April
2010
, Volume
94
, Number
4
Pages
432
-
438
Authors
Thomas Sundelin, Department of Plant Biology and Biotechnology, Faculty of Life Sciences, University of Copenhagen, Thorvaldsensvej 40, DK-1871 Frederiksberg, Denmark;
Camilla Beck Christensen, Department of Plant Biology and Biotechnology, Faculty of Life Sciences, University of Copenhagen, and Department of Integrated Pest Management, Faculty of Agricultural Sciences, University of Aarhus, Forsøgsvej 1, DK-4200 Slagelse, Denmark;
John Larsen and
Kaare Møller, Department of Integrated Pest Management, Faculty of Agricultural Sciences, University of Aarhus;
Mette Lübeck, Section for Sustainable Biotechnology, Department of Biotechnology, Chemistry and Environmental Engineering, Copenhagen Institute of Technology, Aalborg University, Lautrupvang 15, DK-2750 Ballerup, Denmark;
Lars Bødker, Department of Integrated Pest Management, Faculty of Agricultural Sciences, University of Aarhus; and
Birgit Jensen, Department of Plant Biology and Biotechnology, Faculty of Life Sciences, University of Copenhagen, and Department of Integrated Pest Management, Faculty of Agricultural Sciences, University of Aarhus
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RelatedArticle
Accepted for publication 11 December 2009.
Abstract
ABSTRACT
Until now, molecular and biochemical methods have only been used to show whether or not Plasmodiophora brassicae is present in plant or soil samples but not to what extent. Here, in planta quantification of P. brassicae by whole-cell fatty acid (WCFA) measurements and real-time polymerase chain reaction (PCR) was evaluated. Arachidonic acid (ARA, 20:4) was the most abundant fatty acid in resting spores and was only found in infected roots, which indicates a potential of ARA as a biomarker for P. brassicae. A real-time PCR assay was developed using primers designed from the internal transcribed spacer region of the ribosomal DNA. Using these primers, it was possible to detect P. brassicae in infected roots 10 days after germination of plants sown in infested soil. A bioassay showed that the amounts of ARA found by WCFA analysis and the DNA found by real-time PCR in infected plants were well correlated. These measurements also correlated with the soil spore content and the assessed disease incidence and disease severity scores. Therefore, we conclude that WCFA analysis and real-time PCR are good tools for P. brassicae quantification that can be applied to basic studies of the pathogen and in resistance screens.
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© 2010 The American Phytopathological Society
