Detection and Identification of Fungal Pathogens by PCR and by ITS2 and 5.8S Ribosomal DNA Typing in Ocular Infections

doi:10.1128/JCM.39.8.2873-2879.2001

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Journal of Clinical Microbiology, August 2001, p. 2873-2879, Vol. 39, No. 8
0095-1137/01/$04.00+0 DOI: 10.1128/JCM.39.8.2873-2879.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Detection and Identification of Fungal Pathogens by PCR and by ITS2 and 5.8S Ribosomal DNA Typing in Ocular Infections

Consuelo Ferrer,¹^,^* Francisca Colom,² Susana Frasés,² Emilia Mulet,³ José L. Abad,¹ and Jorge L. Alió¹^,³

Departamento de Biología Molecular, Instituto Oftalmológico de Alicante, 03015 Alicante,¹ and Div. Microbiología,² and Patología y Cirugía-Div. Oftalmología,³ Universidad Miguel Hernández, 03550 Alicante, Spain

Received 14 March 2001/Returned for modification 4 April 2001/Accepted 3 June 2001

The goal of this study was to determine whether sequence analysis of internal transcribed spacer/5.8S ribosomal DNA (rDNA)can be used to detect fungal pathogens in patients with ocularinfections (endophthalmitis and keratitis). Internal transcribedspacer 1 (ITS1) and ITS2 and 5.8S rDNA were amplified by PCR andseminested PCR to detect fungal DNA. Fifty strains of 12 fungalspecies (yeasts and molds) were used to test the selected primersand conditions of the PCR. PCR and seminested PCR of this regionwere carried out to evaluate the sensitivity and specificity ofthe method. It proved possible to amplify the ITS2/5.8S regionof all the fungal strains by this PCR method. All negative controls(human and bacterial DNA) were PCR negative. The sensitivity ofthe seminested PCR amplification reaction by DNA dilutions was1 organism per PCR, and the sensitivity by cell dilutions wasfewer than 10 organisms per PCR. Intraocular sampling or cornealscraping was undertaken for all patients with suspected infectiousendophthalmitis or keratitis (nonherpetic), respectively, betweenNovember 1999 and February 2001. PCRs were subsequently performedwith 11 ocular samples. The amplified DNA was sequenced, and alignedagainst sequences in GenBank at the National Institutes of Health.The results were PCR positive for fungal primers for three cornealscrapings, one aqueous sample, and one vitreous sample; one ofthem was negative by culture. Molecular fungal identificationwas successful in all cases. Bacterial detection by PCR was positivefor three aqueous samples and one vitreous sample; one of thesewas negative by culture. Amplification of ITS2/5.8S rDNA and moleculartyping shows potential as a rapid technique for identifying fungiin ocularsamples.

^* Corresponding author. Mailing address: Dpto. Biología Molecular, Instituto Oftalmológico de Alicante, Avenida de Denia no.111, 03015 Alicante, Spain. Phone: 34 965 154062. Fax: 34 965160468. E-mail: cferre{at}umh.es.

Journal of Clinical Microbiology, August 2001, p. 2873-2879, Vol. 39, No. 8
0095-1137/01/$04.00+0 DOI: 10.1128/JCM.39.8.2873-2879.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

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