Limit of detection ofSalmonellaser. Enteritidis using culture-based versus culture-independent diagnostic approaches

Author:

Bradford L.M.ORCID,Yao L.,Anastasiadis C.,Cooper A.L.,Blais B.,Deckert A.,Reid-Smith R.,Lau C.,Diarra M.S.,Carrillo C.,Wong A.ORCID

Abstract

ABSTRACTIn order to prevent the spread of foodborne illnesses, the presence of pathogens in the food chain is monitored by government agencies and food producers. The culture-based methods currently employed are sensitive but time-and labour-intensive, leading to increasing interest in exploring culture-independent diagnostic tests (CIDTs) for pathogen detection. However, sensitivity and reliability of these CIDTs relative to current approaches has not been well established. To address this issue, we conducted a comparison of the limit of detection (LOD50) forSalmonellabetween a culture-based method and three CIDT methods: qPCR (targetinginvAandstn), metabarcode (16S) sequencing, and shotgun metagenomic sequencing. Samples of chicken feed and chicken caecal contents were spiked withSalmonellaserovar Enteritidis and subjected to culture-and DNA-based detection methods. To explore the impact of non-selective enrichment on LOD50, all samples underwent both immediate DNA extraction and an overnight enrichment prior to gDNA extraction. In addition to this spike-in experiment, feed and caecal samples acquired from the field were tested with culturing, qPCR, and metabarcoding. In general, LOD50was comparable between qPCR and shotgun sequencing methods. Overnight microbiological enrichment resulted in an improvement in LOD50with up to a three log decrease, comparable to culture-based detection. However,Salmonellareads were detected in some unspiked feed samples, suggesting false-positive detection ofSalmonella. Additionally, the LOD50in feeds was three logs lower than in caecal contents, underscoring the impact of background microbiota onSalmonelladetection using all methods.IMPORTANCEThe appeal of CIDTs is increased speed with lowered cost, as well as the potential to detect multiple pathogen species in a single analysis and to monitor other areas of concern such as antimicrobial resistance genes or virulence factors. Understanding the sensitivity of CIDTs relative to current approaches will help determine the feasibility of implementing these methods in pathogen surveillance programs.

Publisher

Cold Spring Harbor Laboratory

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