A PCR-based method for detecting the mycelia of stipitate hydnoid fungi in soil |
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Authors: | van der Linde Sietse Alexander Ian Anderson Ian C |
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Affiliation: | The Macaulay Institute, Craigiebuckler, Aberdeen, AB15 8QH, United Kingdom; University of Aberdeen, School of Biological Sciences (Plant & Soil Sciences), St Machar Drive, Cruickshank Building, Aberdeen, AB24 3UU, United Kingdom. |
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Abstract: | To reduce the reliance on sporocarp records for conservation efforts, information on the below-ground distribution of specific fungal species, such as stipitate hydnoid fungi, is required. Species-specific primers were developed within the internal transcribed spacer (ITS1 and ITS2) regions for 12 hydnoid fungal species including Bankera fuligineoalba, Hydnellum aurantiacum, H. caeruleum, H. concrescens, H. ferrugineum, H. peckii, Phellodon confluens, P. melaleucus, P. niger, P. tomentosus, Sarcodon glaucopus and S. squamosus. The specificity of the primer pairs was tested using BLAST searches and PCR amplifications. All primers amplified DNA only of the target species with the exception of those designed for P. melaleucus. In order to assess the ability of the primers to detect DNA from mycelium in soil, DNA extracted from soil samples taken from around solitary H. peckii sporocarps was amplified with the H. peckii primer 1peck and ITS2. H. peckii DNA was detected in 70% of all soil samples and up to 40 cm away from the base of individual sporocarps. The development of these species-specific primers provides a below-ground alternative for monitoring the distribution of these rare fungi. |
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Keywords: | Below-ground detection Ectomycorrhizal fungi ECM mycelium Rare fungi Species-specific primers Stipitate hydnoid fungi |
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