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Journal of microbiological methods
04, 2024;219 106895.

Optimized bacterial absolute quantification method by qPCR using an exogenous bacterial culture as a normalization strategy in triple-species BV-like biofilms.

In��s Lameira, Ana S Pinto, ��ngela Lima, Christina A Muzny, Nuno Cerca
Author Information
  1. In��s Lameira: Centre of Biological Engineering (CEB), Laboratory of Research in Biofilms Ros��rio Oliveira (LIBRO), University of Minho, Campus de Gualtar, Braga, Portugal.
  2. Ana S Pinto: Centre of Biological Engineering (CEB), Laboratory of Research in Biofilms Ros��rio Oliveira (LIBRO), University of Minho, Campus de Gualtar, Braga, Portugal.
  3. ��ngela Lima: Centre of Biological Engineering (CEB), Laboratory of Research in Biofilms Ros��rio Oliveira (LIBRO), University of Minho, Campus de Gualtar, Braga, Portugal.
  4. Christina A Muzny: Division of Infectious Diseases, University of Alabama at Birmingham, Birmingham, AL, United States.
  5. Nuno Cerca: Centre of Biological Engineering (CEB), Laboratory of Research in Biofilms Ros��rio Oliveira (LIBRO), University of Minho, Campus de Gualtar, Braga, Portugal; LABBELS -Associate Laboratory, Braga, Guimar��es, Portugal. Electronic address: nunocerca@ceb.uminho.pt.
PMID: 38331102 DOI: 10.1016/j.mimet.2024.106895

Abstract

Quantitative Polymerase Chain Reaction (qPCR) is a widely used method in molecular biology to quantify target DNA sequences. Despite its accuracy, there are important experimental controls that should be considered to avoid biased results. One of them is gDNA loss during extraction, which is higher among samples with lower bacterial concentrations. Improvement in qPCR quantification procedures is mandatory to obtain reproducible and accurate results. Herein, we report an improved qPCR method for bacterial quantification of Gardnerella vaginalis, Prevotella bivia, and Fannyhessea vaginae, three key-bacterial vaginosis (BV)-associated bacteria (BVAB) thought to play important roles in the pathogenesis of this common vaginal infection. The formation of a mature biofilm on vaginal epithelial cells is an unique feature of BV and, despite over 60 years of research, the exact etiology of BV remains unknown. Here, we optimized a qPCR method that accurately quantified triple-species biofilms containing these key BVAB, after the addition of an exogenous bacterial control containing a fixed concentration of Escherichia coli, prior to gDNA extraction. This improved method minimized and normalized the inherent losses associated with bacterial centrifugation, which allows better sensitivity at lower bacterial concentrations.

Keywords

Bacterial quantification Bacterial vaginosis Calibration curves Centrifugation loss Exogenous control qPCR

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Grants

  1. R01 AI146065/NIAID NIH HHS

MeSH Term

Female
Humans
Vaginosis, Bacterial
Gardnerella vaginalis
Bacteria
Biofilms
Vagina
Journal Article Research Support, Non-U.S. Gov't Research Support, N.I.H., Extramural

Word Cloud

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