Challenging the "gold standard" of colony-forming units - Validation of a multiplex real-time PCR for quantification of viable Campylobacter spp. in meat rinses

Kerstin Stingl; Janine Heise; Maja Thieck; Imke F Wulsten; Ewa Pacholewicz; Azuka N Iwobi; Janani Govindaswamy; Véronique Zeller-Péronnet; Sandra Scheuring; Huong Quynh Luu; Vala Fridriksdottir; Greta Gölz; Florian Priller; Igor Gruntar; Frieda Jorgensen; Miriam Koene; Jasna Kovac; Sonja Lick; Elisabeth Répérant; Annika Rohlfing; Anna Zawilak-Pawlik; Marko Rossow; Anja Schlierf; Kirstin Frost; Kirsten Simon; Steffen Uhlig; Ingrid Huber

doi:10.1016/j.ijfoodmicro.2021.109417

Challenging the "gold standard" of colony-forming units - Validation of a multiplex real-time PCR for quantification of viable Campylobacter spp. in meat rinses

Int J Food Microbiol. 2021 Dec 2:359:109417. doi: 10.1016/j.ijfoodmicro.2021.109417. Epub 2021 Sep 24.

Authors

Kerstin Stingl¹, Janine Heise², Maja Thieck², Imke F Wulsten², Ewa Pacholewicz³, Azuka N Iwobi⁴, Janani Govindaswamy⁴, Véronique Zeller-Péronnet⁴, Sandra Scheuring⁴, Huong Quynh Luu⁵, Vala Fridriksdottir⁶, Greta Gölz⁷, Florian Priller⁸, Igor Gruntar⁹, Frieda Jorgensen¹⁰, Miriam Koene¹¹, Jasna Kovac¹², Sonja Lick¹³, Elisabeth Répérant¹⁴, Annika Rohlfing¹⁵, Anna Zawilak-Pawlik¹⁶, Marko Rossow¹⁷, Anja Schlierf¹⁸, Kirstin Frost¹⁸, Kirsten Simon¹⁸, Steffen Uhlig¹⁸, Ingrid Huber⁴

Affiliations

¹ German Federal Institute for Risk Assessment (BfR), Department of Biological Safety, National Reference Laboratory for Campylobacter, Berlin, Germany. Electronic address: kerstin.stingl@bfr.bund.de.
² German Federal Institute for Risk Assessment (BfR), Department of Biological Safety, National Reference Laboratory for Campylobacter, Berlin, Germany.
³ German Federal Institute for Risk Assessment (BfR), Department of Biological Safety, National Reference Laboratory for Campylobacter, Berlin, Germany; Wageningen Bioveterinary Research, Lelystad, the Netherlands.
⁴ Bavarian Health and Food Safety Authority (LGL), Oberschleissheim, Germany.
⁵ National Institute of Veterinary Research (NIVR), Hanoi, Viet Nam.
⁶ Institute for Experimental Pathology at Keldur, Reykjavík, Iceland.
⁷ Freie Universitaet Berlin, Institute of Food Safety and Food Hygiene, Berlin, Germany.
⁸ BIOTECON Diagnostics GmbH, Potsdam, Germany.
⁹ University of Ljubljana, Institute of Microbiology and Parasitology, Ljubljana, Slovenia.
¹⁰ Public Health England, Food, Water and Environmental Laboratory - Porton, Salisbury, United Kingdom.
¹¹ Wageningen Bioveterinary Research, Lelystad, the Netherlands.
¹² The Pennsylvania State University, Department of Food Science, State College, PA, United States.
¹³ Max Rubner-Institute (MRI), Department of Safety and Quality of Meat, Kulmbach, Germany.
¹⁴ ANSES, Laboratoire de Ploufragan-Plouzané-Niort, Ploufragan, France.
¹⁵ Impetus GmbH & Co. Bioscience KG, Microbiology, Bremerhaven, Germany.
¹⁶ Hirszfeld Institute of Immunology and Experimental Therapy, PAS, Microbiology Department, Wroclaw, Poland.
¹⁷ State Office for Consumer Protection Saxony-Anhalt, Department of Food Safety, Halle (Saale), Germany.
¹⁸ QuoData Quality & Statistics, Dresden, Germany.

PMID: 34624596
DOI: 10.1016/j.ijfoodmicro.2021.109417

Abstract

Campylobacter jejuni is the leading bacterial food-borne pathogen in Europe. Despite the accepted limits of cultural detection of the fastidious bacterium, the "gold standard" in food microbiology is still the determination of colony-forming units (CFU). As an alternative, a live/dead differentiating qPCR has been established, using propidium monoazide (PMA) as DNA-intercalating crosslink agent for inactivating DNA from dead, membrane-compromised cells. The PMA treatment was combined with the addition of an internal sample process control (ISPC), i.e. a known number of dead C. sputorum cells to the samples. The ISPC enables i), monitoring the effective reduction of dead cell signal by the light-activated DNA-intercalating dye PMA, and ii), compensation for potential DNA losses during processing. Here, we optimized the method for routine application and performed a full validation of the method according to ISO 16140-2:2016(E) for the quantification of live thermophilic Campylobacter spp. in meat rinses against the classical enumeration method ISO 10272-2:2017. In order to render the method applicable and cost-effective for practical application, the ISPC was lyophilized to be distributable to routine laboratories. In addition, a triplex qPCR was established to simultaneously quantify thermophilic Campylobacter, the ISPC and an internal amplification control (IAC). Its performance was statistically similar to the two duplex qPCRs up to a contamination level of 4.7 log₁₀Campylobacter per ml of meat rinse. The limit of quantification (LOQ) of the alternative method was around 20 genomic equivalents per PCR reaction, i.e. 2.3 log₁₀ live Campylobacter per ml of sample. The alternative method passed a relative trueness study, confirming the robustness against different meat rinses, and displayed sufficient accuracy within the limits set in ISO 16140-2:2016(E). Finally, the method was validated in an interlaboratory ring trial, confirming that the alternative method was fit for purpose with a tendency of improved repeatability and reproducibility compared to the reference method for CFU determination. Campylobacter served as a model organism, challenging CFU as "gold standard" and could help in guidance to the general acceptance of live/dead differentiating qPCR methods for the detection of food-borne pathogens.

Keywords: Enumeration; Food safety; Interlaboratory validation; Propidium monoazide; VBNC.

MeSH terms

Azides
Campylobacter* / genetics
DNA, Bacterial
Food Microbiology
Meat*
Propidium
Real-Time Polymerase Chain Reaction
Reproducibility of Results
Stem Cells

Substances

Azides
DNA, Bacterial
Propidium