Real-Time qPCR as a Method for Detection of Antibody-Neutralized Phage Particles

The most common method for phage quantitation is the plaque assay, which relies on phage ability to infect bacteria. However, non-infective phage particles may preserve other biological properties; specifically, they may enter interactions with the immune system of animals and humans. Here, we demon...

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Autores principales: Kłopot, Anna, Zakrzewska, Adriana, Lecion, Dorota, Majewska, Joanna M., Harhala, Marek A., Lahutta, Karolina, Kaźmierczak, Zuzanna, Łaczmański, Łukasz, Kłak, Marlena, Dąbrowska, Krystyna
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Frontiers Media S.A. 2017
Materias:
Microbiology
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5672142/
https://www.ncbi.nlm.nih.gov/pubmed/29163448
http://dx.doi.org/10.3389/fmicb.2017.02170
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author Kłopot, Anna
Zakrzewska, Adriana
Lecion, Dorota
Majewska, Joanna M.
Harhala, Marek A.
Lahutta, Karolina
Kaźmierczak, Zuzanna
Łaczmański, Łukasz
Kłak, Marlena
Dąbrowska, Krystyna
author_facet Kłopot, Anna
Zakrzewska, Adriana
Lecion, Dorota
Majewska, Joanna M.
Harhala, Marek A.
Lahutta, Karolina
Kaźmierczak, Zuzanna
Łaczmański, Łukasz
Kłak, Marlena
Dąbrowska, Krystyna
author_sort Kłopot, Anna
collection PubMed
description The most common method for phage quantitation is the plaque assay, which relies on phage ability to infect bacteria. However, non-infective phage particles may preserve other biological properties; specifically, they may enter interactions with the immune system of animals and humans. Here, we demonstrate real-time quantitative polymerase chain reaction (qPCR) detection of bacteriophages as an alternative to the plaque assay. The closely related staphylococcal bacteriophages A3R and 676Z and the coliphage T4 were used as model phages. They were tested in vivo in mice, ex vivo in human sera, and on plastic surfaces designed for ELISAs. T4 phage was injected intravenously into pre-immunized mice. The phage was completely neutralized by specific antibodies within 5 h (0 pfu/ml of serum, as determined by the plaque assay), but it was still detected by qPCR in the amount of approximately 10(7) pfu/ml of serum. This demonstrates a substantial timelapse between “microbiological disappearance” and true clearance of phage particles from the circulation. In human sera ex vivo, qPCR was also able to detect neutralized phage particles that were not detected by the standard plaque assay. The investigated bacteriophages differed considerably in their ability to immobilize on plastic surfaces: this difference was greater than one order of magnitude, as shown by qPCR of phage recovered from plastic plates. The ELISA did not detect differences in phage binding to plates. Major limitations of qPCR are possible inhibitors of the PCR reaction or free phage DNA, which need to be considered in procedures of phage sample preparation for qPCR testing. We propose that phage pharmacokinetic and pharmacodynamic studies should not rely merely on detection of antibacterial activity of a phage. Real-time qPCR can be an alternative for phage detection, especially in immunological studies of bacteriophages. It can also be useful for studies of phage-based drug nanocarriers or biosensors.
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spelling pubmed-56721422017-11-21 Real-Time qPCR as a Method for Detection of Antibody-Neutralized Phage Particles Kłopot, Anna Zakrzewska, Adriana Lecion, Dorota Majewska, Joanna M. Harhala, Marek A. Lahutta, Karolina Kaźmierczak, Zuzanna Łaczmański, Łukasz Kłak, Marlena Dąbrowska, Krystyna Front Microbiol Microbiology The most common method for phage quantitation is the plaque assay, which relies on phage ability to infect bacteria. However, non-infective phage particles may preserve other biological properties; specifically, they may enter interactions with the immune system of animals and humans. Here, we demonstrate real-time quantitative polymerase chain reaction (qPCR) detection of bacteriophages as an alternative to the plaque assay. The closely related staphylococcal bacteriophages A3R and 676Z and the coliphage T4 were used as model phages. They were tested in vivo in mice, ex vivo in human sera, and on plastic surfaces designed for ELISAs. T4 phage was injected intravenously into pre-immunized mice. The phage was completely neutralized by specific antibodies within 5 h (0 pfu/ml of serum, as determined by the plaque assay), but it was still detected by qPCR in the amount of approximately 10(7) pfu/ml of serum. This demonstrates a substantial timelapse between “microbiological disappearance” and true clearance of phage particles from the circulation. In human sera ex vivo, qPCR was also able to detect neutralized phage particles that were not detected by the standard plaque assay. The investigated bacteriophages differed considerably in their ability to immobilize on plastic surfaces: this difference was greater than one order of magnitude, as shown by qPCR of phage recovered from plastic plates. The ELISA did not detect differences in phage binding to plates. Major limitations of qPCR are possible inhibitors of the PCR reaction or free phage DNA, which need to be considered in procedures of phage sample preparation for qPCR testing. We propose that phage pharmacokinetic and pharmacodynamic studies should not rely merely on detection of antibacterial activity of a phage. Real-time qPCR can be an alternative for phage detection, especially in immunological studies of bacteriophages. It can also be useful for studies of phage-based drug nanocarriers or biosensors. Frontiers Media S.A. 2017-11-06 /pmc/articles/PMC5672142/ /pubmed/29163448 http://dx.doi.org/10.3389/fmicb.2017.02170 Text en Copyright © 2017 Kłopot, Zakrzewska, Lecion, Majewska, Harhala, Lahutta, Kaźmierczak, Łaczmański, Kłak and Dąbrowska. http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) or licensor are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
spellingShingle Microbiology
Kłopot, Anna
Zakrzewska, Adriana
Lecion, Dorota
Majewska, Joanna M.
Harhala, Marek A.
Lahutta, Karolina
Kaźmierczak, Zuzanna
Łaczmański, Łukasz
Kłak, Marlena
Dąbrowska, Krystyna
Real-Time qPCR as a Method for Detection of Antibody-Neutralized Phage Particles
title Real-Time qPCR as a Method for Detection of Antibody-Neutralized Phage Particles
title_full Real-Time qPCR as a Method for Detection of Antibody-Neutralized Phage Particles
title_fullStr Real-Time qPCR as a Method for Detection of Antibody-Neutralized Phage Particles
title_full_unstemmed Real-Time qPCR as a Method for Detection of Antibody-Neutralized Phage Particles
title_short Real-Time qPCR as a Method for Detection of Antibody-Neutralized Phage Particles
title_sort real-time qpcr as a method for detection of antibody-neutralized phage particles
topic Microbiology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5672142/
https://www.ncbi.nlm.nih.gov/pubmed/29163448
http://dx.doi.org/10.3389/fmicb.2017.02170
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