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A new mechanism for reduced sensitivity to demethylation‐inhibitor fungicides in the fungal banana black Sigatoka pathogen Pseudocercospora fijiensis
Authors:Caucasella Diaz‐Trujillo  Pablo Chong  Ioannis Stergiopoulos  Viviane Cordovez  Mauricio Guzman  Pierre J G M De Wit  Harold J G Meijer  Gabriel Scalliet  Helge Sierotzki  Esther Lilia Peralta  Rafael E Arango Isaza  Gerrit H J Kema
Institution:1. Wageningen University and Research, Wageningen Plant Research, 6700 AA Wageningen, the Netherlands;2. Wageningen University and Research, Laboratory for Phytopathology, 6700 AA Wageningen, the Netherlands;3. Escuela Superior Politécnica del Litoral, ESPOL, Centro de Investigaciones Biotecnológicas del Ecuador, CIBE, Laboratorio de Fitopatología, ESPOL Polythecnic University, Guayaquil 09‐01‐5663, Ecuador;4. Department of Plant Pathology, University of California, Davis, Davis, CA 95616‐8751, USA;5. Department of Microbial Ecology, Netherlands Institute of Ecology, Wageningen 6708 PB, the Netherlands;6. Department of Phytopathology, National Banana Corporation of Costa Rica (CORBANA), La Rita de Pococí, Limón 6504‐1000, Costa Rica;7. Crop Protection Disease Control, Syngenta Crop Protection Münchwilen AG, Stein 4333, Switzerland;8. Plant Biotechnology Unit, Corporación para Investigaciones Biológicas (CIB), Medellín 050034, Colombia;9. School of Biosciences, Faculty of Sciences, National University of Colombia, Medellín 050034, Colombia
Abstract:The Dothideomycete Pseudocercospora fijiensis, previously Mycosphaerella fijiensis, is the causal agent of black Sigatoka, one of the most destructive diseases of bananas and plantains. Disease management depends on fungicide applications, with a major contribution from sterol demethylation‐inhibitors (DMIs). The continued use of DMIs places considerable selection pressure on natural P. fijiensis populations, enabling the selection of novel genotypes with reduced sensitivity. The hitherto explanatory mechanism for this reduced sensitivity was the presence of non‐synonymous point mutations in the target gene Pfcyp51, encoding the sterol 14α‐demethylase enzyme. Here, we demonstrate a second mechanism involved in DMI sensitivity of P. fijiensis. We identified a 19‐bp element in the wild‐type (wt) Pfcyp51 promoter that concatenates in strains with reduced DMI sensitivity. A polymerase chain reaction (PCR) assay identified up to six Pfcyp51 promoter repeats in four field populations of P. fijiensis in Costa Rica. We used transformation experiments to swap the wt promoter of a sensitive field isolate with a promoter from a strain with reduced DMI sensitivity that comprised multiple insertions. Comparative in vivo phenotyping showed a functional and proportional up‐regulation of Pfcyp51, which consequently decreased DMI sensitivity. Our data demonstrate that point mutations in the Pfcyp51 coding domain, as well as promoter inserts, contribute to the reduced DMI sensitivity of P. fijiensis. These results provide new insights into the importance of the appropriate use of DMIs and the need for the discovery of new molecules for black Sigatoka management.
Keywords:DMI  fungicide  Pfcyp51 promoter
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