Isolation and Detection of Extended Spectrum β-Lactamase (ESBL)-Producing Enterobacteriaceae from Meat using Chromogenic Agars and Isothermal Loop-Mediated Amplification (LAMP) Assays

The aim of this work was to develop a molecular method using loop‐mediated isothermal amplification (LAMP) for detection of extended spectrum β‐lactamase (ESBL)‐producing Enterobacteriaceae from meat, and to compare it with different isolation agars and microarrays. LAMP assays were developed for CT...

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Bibliographic Details
Published in:	Journal of food science Vol. 78; no. 12; pp. M1892 - M1898
Main Authors:	Anjum, M.F., Lemma, F., Cork, D.J., Meunier, D., Murphy, N., North, S.E., Woodford, N., Haines, J., Randall, L.P.
Format:	Journal Article
Language:	English
Published:	Hoboken, NJ Blackwell Publishing Ltd 01-12-2013 Wiley
Subjects:	Animals Anti-Bacterial Agents antibiotic resistance beta-Lactamases - metabolism Biological and medical sciences Cattle Chicken Chickens CTX-M Culture Media Enterobacteriaceae Enterobacteriaceae - enzymology Enterobacteriaceae - isolation & purification ESBLs Food Contamination - analysis Food industries Food Microbiology Fundamental and applied biological sciences. Psychology meat Meat - microbiology Nucleic Acid Amplification Techniques Reproducibility of Results Sensitivity and Specificity Sheep, Domestic Swine Enzyme Poultry Meat product Agar ESBLs β-Lactamase Spectrum Meat Amplification Resistance CTX-M Vertebrata Antibiotic Meat animals Analysis method antibiotic resistance Bacteria Hydrolases Isolation Control method Chicken Aves Detection Enterobacteriaceae meat
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Summary:	The aim of this work was to develop a molecular method using loop‐mediated isothermal amplification (LAMP) for detection of extended spectrum β‐lactamase (ESBL)‐producing Enterobacteriaceae from meat, and to compare it with different isolation agars and microarrays. LAMP assays were developed for CTX‐M groups 1, 2, and 9 and OXA‐10‐like genes. Chicken, lamb, beef, pork, and turkey samples were spiked with 10, 100, and 1,000 cfu/gram using 8 strains of ESBL‐producing Enterobacteriaceae (CTX‐M sequence types 1, 2, 3, 14, 15, OXA‐11, SHV‐2, TEM‐52) +/– a mix of competitor organisms. Samples were enriched overnight in buffered peptone water (BPW) +/– antibacterials before plating to CHROMagar CTX, OXOID ESBL Brilliance agar, and MacConkey agar with 1 mg/L cefotaxime. Selected BPW broths were also tested using LAMP assays, microarrays and using cefpodoxime discs on agar. For isolation/detection of ESBL producers from beef, pork, lamb, and turkey spiked with 10 or 100 cfu/gram ESBL (natural flora only), all agars and the LAMP assays showed 100% sensitivity and specificity for ESBL spike strains. For chicken samples, both LAMP and chromogenic agars showed improved sensitivity and specificity for isolation of ESBLs compared with MacConkey agar, particularly with competitor bacteria added. In comparison, the cefpodoxime disc method and microarray showed reduced sensitivity. Practical application Isolation and detection of ESBL‐producing Enterobacteriaceae from meat is an important part of monitoring for food safety as such organisms can cause disease in humans. The LAMP assays developed in this study combined with use of chromogenic agars have the potential to provide robust, rapid detection, isolation, and preliminary characterization of ESBLs in meat.
Bibliography:	ark:/67375/WNG-4WZ79JB1-2 FSA - No. FS241023 istex:6A5B45B107A52A593BEF23D958498799A90E5ACB ArticleID:JFDS12297 ObjectType-Article-1 SourceType-Scholarly Journals-1 ObjectType-Feature-2 content type line 23
ISSN:	0022-1147 1750-3841
DOI:	10.1111/1750-3841.12297