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Appl. Environ. Microbiol., Nov 1997, 4401-4407, Vol 63, No. 11
YS Shieh, RS Baric and MD Sobsey
To detect less prevalent viruses, such as wild-type polioviruses in sewage
from a highly immunized community, a method was developed to efficiently
recover viruses and remove PCR inhibitors. The method consisted of initial
separation of solids from liquid, followed by solvent extractions,
polyethylene glycol precipitations, Sephadex G-200 chromatography, and
guanidinium isothiocyanate (GIT) extraction. To elute viruses from the
separated solids, 0.5 M threonine (pH 7.5) was as efficient as 3% beef
extract but conferred no PCR inhibition. In samples that were concentrated
approximately 1,000-fold, 21% of the initially seeded viruses were
recovered. When poliovirus type 3 (PV3) Sabin strain at low levels and PV1
LSc strain at high levels were seeded in raw sewage, PV3 was specifically
detected in the final sample concentrates at sensitivities of 14 PFU by
direct PCR and 0.7 PFU by GIT extraction-PCR. While applying the method to
international airplane sewage, which contains high levels of solids as well
as commercial sanitizers, 44% (7 of 16) of the samples were found to harbor
enteroviruses by both cell culture infectivity and pan-enterovirus PCR
analyses. Nucleotide sequencing of the PCR products revealed that multiple
enterovirus genotypes were amplified from each final sewage concentrate,
whereas the fewer virus genotypes detected by cell culture infectivity were
probably the better growing strains. By this method, we demonstrated that
air travel may contribute to the intercontinental dissemination of enteric
pathogens.
Copyright © 1997, American Society for Microbiology
Detection of low levels of enteric viruses in metropolitan and airplane sewage
Department of Environmental Sciences and Engineering, University of North Carolina, Chapel Hill 27599-7400, USA.
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