Two multiplex PCRs, based on 10 taxon-specific primers designed on rDNA regions, were developed for the identification of taxa within the lignivorous genera Ganoderma, Inonotus s.l. and Phellinus s.l., each comprising both secondary and primary aggressive decay fungi. Each multiplex PCR proved to correctly identify 1 ÷ 10-2 pg of fungal target DNA directly from wood. This method can be helpful to detect decay in standing trees independently of its stage of advancement, and to identify the associated decay agents.

A PCR-based method for the identification of important wood rotting fungal taxa within Ganoderma, Inonotus s.l. and Phellinus s.l.

GUGLIELMO, FABIO;GONTHIER, Paolo;NICOLOTTI, Giovanni
2008-01-01

Abstract

Two multiplex PCRs, based on 10 taxon-specific primers designed on rDNA regions, were developed for the identification of taxa within the lignivorous genera Ganoderma, Inonotus s.l. and Phellinus s.l., each comprising both secondary and primary aggressive decay fungi. Each multiplex PCR proved to correctly identify 1 ÷ 10-2 pg of fungal target DNA directly from wood. This method can be helpful to detect decay in standing trees independently of its stage of advancement, and to identify the associated decay agents.
2008
282 (2)
228
237
multiplex PCR; rDNA; taxon-specific primer; wood decay.
GUGLIELMO F; GONTHIER P; GARBELOTTO M; NICOLOTTI G.
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/2318/27843
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