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Detection of Salmonella Typhi bacteriophages in surface waters as a scalable approach to environmental surveillance. | LitMetric

AI Article Synopsis

  • Environmental surveillance via Salmonella Typhi DNA detection is costly, prompting a study on the abundance of S. Typhi bacteriophages in water in Nepal as a low-cost alternative.
  • Water samples were collected from various areas in Nepal and tested for S. Typhi-specific bacteriophages, showing a high detection rate in urban and peri-urban settings but low in areas with low typhoid incidence.
  • The research found that bacteriophages showed specificity to S. Typhi without infecting other strains, indicating their potential role in monitoring typhoid-endemic environments.

Article Abstract

Background: Environmental surveillance, using detection of Salmonella Typhi DNA, has emerged as a potentially useful tool to identify typhoid-endemic settings; however, it is relatively costly and requires molecular diagnostic capacity. We sought to determine whether S. Typhi bacteriophages are abundant in water sources in a typhoid-endemic setting, using low-cost assays.

Methodology: We collected drinking and surface water samples from urban, peri-urban and rural areas in 4 regions of Nepal. We performed a double agar overlay with S. Typhi to assess the presence of bacteriophages. We isolated and tested phages against multiple strains to assess their host range. We performed whole genome sequencing of isolated phages, and generated phylogenies using conserved genes.

Findings: S. Typhi-specific bacteriophages were detected in 54.9% (198/361) of river and 6.3% (1/16) drinking water samples from the Kathmandu Valley and Kavrepalanchok. Water samples collected within or downstream of population-dense areas were more likely to be positive (72.6%, 193/266) than those collected upstream from population centers (5.3%, 5/95) (p=0.005). In urban Biratnagar and rural Dolakha, where typhoid incidence is low, only 6.7% (1/15, Biratnagar) and 0% (0/16, Dolakha) river water samples contained phages. All S. Typhi phages were unable to infect other Salmonella and non-Salmonella strains, nor a Vi-knockout S. Typhi strain. Representative strains from S. Typhi lineages were variably susceptible to the isolated phages. Phylogenetic analysis showed that S. Typhi phages belonged to the class Caudoviricetes and clustered in three distinct groups.

Conclusions: S. Typhi bacteriophages were highly abundant in surface waters of typhoid-endemic communities but rarely detected in low typhoid burden communities. Bacteriophages recovered were specific for S. Typhi and required Vi polysaccharide for infection. Screening small volumes of water with simple, low-cost (~$2) plaque assays enables detection of S. Typhi phages and should be further evaluated as a scalable tool for typhoid environmental surveillance.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC10852241PMC
http://dx.doi.org/10.1371/journal.pntd.0011912DOI Listing

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