To address this, we have developed FungiQuant analysis guideline for differentiating random noise from true detection. Lastly, to address the potential presence of exogenous fungal DNA, we recommend the use of negative controls at each sample processing and analysis step. With respect to FungiQuant LOD, it is worth noting that a concentration of 1.8 copies/μl of 18S rRNA gene is the equivalent of 0.5 fg/μl of C. albicans DNA, with the assumption of 55 18S rRNA gene copy number per haploid genome [40]. This concentration, using the published haploid genome size of 15.185 × 10-3 pg for C. albicans shows that 0.5 fg is the equivalent of 1/30 of a single C. albicans genome [40]. Using the
same estimates, the 5-copy LOD of FungiQuant 4-Hydroxytamoxifen solubility dmso is thus the equivalent of 1.38 fg/μl of C. albicans DNA, or the 1/11 of a single C. albicans genome. Similar conversions of DNA concentration and genomic equivalents for LOD estimation for other fungal species can be performed accordingly; this can help to facilitate estimation of DNA concentrations and genomic equivalents of fungi present at levels below other quantitation approaches, including spectrometric and fluorimetric methods. Use of a probe-based reporting mechanism is Raf inhibitor an important feature in FungiQuant in two respects. First, it enhances the quantitative capability of FungiQuant, and secondly, improves
assay specificity. An example illustrating the advantage of probe-based reporting is the comparison of FungiQuant with an intercalating dye-based qPCR assay, which had amplification efficiencies ranging from Bucladesine solubility dmso 67-103% and a LOD of 500pg of fungal DNA [30]. Additionally, the intercalating dye can generate amplification signal irrespective of amplicon size or composition. In summary, we have developed and evaluated a new broad-coverage qPCR assay—FungiQuant—for diverse Evodiamine fungal detection and quantification that showed broad assay coverage and favorable quantitative parameters. A limitation of the current manuscript is the conversion from 18S rRNA gene copy number to the number of cells or biomass. In order to generate an estimated genomic equivalent, improved knowledge of 18S rRNA gene copy number of
diverse fungi is required. And given that 18S rRNA gene copy number varies among fungal species and even among strains or over the lifetime of the fungi [41–43], this challenge will likely to persist. In addition to the design and validation of a broad-coverage fungal qPCR assay, our manuscript also sought to address basic limitations of evaluating combined primer and probe coverage, as well as generating reference standards for absolute quantification. Our approach of evaluating assay coverage by considering the primer and probe sequences as a single unit is appropriate and necessary. Additionally, our approach of quantifying plasmid standards using the intrinsic property of real-time PCR is another important step for any absolute quantification experiments using qPCR.