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water-damaged building materials, two aflatoxin producing strains of Aspergillus
flavus (American Type Culture Collection 16875 and 15547) were inoculated onto
culture media, plain wallboard, and vinyl wallpapered wallboard (cellulose-based and
wheat-based wallpaper paste) and incubated at high relative humidity and room temperature
for up to 16 weeks. Each sample was extracted with 60% methanol and aflatoxins in the
crude extract were collected by immunoaffinity chromatography and quantified by
fluorometry. Analysis by high performance liquid chromatography was performed for
confirmation. Varying degrees of fungal growth were evident on all tested substrate types.
Up to 4800 ppb of aflatoxin was detected when strain ATCC 16875 was grown on potato
dextrose agar. However, when inoculation was standardized to minimize initial aflatoxin
concentration in the inoculum, aflatoxin production was not detected on any wallboard
sample under any of the incubation conditions provided. The presence of a toxigenic fungal
strain on an indoor substrate does not necessarily indicate that the fungus is producing
mycotoxins and our data provide evidence that wet wallboard is unlikely to provide
appropriate conditions for aflatoxin production.
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