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Rapid and Sensitive Multiplex Assay for the Detection of B. anthracis Spores from Environmental Samples

Prompt and accurate detection of Bacillus anthracis spores is crucial in the event of intentional spore dissemination in order to reduce the number of expected casualties. Specific identification of these spores from environmental samples is both challenging and time-consuming. This is due to the hi...

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Autores principales: Makdasi, Efi, Laskar, Orly, Glinert, Itai, Alcalay, Ron, Mechaly, Adva, Levy, Haim
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2020
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7157734/
https://www.ncbi.nlm.nih.gov/pubmed/32120986
http://dx.doi.org/10.3390/pathogens9030164
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author Makdasi, Efi
Laskar, Orly
Glinert, Itai
Alcalay, Ron
Mechaly, Adva
Levy, Haim
author_facet Makdasi, Efi
Laskar, Orly
Glinert, Itai
Alcalay, Ron
Mechaly, Adva
Levy, Haim
author_sort Makdasi, Efi
collection PubMed
description Prompt and accurate detection of Bacillus anthracis spores is crucial in the event of intentional spore dissemination in order to reduce the number of expected casualties. Specific identification of these spores from environmental samples is both challenging and time-consuming. This is due to the high homology with other Bacillus species as well as the complex composition of environmental samples, which further impedes assay sensitivity. Previously, we showed that a short incubation of B.anthracis spores in a defined growth medium results in rapid germination, bacterial growth, and secretion of toxins, including protective antigen. In this work, we tested whether coupling the incubation process to a newly developed immune-assay will enable the detection of secreted toxins as markers for the presence of spores in environmental samples. The new immune assay is a flow cytometry-based multiplex that simultaneously detects a protective antigen, lethal factor, and edema factor. Our combined assay detects 1 × 10(3)–1 × 10(4)/mL spores after a 2 h incubation followed by the ~80 min immune-multiplex detection. Extending the incubation step to 5 h increased assay sensitivity to 1 × 10(2)/mL spore. The protocol was validated in various environmental samples using attenuated or fully virulent B. anthracis spores. There was no substantial influence of contaminants derived from real environmental samples on the performance of the assay compared to clean samples, which allow the unequivocal detection of 3 × 10(3)/mL and 3 × 10(2)/mL spores following 2 and 5 hour’s incubation, respectively. Overall, we propose this method as a rapid, sensitive, and specific procedure for the identification of B. anthracis spores in environmental samples.
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spelling pubmed-71577342020-04-21 Rapid and Sensitive Multiplex Assay for the Detection of B. anthracis Spores from Environmental Samples Makdasi, Efi Laskar, Orly Glinert, Itai Alcalay, Ron Mechaly, Adva Levy, Haim Pathogens Article Prompt and accurate detection of Bacillus anthracis spores is crucial in the event of intentional spore dissemination in order to reduce the number of expected casualties. Specific identification of these spores from environmental samples is both challenging and time-consuming. This is due to the high homology with other Bacillus species as well as the complex composition of environmental samples, which further impedes assay sensitivity. Previously, we showed that a short incubation of B.anthracis spores in a defined growth medium results in rapid germination, bacterial growth, and secretion of toxins, including protective antigen. In this work, we tested whether coupling the incubation process to a newly developed immune-assay will enable the detection of secreted toxins as markers for the presence of spores in environmental samples. The new immune assay is a flow cytometry-based multiplex that simultaneously detects a protective antigen, lethal factor, and edema factor. Our combined assay detects 1 × 10(3)–1 × 10(4)/mL spores after a 2 h incubation followed by the ~80 min immune-multiplex detection. Extending the incubation step to 5 h increased assay sensitivity to 1 × 10(2)/mL spore. The protocol was validated in various environmental samples using attenuated or fully virulent B. anthracis spores. There was no substantial influence of contaminants derived from real environmental samples on the performance of the assay compared to clean samples, which allow the unequivocal detection of 3 × 10(3)/mL and 3 × 10(2)/mL spores following 2 and 5 hour’s incubation, respectively. Overall, we propose this method as a rapid, sensitive, and specific procedure for the identification of B. anthracis spores in environmental samples. MDPI 2020-02-27 /pmc/articles/PMC7157734/ /pubmed/32120986 http://dx.doi.org/10.3390/pathogens9030164 Text en © 2020 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Makdasi, Efi
Laskar, Orly
Glinert, Itai
Alcalay, Ron
Mechaly, Adva
Levy, Haim
Rapid and Sensitive Multiplex Assay for the Detection of B. anthracis Spores from Environmental Samples
title Rapid and Sensitive Multiplex Assay for the Detection of B. anthracis Spores from Environmental Samples
title_full Rapid and Sensitive Multiplex Assay for the Detection of B. anthracis Spores from Environmental Samples
title_fullStr Rapid and Sensitive Multiplex Assay for the Detection of B. anthracis Spores from Environmental Samples
title_full_unstemmed Rapid and Sensitive Multiplex Assay for the Detection of B. anthracis Spores from Environmental Samples
title_short Rapid and Sensitive Multiplex Assay for the Detection of B. anthracis Spores from Environmental Samples
title_sort rapid and sensitive multiplex assay for the detection of b. anthracis spores from environmental samples
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7157734/
https://www.ncbi.nlm.nih.gov/pubmed/32120986
http://dx.doi.org/10.3390/pathogens9030164
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