A qPCR Assay for the Fast Detection and Quantification of <i>Colletotrichum lupini</i>

Tim Kamber; Nachelli Malpica-López; Monika M. Messmer; Thomas Oberhänsli; Christine Arncken; Joris A. Alkemade; Pierre Hohmann

doi:10.3390/plants10081548

Plants (Jul 2021)

A qPCR Assay for the Fast Detection and Quantification of <i>Colletotrichum lupini</i>

Tim Kamber,
Nachelli Malpica-López,
Monika M. Messmer,
Thomas Oberhänsli,
Christine Arncken,
Joris A. Alkemade,
Pierre Hohmann

Affiliations

Tim Kamber: Department of Crop Sciences, Research Institute of Organic Agriculture (FiBL), Ackerstrasse 113, 5070 Frick, Switzerland
Nachelli Malpica-López: Department of Environmental Sciences, University of Basel, Bernoullistrasse 30/32, 4056 Basel, Switzerland
Monika M. Messmer: Department of Crop Sciences, Research Institute of Organic Agriculture (FiBL), Ackerstrasse 113, 5070 Frick, Switzerland
Thomas Oberhänsli: Department of Crop Sciences, Research Institute of Organic Agriculture (FiBL), Ackerstrasse 113, 5070 Frick, Switzerland
Christine Arncken: Department of Crop Sciences, Research Institute of Organic Agriculture (FiBL), Ackerstrasse 113, 5070 Frick, Switzerland
Joris A. Alkemade: Department of Crop Sciences, Research Institute of Organic Agriculture (FiBL), Ackerstrasse 113, 5070 Frick, Switzerland
Pierre Hohmann: Department of Crop Sciences, Research Institute of Organic Agriculture (FiBL), Ackerstrasse 113, 5070 Frick, Switzerland

DOI: https://doi.org/10.3390/plants10081548
Journal volume & issue: Vol. 10, no. 8
p. 1548

Abstract

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White lupin (Lupinus albus) represents an important legume crop in Europe and other parts of the world due to its high protein content and potential for low-input agriculture. However, most cultivars are susceptible to anthracnose caused by Colletotrichum lupini, a seed- and air-borne fungal pathogen that causes severe yield losses. The aim of this work was to develop a C. lupini-specific quantitative real-time TaqMan PCR assay that allows for quick and reliable detection and quantification of the pathogen in infected seed and plant material. Quantification of C. lupini DNA in dry seeds allowed us to distinguish infected and certified (non-infected) seed batches with DNA loads corresponding to the disease score index and yield of the mother plants. Additionally, C. lupini DNA could be detected in infected lupin shoots and close to the infection site, thereby allowing us to study the disease cycle of this hemibiotrophic pathogen. This qPCR assay provides a useful diagnostic tool to determine anthracnose infection levels of white lupin seeds and will facilitate the use of seed health assessments as a strategy to reduce the primary infection source and spread of this disease.

Published in Plants

ISSN: 2223-7747 (Online)
Publisher: MDPI AG
Country of publisher: Switzerland
LCC subjects: Science: Botany
Website: http://www.mdpi.com/journal/plants

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