Literature DB >> 11158128

Rapid discrimination among dermatophytes, Scytalidium spp., and other fungi with a PCR-restriction fragment length polymorphism ribotyping method.

M Machouart-Dubach1, C Lacroix, M F de Chauvin , I Le Gall , C Giudicelli, F Lorenzo, F Derouin.   

Abstract

Dermatomycoses are very common infections caused mainly by dermatophytes. Scytalidiosis is a differential mycological diagnosis, especially in tropical and subtropical areas. Since a culture-based diagnosis takes 2 to 3 weeks, we set up a PCR-restriction fragment length polymorphism (RFLP) method for rapid discrimination of these fungi in clinical samples. The hypervariable V4 domain of the small ribosomal subunit 18S gene was chosen as the target for PCR. The corresponding sequences from 19 fungal species (9 dermatophytes, 2 Scytalidium species, 6 other filamentous fungi, and 2 yeasts) were obtained from databases or were determined in the laboratory. Sequences were aligned to design primers for dermatophyte-specific PCR and to identify digestion sites for RFLP analysis. The reliability of PCR-RFLP for the diagnosis of dermatomycosis was assessed on fungal cultures and on specimens from patients with suspected dermatomycosis. Two sets of primers preferentially amplified fungal DNA from dermatophytes (DH1L and DH1R) or from Scytalidium spp. (DH2L and DH1R) relative to DNA from bacteria, yeasts, some other filamentous fungi, and humans. Digestion of PCR products with EaeI or BamHI discriminated between dermatophytes and Scytalidium species, as shown with cultures of 31 different fungal species. When clinical samples were tested by PCR-RFLP, blindly to mycological findings, the results of the two methods agreed for 74 of 75 samples. Dermatophytes and Scytalidium spp. can thus be readily discriminated by PCR-RFLP within 24 h. This method can be applied to clinical samples and is suited to rapid etiologic diagnosis and treatment selection for patients with dermatomycosis.

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Year:  2001        PMID: 11158128      PMCID: PMC87797          DOI: 10.1128/JCM.39.2.685-690.2001

Source DB:  PubMed          Journal:  J Clin Microbiol        ISSN: 0095-1137            Impact factor:   5.948


  15 in total

1.  Molecular taxonomy and GC/MS of metabolites of Scytalidium hyalinum and Nattrassia mangiferae (Hendersonula toruloidea).

Authors:  H J Roeijmans; G S De Hoog; C S Tan; M J Figge
Journal:  J Med Vet Mycol       Date:  1997 May-Jun

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4.  A phylogenetic analysis of the genus Saccharomyces based on 18S rRNA gene sequences: description of Saccharomyces kunashirensis sp. nov. and Saccharomyces martiniae sp. nov.

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Journal:  Int J Syst Bacteriol       Date:  1997-04

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6.  Polymerase chain reaction-based detection of dermatophyte DNA with a fungus-specific primer system.

Authors:  M Bock; M Maiwald; R Kappe; P Nickel; H Näher
Journal:  Mycoses       Date:  1994 Mar-Apr       Impact factor: 4.377

Review 7.  Hendersonula toruloidea and Scytalidium hyalinum. Review and update.

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8.  Hendersonula toruloidea as an agent of mycotic foot infection in Gabon.

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9.  A U.S. epidemiologic survey of superficial fungal diseases.

Authors:  M E Kemna; B E Elewski
Journal:  J Am Acad Dermatol       Date:  1996-10       Impact factor: 11.527

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Journal:  Mycoses       Date:  1996 Jan-Feb       Impact factor: 4.377

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  8 in total

1.  Identification of infectious agents in onychomycoses by PCR-terminal restriction fragment length polymorphism.

Authors:  Julie Verrier; Marina Pronina; Corinne Peter; Olympia Bontems; Marina Fratti; Karine Salamin; Stéphanie Schürch; Katia Gindro; Jean-Luc Wolfender; Keith Harshman; Michel Monod
Journal:  J Clin Microbiol       Date:  2011-12-14       Impact factor: 5.948

Review 2.  Conventional methods for the diagnosis of dermatophytosis.

Authors:  Raymond Robert; Marc Pihet
Journal:  Mycopathologia       Date:  2008-05-14       Impact factor: 2.574

3.  Molecular analysis of fungal microbiota in samples from healthy human skin and psoriatic lesions.

Authors:  Luciana C Paulino; Chi-Hong Tseng; Bruce E Strober; Martin J Blaser
Journal:  J Clin Microbiol       Date:  2006-08       Impact factor: 5.948

Review 4.  Diagnosis of Dermatophytosis Using Molecular Biology.

Authors:  Julie Verrier; Michel Monod
Journal:  Mycopathologia       Date:  2016-08-01       Impact factor: 2.574

5.  Multicenter evaluation of a commercial PCR-enzyme-linked immunosorbent assay diagnostic kit (Onychodiag) for diagnosis of dermatophytic onychomycosis.

Authors:  C Savin; S Huck; C Rolland; M Benderdouche; O Faure; G Noacco; J Menotti; E Candolfi; H Pelloux; R Grillot; S Coupe; F Derouin
Journal:  J Clin Microbiol       Date:  2007-02-07       Impact factor: 5.948

6.  Optimization of PCR-RFLP Directly from the Skin and Nails in Cases of Dermatophytosis, Targeting the ITS and the 18S Ribosomal DNA Regions.

Authors:  Elangovan Elavarashi; Anupma Jyoti Kindo; Jagannathan Kalyani
Journal:  J Clin Diagn Res       Date:  2013-02-12

7.  Application of polymerase chain reaction (PCR) and PCR based restriction fragment length polymorphism for detection and identification of dermatophytes from dermatological specimens.

Authors:  R Bagyalakshmi; B Senthilvelan; K L Therese; S Murugusundram; H N Madhavan
Journal:  Indian J Dermatol       Date:  2008-01       Impact factor: 1.494

8.  High prevalence of mixed infections in global onychomycosis.

Authors:  Aditya K Gupta; Valeria B A Taborda; Paulo R O Taborda; Avner Shemer; Richard C Summerbell; Kerry-Ann Nakrieko
Journal:  PLoS One       Date:  2020-09-29       Impact factor: 3.240

  8 in total

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