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. 2016 Jul 15;82(15):4767-4775.
doi: 10.1128/AEM.00798-16. Print 2016 Aug 1.

Detection of Antibiotic Resistance Genes in Source and Drinking Water Samples from a First Nations Community in Canada

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Detection of Antibiotic Resistance Genes in Source and Drinking Water Samples from a First Nations Community in Canada

Dinesh M Fernando et al. Appl Environ Microbiol. .

Abstract

Access to safe drinking water is now recognized as a human right by the United Nations. In developed countries like Canada, access to clean water is generally not a matter of concern. However, one in every five First Nations reserves is under a drinking water advisory, often due to unacceptable microbiological quality. In this study, we analyzed source and potable water from a First Nations community for the presence of coliform bacteria as well as various antibiotic resistance genes. Samples, including those from drinking water sources, were found to be positive for various antibiotic resistance genes, namely, ampC, tet(A), mecA, β-lactamase genes (SHV-type, TEM-type, CTX-M-type, OXA-1, and CMY-2-type), and carbapenemase genes (KPC, IMP, VIM, NDM, GES, and OXA-48 genes). Not surprisingly, substantial numbers of total coliforms, including Escherichia coli, were recovered from these samples, and this result was also confirmed using Illumina sequencing of the 16S rRNA gene. These findings deserve further attention, as the presence of coliforms and antibiotic resistance genes potentially puts the health of the community members at risk.

Importance: In this study, we highlight the poor microbiological quality of drinking water in a First Nations community in Canada. We examined the coliform load as well as the presence of antibiotic resistance genes in these samples. This study examined the presence of antibiotic-resistant genes in drinking water samples from a First Nations Community in Canada. We believe that our findings are of considerable significance, since the issue of poor water quality in First Nations communities in Canada is often ignored, and our findings will help shed some light on this important issue.

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Figures

FIG 1
FIG 1
Microbial community composition in water samples determined by amplification of V4 region of 16S rRNA and MiSeq Illumina sequencing. Sample descriptions are provided in Table 1.
FIG 2
FIG 2
Quantification of ampC (A), tet(A) (B), and mecA (C) genes in water samples. Copy number/ng of total DNA was determined using qPCR and calculated using a standard curve created using control bacterial strains. Sample description is provided in Table 1.

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