Comparison of concentration methods for quantitative detection of sewage-associated viral markers in environmental waters

W Ahmed; V J Harwood; P Gyawali; J P S Sidhu; S Toze

doi:10.1128/AEM.03851-14

Comparison of concentration methods for quantitative detection of sewage-associated viral markers in environmental waters

Appl Environ Microbiol. 2015 Mar;81(6):2042-9. doi: 10.1128/AEM.03851-14. Epub 2015 Jan 9.

Authors

W Ahmed¹, V J Harwood², P Gyawali³, J P S Sidhu⁴, S Toze³

Affiliations

¹ CSIRO Land and Water, Ecosciences Precinct, Brisbane, Queensland, Australia Faculty of Science, Health, and Education, University of the Sunshine Coast, Maroochydore, Queensland, Australia warish.ahmed@csiro.au.
² Department of Integrative Biology, University of South Florida, Tampa, Florida, USA.
³ CSIRO Land and Water, Ecosciences Precinct, Brisbane, Queensland, Australia School of Population Health, University of Queensland, Brisbane, Queensland, Australia.
⁴ CSIRO Land and Water, Ecosciences Precinct, Brisbane, Queensland, Australia Faculty of Science, Health, and Education, University of the Sunshine Coast, Maroochydore, Queensland, Australia School of Population Health, University of Queensland, Brisbane, Queensland, Australia.

Abstract

Pathogenic human viruses cause over half of gastroenteritis cases associated with recreational water use worldwide. They are relatively difficult to concentrate from environmental waters due to typically low concentrations and their small size. Although rapid enumeration of viruses by quantitative PCR (qPCR) has the potential to greatly improve water quality analysis and risk assessment, the upstream steps of capturing and recovering viruses from environmental water sources along with removing PCR inhibitors from extracted nucleic acids remain formidable barriers to routine use. Here, we compared the efficiency of virus recovery for three rapid methods of concentrating two microbial source tracking (MST) viral markers human adenoviruses (HAdVs) and polyomaviruses (HPyVs) from one liter tap water and river water samples on HA membranes (90 mm in diameter). Samples were spiked with raw sewage, and viral adsorption to membranes was promoted by acidification (method A) or addition of MgCl2 (methods B and C). Viral nucleic acid was extracted directly from membranes (method A), or viruses were eluted with NaOH and concentrated by centrifugal ultrafiltration (methods B and C). No inhibition of qPCR was observed for samples processed by method A, but inhibition occurred in river samples processed by B and C. Recovery efficiencies of HAdVs and HPyVs were ∼10-fold greater for method A (31 to 78%) than for methods B and C (2.4 to 12%). Further analysis of membranes from method B revealed that the majority of viruses were not eluted from the membrane, resulting in poor recovery. The modification of the originally published method A to include a larger diameter membrane and a nucleic acid extraction kit that could accommodate the membrane resulted in a rapid virus concentration method with good recovery and lack of inhibitory compounds. The frequently used strategy of viral absorption with added cations (Mg(2+)) and elution with acid were inefficient and more prone to inhibition, and will result in underestimation of the prevalence and concentrations of HAdVs and HPyVs markers in environmental waters.

Publication types

Comparative Study
Evaluation Study
Research Support, Non-U.S. Gov't

MeSH terms

Adenoviruses, Human / isolation & purification*
Biomarkers / analysis
Humans
Polyomavirus / isolation & purification*
Water Microbiology*

Substances

Biomarkers