Differentiation of S. chartarum (Ehrenb.) S. Hughes Chemotypes A and S via FT-IR Spectroscopy.

Fourier-transform-infrared spectroscopy Macrocyclic trichothecenes Stachybotrys chartarum Triplex PCR

Journal

Mycopathologia
ISSN: 1573-0832
Titre abrégé: Mycopathologia
Pays: Netherlands
ID NLM: 7505689

Informations de publication

Date de publication:
Dec 2020
Historique:
received: 17 06 2020
accepted: 24 09 2020
pubmed: 11 10 2020
medline: 4 9 2021
entrez: 10 10 2020
Statut: ppublish

Résumé

Stachybotrys (S.) chartarum is a cellulolytic mould with the ability to produce highly cytotoxic macrocyclic trichothecenes. Two chemotypes are defined according to their ability to produce either atranones or satratoxins. S. chartarum has been well known as the causative agent of the lethal disease stachybotryotoxicosis in horses. Further investigations revealed that this disease is strictly correlated with the presence of macrocyclic trichothecenes. Furthermore, their occurrence in water-damaged buildings has been linked to adverse health effects such as the sick building syndrome. As the chemotypes cannot be characterized via phenotypic criteria, different methods such as PCR, MALDI-TOF MS, LC-MS/MS, thin-layer chromatography and cytotoxicity assays have been used so far. Fourier-transform-infrared spectroscopy (FT-IR) is commonly used for the differentiation of bacteria and yeasts, but this technique is also applicable to filamentous fungi. Hence, this study aimed at evaluating to which extent a reliable differentiation of S. chartarum chemotypes A and S is possible. Besides, another objective was to verify if the recently introduced third genotype of S. chartarum can be identified. Therefore, 28 strains including the two chemotypes and the third genotype H were cultivated on malt extract agar (MEA) and potato dextrose agar in three biological replicates. Each sample was applied to FT-IR measurements on day 7, 14 and 21 of cultivation. In this study, we achieved a distinction of the chemotypes A and S via FT-IR spectroscopy after incubation for 7 days on MEA. In terms of genotype differentiation, the PCR detecting satratoxin- and atranone-gene clusters remained the only applicable method.

Identifiants

pubmed: 33037964
doi: 10.1007/s11046-020-00495-0
pii: 10.1007/s11046-020-00495-0
pmc: PMC7779419
doi:

Types de publication

Journal Article

Langues

eng

Sous-ensembles de citation

IM

Pagination

993-1004

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Auteurs

Julia Ekruth (J)

Chair of Food Safety, Faculty of Veterinary Medicine, Ludwig-Maximilians-University Munich, Schoenleutnerstr. 8, 85764, Oberschleissheim, Germany. Julia.Ekruth@ls.vetmed.uni-muenchen.de.

Christoph Gottschalk (C)

Chair of Food Safety, Faculty of Veterinary Medicine, Ludwig-Maximilians-University Munich, Schoenleutnerstr. 8, 85764, Oberschleissheim, Germany.

Sebastian Ulrich (S)

Chair of Food Safety, Faculty of Veterinary Medicine, Ludwig-Maximilians-University Munich, Schoenleutnerstr. 8, 85764, Oberschleissheim, Germany.
Bacteriology and Mycology, Institute for Infectious Diseases and Zoonoses, Department of Veterinary Science, Faculty of Veterinary Medicine, Ludwig-Maximilians-University Munich, Veterinaerstr. 13, 80539, Munich, Germany.

Manfred Gareis (M)

Chair of Food Safety, Faculty of Veterinary Medicine, Ludwig-Maximilians-University Munich, Schoenleutnerstr. 8, 85764, Oberschleissheim, Germany.

Karin Schwaiger (K)

Chair of Food Safety, Faculty of Veterinary Medicine, Ludwig-Maximilians-University Munich, Schoenleutnerstr. 8, 85764, Oberschleissheim, Germany.

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Classifications MeSH