PCR-terminal restriction fragment length polymorphism for direct detection and identification of dermatophytes in veterinary mycology.

Med Mycol

Groupe d'Etude des Interactions Hôte-Pathogène (GEIHP, EA 3142), SFR ICAT 4208, UNIV Angers, UNIV Brest, Angers, France.

Published: June 2019

AI Article Synopsis

  • The traditional method for diagnosing dermatophytosis in animals uses microscopy and culture, which can be slow and sensitive to contamination.
  • A new PCR assay using TRFLP was developed to enhance the sensitivity and speed of diagnosis, involving 27 dermatophyte species and confirming its effectiveness on veterinary samples.
  • This PCR-TRFLP method showed high accuracy, correctly identifying dermatophytes in 97.1% of clinically relevant cases, making it a promising tool for veterinary practice.

Article Abstract

The biological diagnosis of dermatophytosis in veterinary medicine usually relies on direct microscopic examination and inoculation of the samples on appropriate culture media. However, identification of dermatophytes needs expertise, and cultures which require from days to weeks to be conclusive, may lack of sensitivity because of the quite common overgrowth of contaminants. Here we developed a polymerase chain reaction (PCR) assay based on terminal restriction fragment length polymorphism (TRFLP), which may improve sensitivity of the biological diagnosis and reduce the delay for initiation of treatment. This study was first conducted on pure cultures of various dermatophytes (27 species), yeasts (14 species) and moulds (45 species). After DNA extraction, the internal transcribed spacer (ITS)-28S region of ribosomal DNA was amplified with primers targeting specifically pathogenic dermatophytes, and species of interest were identified by TRFLP with appropriate restriction enzymes. After validation, this assay was applied to veterinary samples and results were compared to those obtained by direct microscopic examination and cultures. All target species were correctly identified, and none of the yeast or mould species was amplified, demonstrating specificity of the assay. Regarding clinical samples, the causative agent was detected by PCR-TRFLP from 97.1% of the samples with both positive direct microscopic examination and cultures. No dermatophytes were detected when both conventional tests were negative. PCR-TRFLP developed here demonstrated to be highly sensitive and specific, allowing rapid detection and direct identification of dermatophytes in veterinary practice. Therefore, this assay is especially suitable for the biological diagnosis of dermatophytosis in different animal species.

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Source
http://dx.doi.org/10.1093/mmy/myy058DOI Listing

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