A real-time PCR assay to accurately quantify polar bear DNA in fecal extracts
Author(s) -
Kristen M. Hayward,
Michelle P. Harwood,
Stephen C. Lougheed,
Zhengxin Sun,
Peter van Coeverden de Groot,
Evelyn L. Jensen
Publication year - 2020
Publication title -
peerj
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.927
H-Index - 70
ISSN - 2167-8359
DOI - 10.7717/peerj.8884
Subject(s) - feces , real time polymerase chain reaction , biology , computational biology , dna , polar , genetics , microbiology and biotechnology , gene , physics , astronomy
DNA extracted from fecal samples contains DNA from the focal species, food, bacteria and pathogens. Most DNA quantification methods measure total DNA and cannot differentiate among sources. Despite the desirability of noninvasive fecal sampling for studying wildlife populations, low amounts of focal species DNA make it difficult to use for next-generation sequencing (NGS), where accurate DNA quantification is critical for normalization. Two factors are required prior to using fecal samples in NGS libraries: (1) an accurate quantification method for the amount of target DNA and (2) a determination of the relative amount of target DNA needed for successful single nucleotide polymorphism genotyping assays. Here, we address these needs by developing primers to amplify a 101 bp region of the nuclear gene and a quantitative PCR (qPCR) assay that allows the accurate quantification of the amount of polar bear () DNA in fecal extracts. We test the assay on pure polar bear DNA extracted from muscle tissue and find a high correlation between fluorometric and qPCR quantifications. The qPCR assay was also successfully used to quantify the amount of DNA derived from polar bears in fecal extractions. Orthologs of the gene have been identified across vertebrates; thus, similar qPCR assays could be developed for other species to enable noninvasive studies.
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