Literature DB >> 20599560

Discrimination of infectious bacteriophage T4 virus by propidium monoazide real-time PCR.

Mariana Fittipaldi1, Nancy J Pino Rodriguez, Francesc Codony, Bárbara Adrados, Gustavo A Peñuela, Jordi Morató.   

Abstract

The advent of quantitative PCR has improved the detection of human viral pathogens in the environment. However, a serious limitation of this method may arise from the inability to discriminate between viruses that are infectious and viruses that have been inactivated and do not represent a human health hazard. To assess whether propidium monoazide (PMA) pre-treatment is a good approach to inhibiting DNA amplification from non-infectious viruses, bacteriophage T4 survival was measured using cell culture titration and real-time PCR with and without PMA pre-treatment. Heat (85 degrees C) and proteolysis methods were carried out. After these inactivation treatments, the results indicated that the PMA pre-treatment approach is not appropriate for differentiating infectious viruses. However, when a heat treatment at 110 degrees C was undertaken, PMA pre-treatment did allow differentiation of non-infectious from infectious viruses. In this case, effective binding of PMA to bacteriophage T4 DNA could be taken to indicate capsid damage. Therefore, PMA pre-treatment may be appropriate for assessing effective disinfection treatments and for a more reliable understanding of the factors that contribute to viral inactivation through capsid damage monitoring. The PMA-PCR approach could be useful as a rapid and inexpensive analytical tool for screening and evaluation of the efficacy of disinfectants. Copyright 2010 Elsevier B.V. All rights reserved.

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Year:  2010        PMID: 20599560     DOI: 10.1016/j.jviromet.2010.06.011

Source DB:  PubMed          Journal:  J Virol Methods        ISSN: 0166-0934            Impact factor:   2.014


  24 in total

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Review 2.  Dead or alive: molecular assessment of microbial viability.

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3.  Enzyme treatment reverse transcription-PCR to differentiate infectious and inactivated F-specific RNA phages.

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5.  Selective quantification of viable Escherichia coli bacteria in biosolids by quantitative PCR with propidium monoazide modification.

Authors:  Bilgin Taskin; Ayse Gul Gozen; Metin Duran
Journal:  Appl Environ Microbiol       Date:  2011-05-20       Impact factor: 4.792

6.  Discrimination of infectious hepatitis A viruses by propidium monoazide real-time RT-PCR.

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Journal:  Food Environ Virol       Date:  2011-12-17       Impact factor: 2.778

7.  Quantification of viable Giardia cysts and Cryptosporidium oocysts in wastewater using propidium monoazide quantitative real-time PCR.

Authors:  José L Alonso; Inmaculada Amorós; Rebecca A Guy
Journal:  Parasitol Res       Date:  2014-04-30       Impact factor: 2.289

8.  Evaluation of Assays to Quantify Infectious Human Norovirus for Heat and High-Pressure Inactivation Studies Using Tulane Virus.

Authors:  Xinhui Li; Runze Huang; Haiqiang Chen
Journal:  Food Environ Virol       Date:  2017-02-25       Impact factor: 2.778

9.  Capsid-Damaging Effects of UV Irradiation as Measured by Quantitative PCR Coupled with Ethidium Monoazide Treatment.

Authors:  J Sangsanont; H Katayama; F Kurisu; H Furumai
Journal:  Food Environ Virol       Date:  2014-08-09       Impact factor: 2.778

10.  Quantification of M13 and T7 bacteriophages by TaqMan and SYBR green qPCR.

Authors:  Xiujuan Peng; Alex Nguyen; Debadyuti Ghosh
Journal:  J Virol Methods       Date:  2017-12-02       Impact factor: 2.014

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