Detection of the ectomycorrhizal fungusTricholoma matsutake and some related species with specific ITS primers |
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| Authors: | William Alexander Dunstan Bernard Dell Nicholas Malajczuk Koji Iwase |
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| Affiliation: | (1) Present address: School of Biological Sciences & Biotechnology, Murdoch University, 6150 Perth, Western Australia, Australia;(2) CSIRO Forestry & Forest Products, CSIRO Centre for Mediterranean Agricultural Research, 6014 Wembley, Western Australia, Australia;(3) Biological Environment Institute, Kansai Environmental Engineering Centre Co., Ltd., 8-4, Ujimatafuri, Uji, 611-0021 Kyoto, Japan |
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| Abstract: | Oligonucleotide primers (Tm1 and Tm4) were designed to amplify a 447–448 base pair fragment, comprising sections of the rDNA internal transcribed spacers (ITS) and the entire 5.8S rDNA, ofTricholoma matsutake. PCR products of predicted size were produced for six of eight isolates ofT. matsutake from across its natural range in Asia, and for isolates of some closely related fungi includingT. bakamatsutake, T. magnivelare, andT. caligatum. The closely relatedT. robustum could be discriminated fromT. matsutake by PCR fragment size. No PCR products were produced where the primers were tested against 16 species of ectomycorrhizal fungi associated withPinus spp. in the Southern Hemisphere. The specific primers were also used successfully to produce PCR products from matsutake infected roots collected in natural forests in China and Japan, and from pure culture synthesisedPinus radiata-T. matsutake material. These primers will be useful in research directed at establishing matsutake in the Southern Hemisphere, and also have the potential to be applied to the study of matsutake within its natural range. |
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| Keywords: | ectomycorrhizas internal transcribed spacers polymerase chain reaction Tricholoma matsutake |
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