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Genetics and Molecular Biology

A Viability Quantitative PCR Dilemma: Are Longer Amplicons Better?

Wannes Van Holm, Justien Ghesquière, Nico Boon, Tim Verspecht, Kristel Bernaerts, Naiera Zayed, Ioanna Chatzigiannidou, Wim Teughels
Maia Kivisaar, Editor
Wannes Van Holm
aDepartment of Oral Health Sciences, University of Leuven (KU Leuven), Leuven, Belgium
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Justien Ghesquière
bBio- and Chemical Systems Technology, Reactor Engineering and Safety, Department of Chemical Engineering, University of Leuven (KU Leuven), Leuven, Belgium
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Nico Boon
cCenter for Microbial Ecology and Technology (CMET), Ghent University (UGent), Ghent, Belgium
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Tim Verspecht
aDepartment of Oral Health Sciences, University of Leuven (KU Leuven), Leuven, Belgium
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Kristel Bernaerts
bBio- and Chemical Systems Technology, Reactor Engineering and Safety, Department of Chemical Engineering, University of Leuven (KU Leuven), Leuven, Belgium
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Naiera Zayed
aDepartment of Oral Health Sciences, University of Leuven (KU Leuven), Leuven, Belgium
dFaculty of Pharmacy, Menoufia University, Shebeen El-Kom, Egypt
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Ioanna Chatzigiannidou
cCenter for Microbial Ecology and Technology (CMET), Ghent University (UGent), Ghent, Belgium
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Wim Teughels
aDepartment of Oral Health Sciences, University of Leuven (KU Leuven), Leuven, Belgium
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Maia Kivisaar
University of Tartu
Roles: Editor
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DOI: 10.1128/AEM.02653-20
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ABSTRACT

The development of viability quantitative PCR (v-qPCR) has allowed for a more accurate assessment of the viability of a microbial sample by limiting the amplification of DNA from dead cells. Although valuable, v-qPCR is not infallible. One of the most limiting factors for accurate live/dead distinction is the length of the qPCR amplicon used. However, no consensus or guidelines exist for selecting and designing amplicon lengths for optimal results. In this study, a wide range of incrementally increasing amplicon lengths (68 to 906 base pairs [bp]) was used on live and killed cells of nine bacterial species treated with a viability dye (propidium monoazide [PMA]). Increasing amplicon lengths up to approximately 200 bp resulted in increasing quantification cycle (Cq) differences between live and killed cells while maintaining a good qPCR efficiency. Longer amplicon lengths, up to approximately 400 bp, further increased the Cq difference but at the cost of qPCR efficiency. Above 400 bp, no valuable increase in Cq differences was observed.

IMPORTANCE Viability quantitative PCR (v-qPCR) has evolved into a valuable, mainstream technique for determining the number of viable microorganisms in samples by qPCR. Amplicon length is known to be positively correlated with the ability to distinguish between live and dead bacteria but is negatively correlated with qPCR efficiency. This trade-off is often not taken into account and might have an impact on the accuracy of v-qPCR data. Currently, there is no consensus on the optimal amplicon length. This paper provides methods to determine the optimal amplicon length and suggests an amplicon length range for optimal v-qPCR, taking into consideration the trade-off between qPCR efficiency and live/dead distinction.

FOOTNOTES

    • Received 29 October 2020.
    • Accepted 12 December 2020.
    • Accepted manuscript posted online 23 December 2020.
  • Supplemental material is available online only.

  • Copyright © 2021 American Society for Microbiology.

All Rights Reserved.

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A Viability Quantitative PCR Dilemma: Are Longer Amplicons Better?
Wannes Van Holm, Justien Ghesquière, Nico Boon, Tim Verspecht, Kristel Bernaerts, Naiera Zayed, Ioanna Chatzigiannidou, Wim Teughels
Applied and Environmental Microbiology Feb 2021, 87 (5) e02653-20; DOI: 10.1128/AEM.02653-20

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A Viability Quantitative PCR Dilemma: Are Longer Amplicons Better?
Wannes Van Holm, Justien Ghesquière, Nico Boon, Tim Verspecht, Kristel Bernaerts, Naiera Zayed, Ioanna Chatzigiannidou, Wim Teughels
Applied and Environmental Microbiology Feb 2021, 87 (5) e02653-20; DOI: 10.1128/AEM.02653-20
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KEYWORDS

viability
vitality
v-qPCR
propidium monoazide
PMA
qPCR efficiency
biofilm
microbiome

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