General primer-mediated PCR for detection of Aspergillus species.

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J Clin Microbiol. 1994 July; 32(7): 1710-1717

General primer-mediated PCR for detection of Aspergillus species.

W J Melchers, P E Verweij, P van den Hurk, A van Belkum, B E De Pauw, J A Hoogkamp-Korstanje and J F Meis

Department of Medical Microbiology, University Hospital Nijmegen, The Netherlands.

ABSTRACT

A PCR assay was developed for the diagnosis of invasive aspergillosisin immunocompromised patients. For this purpose, the completenucleotide sequences of the genes encoding the 18S rRNA of Aspergillusnidulans, Aspergillus terreus, Aspergillus niger, and Aspergillusflavus were elucidated and aligned to the sequences of Aspergillusfumigatus and other clinically relevant prokaryotic and eukaryoticmicroorganisms. Genus-specific sequences could be identifiedin the V7 to V9 region of 18S rRNA. By using hot-start PCR,Southern blot hybridization, and restriction enzyme analysis,Aspergillus-specific and -sensitive determination was achieved.Five of six immunosuppressed mice experimentally infected withA. fumigatus developed infection, and rRNA could be detectedin each case, even in livers with the absence of positive cultures.Aspergillus species were detected by PCR in four neutropenicpatients with proven aspergillosis, although Aspergillus specieshad been isolated from only one bronchoalveolar lavage (BAL)fluid sample. Aspergillus species were detected by PCR in twomore patients suspected of having infection. Positive PCR signalswere obtained from the BAL samples of 3 of 8 neutropenic patientswho had developed pulmonary infiltrates, but none were obtainedfrom the samples of 14 nonimmunosuppressed patients. These resultsindicate the potential value of PCR to detect Aspergillus speciesin BAL samples and, therefore, to identify neutropenic patientsat risk for invasive aspergillosis.

J Clin Microbiol. 1994 July; 32(7): 1710-1717

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