application of pcr-rflp to rapid identification of the main pathogenic dermatophytes from clinical specimens

نویسندگان

h mirzahoseini dept. of biotechnology, pasteur institute of iran, tehran, iran

e omidinia dept. of biotechnology, pasteur institute of iran, tehran, iran

m shams-ghahfarokhi dept. of mycology, faculty of medical sciences, tarbiat modares university, tehran, iran

g sadeghi dept. of mycology, faculty of medical sciences, tarbiat modares university, tehran, iran

چکیده

background: in the present study, a pcr-rflp based molecular technique was designed to rapid identification of der­matophytes in clinical specimens. skin scrapings obtained from human cases suspected to dermatophytosis were studied in or­der to identify involved etiological fungi. methods: in this experimental study, the specimens (skin scrapings) of patients referred to mycology department of pas­teur institute of iran were inoculated on petri dishes contained selective agar for pathogenic fungi (sapf) and incubated at 25º c until visible growth of fungal colonies. the colonies were examined for standard morphological characteristics after visi­ble growth on the agar medium. a small portion of each fungal colony was further studied by restriction fragment length poly­morphism (rflp) analysis of the pcr-amplified internal transcribed spacer (its) region of ribosomal dna (rdna). pcr amplicons were electrophoresed on 2% agarose gel after digesting by different restriction enzymes including mva i, hinf i and hae iii. results: among 160 clinical samples examined, 6 dermatophyte species including  trichophyton mentagrophytes, t. ru­brum, t. verrucosum, t. tonsurans, microsporum canis and epidermophyton floccosum were finally identified based on the col­ony morphology and microscopic criteria. specific pcr products and rflp patterns for mva i, hinf i and hae iii en­zymes allowed the rapid identification and reliable differentiation of isolated dermatophytes at the genus or species level for 5-10 day-old colonies. conclusions: the results showed that pcr-rflp analysis of the its region of rdna is a rapid and reliable tool which al­lows identification of major pathogenic dermatophytes isolated in this study at species level in young 5-10 day-old colonies.

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عنوان ژورنال:
iranian journal of public health

جلد ۳۸، شماره ۱، صفحات ۱۸-۲۴

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