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Simultaneous Detection of Feces - specific Bacteriophages of Bacteroides fragilis with a Duplex PCR Assay

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sc-ar-skorn-2018.pdf (1.74 MB)

Issued Date

2018

Resource Type

Research Article

Language

eng

DOI

10.14456/ennrj.2018.8

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Mahidol University

Rights Holder(s)

Faculty of Environment and Resource Studies Mahidol University

Bibliographic Citation

Environment and Natural Resources Journal. Vol. 16, No. 1 (2018), 82-90

Suggested Citation

Natcha Chyerochana, Benjarath Pupacdi Javed, Pornjira Somnark, Skorn Mongkolsuk, Kwanrawee Sirikanchana Simultaneous Detection of Feces - specific Bacteriophages of Bacteroides fragilis with a Duplex PCR Assay. Environment and Natural Resources Journal. Vol. 16, No. 1 (2018), 82-90. doi:10.14456/ennrj.2018.8 Retrieved from: https://repository.li.mahidol.ac.th/handle/20.500.14594/40498

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Title

Simultaneous Detection of Feces - specific Bacteriophages of Bacteroides fragilis with a Duplex PCR Assay

Author(s)

Natcha Chyerochana
 Benjarath Pupacdi Javed
 Pornjira Somnark
 Skorn Mongkolsuk
 Kwanrawee Sirikanchana

Other Contributor(s)

Chulabhorn Research Institute. Research Laboratory of Biotechnology
 Chulabhorn Research Institute. Translational Research Unit
 Mahidol University. Faculty of Science. Department of Biotechnology

Abstract

Bacteriophages of the Bacteroides fragilisstrains HSP40 and RYC2056 are used as indicators of human-specific and general (non-host specific) fecal pollution in water bodies. However, conventional anaerobic cultivation methods require 1-2 days of incubation. To overcome this limitation, in this study, we developed a DNA-based method to simultaneously detect representative bacteriophages (B40-8 and B56-3) that infect B. fragilisstrains HSP40 and RYC2056, respectively. Both phages yielded a 224-bp amplicon with the primer pair BT5414/BT5415, and an additional 152-bp PCR product was observed for B40-8 with the primer pair BT5579/BT5580. The detection limits for B40-8 and B56-3 were 10-5and 10-4ng of pure DNA, and 1 and 50 ng of DNA template when 5 and 5,000 PFU/mL were spiked into distilled water, respectively. The assay exhibited a higher sensitivity for sewage samples, with <0.1 and 15 PFU/mL of phages infecting HSP40 and RYC2056, respectively. The assay did not produce false positive results for the Bacteroides phages PG76, HB13, and GA17 or for the enterococcal phages AIM06 and SR14. The assay also detected RYC2056 phages that were isolated from sewage samples and the phage B40-8 when it was spiked into raw sewage. Thus, the newly developed PCRassay demonstrated potential for the environmental monitoring of Bacteroidesbacteriophages, decreasing the analysis time to a few hours

Keyword(s)

Polymerase chain reaction (PCR)
 Microbial source tracking
 Bacteriophage
 Bacteroides fragilis
 Water quality

Availability

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https://repository.li.mahidol.ac.th/handle/20.500.14594/40498

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SC-Article