Highly accurate and sensitive absolute quantification of bacterial strains in human fecal samples

Fuyong Li; Junhong Liu; María X. Maldonado-Gómez; Steven A. Frese; Michael G. Gänzle; Jens Walter

doi:10.1186/s40168-024-01881-2

Microbiome (Sep 2024)

Highly accurate and sensitive absolute quantification of bacterial strains in human fecal samples

Fuyong Li,
Junhong Liu,
María X. Maldonado-Gómez,
Steven A. Frese,
Michael G. Gänzle,
Jens Walter

Affiliations

Fuyong Li: Department of Animal Science and Technology, College of Animal Sciences, Zhejiang University
Junhong Liu: Department of Agricultural, Food and Nutritional Science, University of Alberta
María X. Maldonado-Gómez: One Bio Inc.
Steven A. Frese: Department of Nutrition, University of Nevada
Michael G. Gänzle: Department of Agricultural, Food and Nutritional Science, University of Alberta
Jens Walter: Department of Agricultural, Food and Nutritional Science, University of Alberta

DOI: https://doi.org/10.1186/s40168-024-01881-2
Journal volume & issue: Vol. 12, no. 1
pp. 1 – 16

Abstract

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Abstract Background Next-generation sequencing (NGS) approaches have revolutionized gut microbiome research and can provide strain-level resolution, but these techniques have limitations in that they are only semi-quantitative, suffer from high detection limits, and generate data that is compositional. The present study aimed to systematically compare quantitative PCR (qPCR) and droplet digital PCR (ddPCR) for the absolute quantification of Limosilactobacillus reuteri strains in human fecal samples and to develop an optimized protocol for the absolute quantification of bacterial strains in fecal samples. Results Using strain-specific PCR primers for L. reuteri 17938, ddPCR showed slightly better reproducibility, but qPCR was almost as reproducible and showed comparable sensitivity (limit of detection [LOD] around 104 cells/g feces) and linearity (R 2 > 0.98) when kit-based DNA isolation methods were used. qPCR further had a wider dynamic range and is cheaper and faster. Based on these findings, we conclude that qPCR has advantages over ddPCR for the absolute quantification of bacterial strains in fecal samples. We provide an optimized and easy-to-follow step-by-step protocol for the design of strain-specific qPCR assays, starting from primer design from genome sequences to the calibration of the PCR system. Validation of this protocol to design PCR assays for two L. reuteri strains, PB-W1 and DSM 20016 T, resulted in a highly accurate qPCR with a detection limit in spiked fecal samples of around 103 cells/g feces. Applying our strain-specific qPCR assays to fecal samples collected from human subjects who received live L. reuteri PB-W1 or DSM 20016 T during a human trial demonstrated a highly accurate quantification and sensitive detection of these two strains, with a much lower LOD and a broader dynamic range compared to NGS approaches (16S rRNA gene sequencing and whole metagenome sequencing). Conclusions Based on our analyses, we consider qPCR with kit-based DNA extraction approaches the best approach to accurately quantify gut bacteria at the strain level in fecal samples. The provided step-by-step protocol will allow scientists to design highly sensitive strain-specific PCR systems for the accurate quantification of bacterial strains of not only L. reuteri but also other bacterial taxa in a broad range of applications and sample types. Video Abstract

Published in Microbiome

ISSN: 2049-2618 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Science: Microbiology: Microbial ecology
Website: https://microbiomejournal.biomedcentral.com

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Abstract

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