Toxicity Screening of Fungal Extracts and Metabolites, Xenobiotic Chemicals, and Indoor Dusts with In Vitro and Ex Vivo Bioassay Methods

Author:

Hintikka Tuomas1ORCID,Andersson Maria A.12,Lundell Taina1ORCID,Marik Tamás3,Kredics László3ORCID,Mikkola Raimo2ORCID,Andersson Magnus C.4,Kurnitski Jarek25ORCID,Salonen Heidi26

Affiliation:

1. Department of Microbiology, Faculty of Agriculture and Forestry, University of Helsinki, 00014 Helsinki, Finland

2. Department of Civil Engineering, Aalto University, 00076 Espoo, Finland

3. Department of Microbiology, Faculty of Science and Informatics, University of Szeged, H-6726 Szeged, Hungary

4. Department of Production Animal Medicine, Faculty of Veterinary Medicine, University of Helsinki, 04920 Saarentaus, Finland

5. Department of Civil Engineering and Architecture, Tallinn University of Technology, Ehitajate Tee 5, 19086 Tallinn, Estonia

6. International Laboratory for Air Quality and Health, Faculty of Science, School of Earth & Atmospheric Sciences, Queensland University of Technology, 2 George Street, Brisbane, QLD 4000, Australia

Abstract

It is controversial how useful bioassays are for identifying the in vivo toxicity of hazardous environmental exposures. In this study, fruiting bodies of forest mushrooms (n = 46), indoor mold colonies (n = 412), fungal secondary metabolites (n = 18), xenobiotic chemicals such as biocides and detergents (n = 6), and methanol extracts of indoor dusts from urban buildings (n = 26) were screened with two different bioactivity assays: boar sperm motility inhibition (BSMI) and inhibition of cell proliferation (ICP) tests. For the forest mushrooms, the toxicity testing result was positive for 100% of poisonous-classified species, 69% of non-edible-classified species, and 18% of edible-classified species. Colonies of 21 isolates of Ascomycota mold fungal species previously isolated from water-damaged buildings proved to be toxic in the tests. Out of the fungal metabolites and xenobiotic chemicals, 94% and 100% were toxic, respectively. Out of the indoor dusts from moldy-classified houses (n = 12) and from dry, mold-free houses (n = 14), 50% and 57% were toxic, respectively. The bioassay tests, however, could not differentiate the samples from indoor dusts of moldy-classified buildings from those from the mold-free buildings. Xenobiotic chemicals and indoor dusts were more toxic in the BSMI assay than in the ICP assay, whereas the opposite results were obtained with the Ascomycota mold colonies and fungal secondary metabolites. The tests recognized unknown methanol-soluble thermoresistant substances in indoor settled dusts. Toxic indoor dusts may indicate a harmful exposure, regardless of whether the toxicity is due to xenobiotic chemicals or microbial metabolites.

Funder

Research Council of Finland

Publisher

MDPI AG

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