Genetic variation, real-time PCR, metabolites and mycotoxins ofFusarium avenaceum and related species |
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Authors: | T. Yli-Mattila S. Paavanen-Huhtala P. Parikka M. Jestoi S. S. Klemsdal A. Rizzo |
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Affiliation: | (1) Laboratory of Plant Physiology and Molecular Biology, Dept of Biology, Univ. of Turku, 20014 Turku, Finland;(2) Plant Production Research, MTT Agrifood Research Finland, FIN-31600 Jokioinen, Finland;(3) Department of Chemistry, National Veterinary and Food Research Institute (EELA), 00581 Helsinki, Finland;(4) Plant Health and Plant Protection Division, Bioforsk-Norwegian Institute of Agricultural and Environmental Research, Hoegskoleveien 7, 1432 Aas, Norway |
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Abstract: | In this paper the latest studies dealing with genetic variation and mycotoxins ofF. avenaceum and related species are reviewed and compared to the data from chromatographic image analyses. Forty-three European strains ofFusarium avenaceum and related species were classified by chromatographic image analysis on full chromatographic matrices. The results were in most cases in agreement with those from morphological and molecular analyses and supported the separation betweenF. avenaceum, F. arthrosporioides andF. tricinctum and betweenF. avenaceum groups I and II. The mycotoxin profiles of the FinnishF. avenaceum, F. arthrosporioides andF tricinctum strains were very similar to each other. Moniliformin and enniatins were the main mycotoxins produced. A fluorogenic TaqMan PCR assay (qPCR) was used for the detection ofF. avenaceum/ F. arthrosporioides DNA in Finnish barley and wheat. The qPCR results obtained from grain samples were compared to mycotoxin levels. A correlation was found betweenF. avenaceum/F. arthrosporioides DNA and moniliformin (MON) and enniatin (ENNs) levels in barley. A correlation was also found between the combinedF. avenaceum/F. arthrosporioides/F. tricinctum contamination and MON and ENNs levels in barley in 2002, but not in 2003. This was probably due to the higher MON and ENNs levels in 2002 than in 2003. It was possible to use the DNA levels ofF. avenaceum/F. arthrosporioides to distinguish between most barley samples containing high amounts of MON and ENNs from those containing low levels of the mycotoxins. Presented at the EU-USA Bilateral Workshop on Toxigenic Fungi & Mycotoxins, New Orleans, USA, July 5–7, 2005 Financial support: Grants from the National Technology Agency of Finland (No. 40168/03) and the Academy of Finland (No. 52104); travel grants from NorFA and the European Commission to the Laboratory of Dr. Ulf Thrane |
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Keywords: | Fusarium avenaceum mycotoxins real-time PCR metabolite profiles Gibberella avenacea |
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