Rapid detection of Bacillus anthracis by γ phage amplification and lateral flow immunochromatography

New, rapid point-of-need diagnostic methods for Bacillus anthracis detection can enhance civil and military responses to accidental or deliberate dispersal of anthrax as a biological weapon. Current laboratory-based methods for clinical identification of B. anthracis require 12 to 120h, and are conf...

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Veröffentlicht in:Journal of microbiological methods 2015-11, Vol.118, p.51-56
Hauptverfasser: Cox, Christopher R., Jensen, Kirk R., Mondesire, Roy R., Voorhees, Kent J.
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Sprache:eng
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Zusammenfassung:New, rapid point-of-need diagnostic methods for Bacillus anthracis detection can enhance civil and military responses to accidental or deliberate dispersal of anthrax as a biological weapon. Current laboratory-based methods for clinical identification of B. anthracis require 12 to 120h, and are confirmed by plaque assay using the well-characterized γ typing phage, which requires an additional minimum of 24h for bacterial culture. To reduce testing time, the natural specificity of γ phage amplification was investigated in combination with lateral flow immunochromatography (LFI) for rapid, point-of-need B. anthracis detection. Phage-based LFI detection of B. anthracis Sterne was validated over a range of bacterial and phage concentrations with optimal detection achieved in as little as 2h from the onset of amplification with a threshold sensitivity of 2.5×104cfu/mL. The novel use of γ phage amplification detected with a simple, inexpensive LFI assay provides a rapid, sensitive, highly accurate, and field-deployable method for diagnostic ID of B. anthracis in a fraction of the time required by conventional techniques, and without the need for extensive laboratory culture. •We exploited phage amplification for rapid point-of-need B. anthracis detection.•Species-specific amplification was combined with LFI for simple, accurate detection.•Detection was achieved in two hours with a sensitivity of ~2.5×104cfu/mL.•Results were achieved in a fraction of the time required by conventional assays.
ISSN:0167-7012
1872-8359
DOI:10.1016/j.mimet.2015.08.011