Laboratory detection of Clostridium difficile in piglets in Australia

D.R. Knight; M.M. Squire; T.V. Riley

doi:10.1128/JCM.01225-14

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Laboratory detection of Clostridium difficile in piglets in Australia

Journal article

Peer reviewed

Laboratory detection of Clostridium difficile in piglets in Australia

D.R. Knight, M.M. Squire and T.V. Riley

Journal of Clinical Microbiology, Vol.52(11), pp.3856-3862

2014

DOI: https://doi.org/10.1128/JCM.01225-14

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Abstract

Clostridium difficile is a well-known enteric pathogen of humans and the causative agent of high-morbidity enteritis in piglets aged 1 to 7 days. C. difficile prevalence in Australian piglets is as high as 70%. The current diagnostic assays have been validated only for human infections, and there are no published studies assessing their performance in Australian piglets. We evaluated the suitability of five assays for detecting C. difficile in 157 specimens of piglet feces. The assays included a loop-mediated isothermal amplification (LMIA)-PCR for tcdA (illumigene C. difficile; Meridian), a real-time PCR for tcdB (GeneOhm Cdiff; Becton Dickinson), two-component enzyme immunoassays (EIA) for C. difficile glutamate dehydrogenase (GDH) (EIA-GDH) and TcdA/TcdB (EIA-TcdA/TcdB) (C. diff Quik Chek; Alere), and direct culture (DC) (C. difficile chromID agar; bioMérieux). The assays for detection of the organism were compared against enrichment culture (EC), and assays for detection of toxins/toxin genes were compared against EC followed by PCR for toxin genes (toxigenic EC [TEC]). The recovery of C. difficile by EC was 39.5% (n = 62/157), and TEC revealed that 58.1% (n = 36/62) of isolates were positive for at least one toxin gene (tcdA/tcdB). Compared with those for EC/TEC, the sensitivities, specificities, positive predictive values, and negative predictive values were, respectively, as follows: DC, 91.9, 100.0, 100.0, and 95.0%; EIA-GDH, 41.9, 92.6, 78.8, and 71.0%; EIA-TcdA/TcdB, 5.6, 99.2, 66.7, and 77.9%; real-time PCR, 42.9, 96.7, 78.9, and 85.4% and LMIA-PCR, 25.0, 95.9, 64.3, and 81.1%. The performance of the molecular methods was poor, suggesting that the current commercially available assays for diagnosis of C. difficile in humans are not suitable for use in piglets. C. difficile recovery by the DC provides a cost-effective alternative.

Details

Title: Laboratory detection of Clostridium difficile in piglets in Australia
Authors/Creators: D.R. Knight (Author/Creator) - Queen Elizabeth II Medical Centre
M.M. Squire (Author/Creator) - Queen Elizabeth II Medical Centre
T.V. Riley (Author/Creator) - The University of Western Australia
Publication Details: Journal of Clinical Microbiology, Vol.52(11), pp.3856-3862
Publisher: American Society for Microbiology
Identifiers: 991005545244207891
Copyright: © 2014, American Society for Microbiology.
Murdoch Affiliation: Murdoch University
Language: English
Resource Type: Journal article

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Collaboration types: Domestic collaboration
Citation topics: 1 Clinical & Life Sciences; 1.120 Inflammatory Bowel Diseases & Infections; 1.120.1133 Clostridium Infections
Web Of Science research areas: Microbiology
ESI research areas: Microbiology