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Modern Methods in Cereal Grain Mycology
Modern Methods in
Cereal Grain Mycology
Johan Olsson
Department of Microbiology
Uppsala
Doctoral thesis
Swedish University of Agricultural Sciences
Uppsala 2000
Acta Universitatis Agriculturae Sueciae
Agraria 24 1
ISSN 1401-6249
ISBN 91-576-5792-0
02000 Johan Olson, Uppsala
Tryck: SLU Service/Repro, Uppsala 2000
Abstract
Olsson, J. 2000. Modem methods in cereal grain mycology. Doctors dissertation.
ISSN 1401-6249, ISBN 91-576-5792-0.
A simple rapid DNA extraction method, equally suitable for spores and mycelia is
proposed. Heating samples in NaOH and SDS provides DNA of high purity, suitable for
Polymerase Chain Reaction (PCR) analysis. For Penicillium roqueforti the detection limit
was 6 x lo3 conidia and 1 mg (fresh weight) mycelium in the extraction liquid. The
method proved efficient with Aspergillus jlavus, Fusarium graminearum, Rhizopus
stolonifer, Eurotium herbariorum, and Cladosporium herbarum, as well.
An optimised competitive PCR (cPCR) method for quantifying fungal growth in
cereal grain was developed using experimental design. DNA extraction efficiency was
quantified by cPCR using primers specific for the internal transcribed spacers (ITS) of the
ribosomal DNA of P. roqueforti. The proposed method can detect P. roqueforti at levels
as low as 10 CFU/g grain and at levels higher than lo2 CFU/g grain. Quantification is
consistent (CV 8%) and highly correlated with results from traditional dilution plating.
The possibilities of using an electronic nose or gas chromatography combined with
mass spectrometry (GC-MS) to quantify ergosterol, colony forming units (CFU),
ochratoxin A, and deoxynivalenol
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