Evaluation of a multiplex PCR method to serotype Salmonella in animal feeds pre-enrichment broth cultures

Junia Jean-Gilles Beaubrun,Laura Ewing,Kim Dudley,Faiza Benhamed,Hua Wang,Darcy E Hanes

doi:10.1016/j.mex.2017.09.003

Abstract

The identification of Salmonella enterica serotypes remains a highly important public health concern for microbiological analysis of foods, feeds, and clinical samples. Outbreaks of human salmonellosis are sometimes linked to contact with infected animals and animal feeds. To possibly reduce the number of outbreaks, it is important to rapidly, efficiently detect Salmonella enterica in animal feeds and food products. A multiplex PCR for molecular serotyping of Salmonella enterica previously used in a single lab validation study for serotyping in multiple human food matrices was used in this investigation to evaluate the effectiveness of the multiplex PCR assay as serotyping method and screening tool for Salmonella in animal feeds. This approach is unique in that:•The multiplex PCR serotyping assay may be used for rapid screening and serotyping of Salmonella enterica from contaminated animal feed at the non-selective pre-enrichment step.•The assay may provide the serotype or identification of Salmonella in positive samples at concentration as low as 10 CFU/25g after a 24h non-selective pre-enrichment step.•In addition to the ability to serotype, this assay contains invA as an internal control for Salmonella positive identification. The invA shows positive indication for Salmonella outside of the 30 serotypic banding patterns.

Highlights

Salmonella enterica is a leading cause of food-borne illness and is a serious public health concern
Using a method described by Benhamed et al [5] six feeds: Wheat Brand (WB), Horse Feed (HF), Dried Molasses (DM), Calf Milk Replacer (CMR), Dried Beet Pulp (DBP), and Whole Oats (OT) obtained from commercial sources were spiked with S. enterica serovar Typhimurium at concentrations of 10 CFU, 50 CFU, 100 CFU per 25 g, to evaluate the detection level using a modified version of the Bacteriological Analytical Manual (BAM), Chapter 5 [1]
A total of 92 samples were analyzed per feed type, 40 feed samples pre-enriched in lactose broth and 40 feed samples pre-enriched in modified buffer peptone water (mBPW)

Summary

Method Article

Evaluation of a multiplex PCR method to serotype Salmonella in animal feeds pre-enrichment broth cultures. Junia Jean-Gilles Beaubruna,*, Laura Ewinga, Kim Dudleya, Faiza Benhamedb, Hua Wangc, Darcy E. Hanesa a U.S Food and Drug Administration, Center for Food Safety and Applied Nutrition, Laurel, MD 207081, United States b U.S Food and Drug Administration, Center for Veterinary Medicine, Laurel, MD 20708, United States c U.S Food and Drug Administration, Center for Food Safety and Applied Nutrition, College Park, MD 20740, United States. Detection and serotyping of Salmonella enterica from 24 h pre-enrichment of animal feed

Methods

Findings

Background