A multicenter study on accuracy and reproducibility of nanopore sequencing-based genotyping of bacterial pathogens

Author:

Dabernig-Heinz Johanna1ORCID,Lohde Mara2,Hölzer Martin3,Cabal Adriana4,Conzemius Rick5,Brandt Christian2,Kohl Matthias6,Halbedel Sven78ORCID,Hyden Patrick4,Fischer Martin A.9,Pietzka Ariane10ORCID,Daza Beatriz4ORCID,Idelevich Evgeny A.11ORCID,Stöger Anna4,Becker Karsten11ORCID,Fuchs Stephan3,Ruppitsch Werner4ORCID,Steinmetz Ivo1ORCID,Kohler Christian11ORCID,Wagner Gabriel E.1ORCID

Affiliation:

1. Diagnostic and Research Institute of Hygiene, Microbiology and Environmental Medicine, Medical University of Graz, Graz, Austria

2. Institute for Infectious Diseases and Infection Control, Jena University Hospital, Jena, Germany

3. Genome Competence Center (MF1), Robert Koch Institute, Berlin, Germany

4. Austrian Agency for Health and Food Safety, Vienna, Austria

5. Ares Genetics GmbH, Vienna, Austria

6. Medical and Life Sciences Faculty, Furtwangen University, Villingen-Schwenningen, Germany

7. Nosocomial Pathogens and Antibiotic Resistances (FG13), Robert Koch Institute, Wernigerode, Germany

8. Institute for Medical Microbiology and Hospital Hygiene, Otto von Guericke University Magdeburg, Magdeburg, Germany

9. Enteropathogenic bacteria and Legionella (FG11), Consultant Laboratory for Listeria, Robert Koch Institute, Wernigerode, Germany

10. Austrian Agency for Health and Food Safety, Graz, Austria

11. Friedrich Loeffler Institute for Medical Microbiology, F.-Sauerbruch-Str., Greifswald, Germany

Abstract

ABSTRACT Nanopore sequencing has shown the potential to democratize genomic pathogen surveillance due to its ease of use and low entry cost. However, recent genotyping studies showed discrepant results compared to gold-standard short-read sequencing. Furthermore, although essential for widespread application, the reproducibility of nanopore-only genotyping remains largely unresolved. In our multicenter performance study involving five laboratories, four public health-relevant bacterial species were sequenced with the latest R10.4.1 flow cells and V14 chemistry. Core genome MLST analysis of over 500 data sets revealed highly strain-specific typing errors in all species in each laboratory. Investigation of the methylation-related errors revealed consistent DNA motifs at error-prone sites across participants at read level. Depending on the frequency of incorrect target reads, this either leads to correct or incorrect typing, whereby only minimal frequency deviations can randomly determine the final result. PCR preamplification, recent basecalling model updates and an optimized polishing strategy notably diminished the non-reproducible typing. Our study highlights the potential for new errors to appear with each newly sequenced strain and lays the foundation for computational approaches to reduce such typing errors. In conclusion, our multicenter study shows the necessity for a new validation concept for nanopore sequencing-based, standardized bacterial typing, where single nucleotide accuracy is critical.

Funder

Ministry for Economics, Sciences and Digital Society of Thuringia

Publisher

American Society for Microbiology

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