Your search keyword '"Merker, N."' showing total 2 results

1. Diagnosis of invasive fungal infections in haematological patients by combined use of galactomannan, 1,3-β-D-glucan, Aspergillus PCR, multifungal DNA-microarray, and Aspergillus azole resistance PCRs in blood and bronchoalveolar lavage samples: results of a prospective multicentre study

Author

Boch, T., Spiess, B., Cornely, O.A., Vehreschild, J.J., Rath, P.M., Steinmann, J., Heinz, W.J., Hahn, J., Krause, S.W., Kiehl, M.G., Egerer, G., Liebregts, T., Koldehoff, M., Klein, M., Nolte, F., Mueller, M.C., Merker, N., Will, S., Mossner, M., and Popp, H.

Subjects

*MYCOSES, *GALACTOMANNANS, *ASPERGILLUS, *BRONCHOALVEOLAR lavage, *DNA microarrays

Abstract

High mortality rates of invasive fungal disease (IFD), especially invasive aspergillosis (IA), in immunocompromised haematological patients and current diagnostic limitations require improvement of detection of fungal pathogens by defining the optimal use of biomarkers and clinical samples. Concurrent bronchoalveolar lavage (BAL) and peripheral blood samples of 99 haematological patients with suspected IFD were investigated within a multicentre prospective study. Diagnostic performance of a galactomannan (GM) enzyme immune assay (EIA), a 1,3-β-D-glucan assay (BDG), an Aspergillus PCR, and a multifungal DNA-microarray (Chip) alone or in combination were calculated. IFD were classified as proven ( n =3), probable ( n =34), possible ( n =33), and no IFD ( n =29) according to EORTC/MSG criteria. GM, PCR, and Chip showed superior diagnostic performance in BAL than in blood, whereas specificity of BDG in BAL was poor (48% (14/29)). The combination of GM (BAL) with BDG (blood) showed sensitivity, specificity, positive predictive value (PPV), negative predictive value (NPV), and DOR (diagnostic odds ratio) of 92% (34/37), 93% (27/29), 94%, 90%, and 153.0, respectively. Combining GM (BAL) with PCR (BAL) showed convincing diagnostic potential for diagnosing IA with sensitivity, specificity, PPV, NPV, and DOR of 85% (17/20), 97% (28/29), 94%, 90%, and 158.7. Addition of the DNA-microarray resulted in further detection of two mucormycetes infections. In 1 out of 15 Aspergillus DNA-positive samples a triazole resistance-mediating Cyp51A mutation was found. Combination of biomarkers is superior to their sole use in diagnosing IFD, particularly IA. Integrating blood and BAL samples into a diagnostic algorithm is an advantageous approach. [ABSTRACT FROM AUTHOR]

Published

2016

2. Identification of invasive fungal diseases in immunocompromised patients by combining an Aspergillus specific PCR with a multifungal DNA-microarray from primary clinical samples.

Author

Boch, T., Reinwald, M., Postina, P., Cornely, O. A., Vehreschild, J. J., Heußel, C. P., Heinz, W. J., Hoenigl, M., Eigl, S., Lehrnbecher, T., Hahn, J., Claus, B., Lauten, M., Egerer, G., Müller, M. C., Will, S., Merker, N., Hofmann, W.‐K., Buchheidt, D., and Spiess, B.

Subjects

*ASPERGILLOSIS diagnosis, *DIAGNOSIS, *MYCOSES, *IMMUNOCOMPROMISED patients, *HISTOPATHOLOGY, *DNA microarrays, *POLYMERASE chain reaction

Abstract

The increasing incidence of invasive fungal diseases ( IFD), most of all invasive aspergillosis ( IA) in immunocompromised patients emphasises the need to improve the diagnostic tools for detection of fungal pathogens. We investigated the diagnostic performance of a multifungal DNA-microarray detecting 15 different fungi [ Aspergillus, Candida, Fusarium, Mucor, Rhizopus, Scedosporium and Trichosporon species (spp.)] in addition to an Aspergillus specific polymerase chain reaction ( PCR) assay. Biopsies, bronchoalveolar lavage and peripheral blood samples of 133 immunocompromised patients (pts) were investigated by a multifungal DNA-microarray as well as a nested Aspergillus specific PCR assay. Patients had proven ( n = 18), probable ( n = 29), possible ( n = 48) and no IFD ( n = 38) and were mostly under antifungal therapy at the time of sampling. The results were compared to culture, histopathology, imaging and serology, respectively. For the non- Aspergillus IFD the microarray analysis yielded in all samples a sensitivity of 64% and a specificity of 80%. Best results for the detection of all IFD were achieved by combining DNA-microarray and Aspergillus specific PCR in biopsy samples (sensitivity 79%; specificity 71%). The molecular assays in combination identify genomic DNA of fungal pathogens and may improve identification of causative pathogens of IFD and help overcoming the diagnostic uncertainty of culture and/or histopathology findings, even during antifungal therapy. [ABSTRACT FROM AUTHOR]

Published

2015