Simultaneous quantification of the most common and proteolytic Pseudomonas species in raw milk by multiplex qPCR

Christopher Maier; Katharina Hofmann; Christopher Huptas; Siegfried Scherer; Mareike Wenning; Genia Lücking

doi:10.1007/s00253-021-11109-0

Simultaneous quantification of the most common and proteolytic Pseudomonas species in raw milk by multiplex qPCR

Appl Microbiol Biotechnol. 2021 Feb;105(4):1693-1708. doi: 10.1007/s00253-021-11109-0. Epub 2021 Feb 1.

Authors

Christopher Maier¹, Katharina Hofmann¹, Christopher Huptas², Siegfried Scherer^{1

2}, Mareike Wenning³, Genia Lücking⁴

Affiliations

¹ ZIEL Institute for Food and Health, Wissenschaftszentrum Weihenstephan, Technische Universität München, Weihenstephaner Berg 1, 85354, Freising, Germany.
² Lehrstuhl für Mikrobielle Ökologie, Wissenschaftszentrum Weihenstephan, Technische Universität München, Weihenstephaner Berg 3, 85354, Freising, Germany.
³ Bavarian Health and Food Safety Authority (LGL), Veterinärstr. 2, 85764, Oberschleißheim, Germany.
⁴ ZIEL Institute for Food and Health, Wissenschaftszentrum Weihenstephan, Technische Universität München, Weihenstephaner Berg 1, 85354, Freising, Germany. genia.luecking@tum.de.

Abstract

The heat-stable peptidase AprX, secreted by psychrotolerant Pseudomonas species in raw milk, is a major cause of destabilization and premature spoilage of ultra-high temperature (UHT) milk and milk products. To enable rapid detection and quantification of seven frequent and proteolytic Pseudomonas species (P. proteolytica, P. gessardii, P. lactis, P. fluorescens, P. protegens, P. lundensis, and P. fragi) in raw milk, we developed two triplex qPCR assays taking into account species-dependent differences in AprX activity. Besides five species-specific hydrolysis probes, targeting the aprX gene, a universal rpoB probe was included in the assay to determine the total Pseudomonas counts. For all six probes, linear regression lines between C_q value and target DNA concentration were obtained in singleplex as well as in multiplex approaches, yielding R² values of > 0.975 and amplification efficiencies of 85-97%. Moreover, high specificity was determined using genomic DNA of 75 Pseudomonas strains, assigned to 57 species, and 40 other bacterial species as templates in the qPCR. Quantification of the target species and total Pseudomonas counts resulted in linear detection ranges of approx. 10³-10⁷ cfu/ml, which correspond well to common Pseudomonas counts in raw milk. Application of the assay using 60 raw milk samples from different dairies showed good agreement of total Pseudomonas counts calculated by qPCR with cell counts derived from cultivation. Furthermore, a remarkably high variability regarding the species composition was observed for each milk sample, whereby P. lundensis and P. proteolytica/P. gessardii were the predominant species detected. KEY POINTS: • Multiplex qPCR for quantification of seven proteolytic Pseudomonas species and total Pseudomonas counts in raw milk • High specificity and sensitivity via hydrolysis probes against aprX and rpoB • Rapid method to determine Pseudomonas contamination in raw milk and predict spoilage potential.

Keywords: Multiplex quantitative PCR; Proteolytic milk spoilage; Pseudomonas; aprX.

MeSH terms

Animals
Hot Temperature
Milk* / metabolism
Peptide Hydrolases / metabolism
Proteolysis
Pseudomonas* / genetics
Pseudomonas* / metabolism

Substances

Peptide Hydrolases