTAATC) (Sigma) with the FAM labeled BactQUANT probe ((6FAM) 5′-CAGCAGCCGCGGTA-3′ (MGBNFQ))30 (link) and G. vaginalis primers (Forward primer: 5′-GGAAACGGGTGGTAATGCTGG, Reverse primer: 5′-CGAAGCCTAGGTGGGCCATT)31 (link) using a SYBR green-based assay on the Applied Biosciences StepOne machine (Thermo Fisher Scientific, Ashford, UK) with StepOne software version 2.3 (Life Technologies). Samples were run in duplicate.
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