The study was conducted in the Parasitology–Mycology laboratory of Farhat Hached hospital (Sousse, Tunisia). The investigated patients were addressed to the laboratory BGB324 by the service of Dermatology of the same hospital and to a lesser extent by private practitioners. Two sample collections were investigated in this study: Two hundred and eighty-one nail specimens were
investigated. They include the following: (i) 201 samples collected from patients with suspected onychomycosis and (ii) 80 nail specimens obtained from healthy individuals with no clinical nor mycological evidence of onychomycosis and considered as negative controls. All collected samples were divided into three portions. The first portion was examined microscopically in 30% KOH for the presence PLX3397 of fungal elements. The second was cultured on Sabouraud dextrose agar supplemented with chloramphenicol and/or cyclohexemide at 27 °C for up to 4 weeks. The third portion of the nail specimen was used for PCR analysis. Clinical isolates were identified at the species level on the basis of macroscopic and microscopic characteristics of the colonies. To optimise the PCR protocol and the specificity of the primers, 70 strains mycologically identified as dermatophytes including 23 T. rubrum (TR), 35 T. mentagrophytes (TM) and five other species obtained from nail scrapings, skin and hair fragments from patients with dermatophytosis were
included. In Pyruvate dehydrogenase addition, six reference strains, 30 non-dermatophyte fungal strains (moulds and yeast) and 2 human DNA specimens were tested (Table 1). Reference strains were purchased from the Central Bureau voor Schimmelcultures (CBS, Utrecht, the Netherlands). DNA was extracted from nail material by using the QiaAmp DNA extraction Kit (Qiagen, Venlo (Pays Bas), Germany). Prior to the extraction, whole nails or relatively large nail fragments weighing between 3 and 5 mg, were cut into small pieces with a surgical blade. Subsequently, nucleic acid extraction was performed according to the manufacturer’s instructions. At the end of the procedure, the DNA pellet was dissolved in 50–70 μl
hydration solution, depending on the amount of the nail material used at the beginning. A quantity of 2 µl of DNA was added to the PCR mixture. To extract DNA from fungal cultures, we used the rapid mini preparation method described by Liu et al. [24] In brief, a small lump of mycelia (1 cm2 of diameter) was added to 500 μl of lysis buffer (Tris–HCl, EDTA, NaCl, SDS) and 150 μl of potassium acetate. The tube was vortexed and an equal volume of isopropyl alcohol was added to the supernatant. Then, the mixture was centrifuged and the resultant DNA pellet was washed in 70% ethanol and dissolved in 50 μl Tris–EDTA. Extracted DNA was kept at −20 °C until use. A quantity of 2 µl of DNA was added in PCR mixture. The nucleotide sequences of the different dermatophytes were selected from the NCBI nucleotide database.
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