Autor: |
Escobar-Niño A; Microbiology Laboratory, Institute for Viticulture and Agri-Food Research (IVAGRO), Faculty of Environmental and Marine Sciences, Department of Biomedicine, Biotechnology and Public Health, University of Cádiz, 11510 Puerto Real, Spain., Harzen A; Protein Mass Spectrometry, Max Planck Institute for Plant Breeding Research, 50829 Cologne, Germany., Stolze SC; Protein Mass Spectrometry, Max Planck Institute for Plant Breeding Research, 50829 Cologne, Germany., Nakagami H; Protein Mass Spectrometry, Max Planck Institute for Plant Breeding Research, 50829 Cologne, Germany.; Basic Immune System of Plants, Max Planck Institute for Plant Breeding Research, 50829 Cologne, Germany., Fernández-Acero FJ; Microbiology Laboratory, Institute for Viticulture and Agri-Food Research (IVAGRO), Faculty of Environmental and Marine Sciences, Department of Biomedicine, Biotechnology and Public Health, University of Cádiz, 11510 Puerto Real, Spain. |
Abstrakt: |
Extracellular vesicles (EVs) are membranous particles released by different organisms. EVs carry several sets of macromolecules implicated in cell communication. EVs have become a relevant topic in the study of pathogenic fungi due to their relationship with fungal-host interactions. One of the essential research areas in this field is the characterization protein profile of EVs since plant fungal pathogens rely heavily on secreted proteins to invade their hosts. However, EVs of Botrytis cinerea are little known, which is one of the most devastating phytopathogenic fungi. The present study has two main objectives: the characterization of B. cinerea EVs proteome changes under two pathogenic conditions and the description of their potential role during the infective process. All the experimental procedure was conducted in B. cinerea growing in a minimal salt medium supplemented with glucose as a constitutive stage and deproteinized tomato cell walls (TCW) as a virulence inductor. The isolation of EVs was performed by differential centrifugation, filtration, ultrafiltration, and sucrose cushion ultracentrifugation. EVs fractions were visualised by TEM using negative staining. Proteomic analysis of EVs cargo was addressed by LC-MS/MS. The methodology used allowed the correct isolation of B. cinerea EVs and the identification of a high number of EV proteins, including potential EV markers. The isolated EVs displayed differences in morphology under both assayed conditions. GO analysis of EV proteins showed enrichment in cell wall metabolism and proteolysis under TCW. KEGG analysis also showed the difference in EVs function under both conditions, highlighting the presence of potential virulence/pathogenic factors implicated in cell wall metabolism, among others. This work describes the first evidence of EVs protein cargo adaptation in B. cinerea , which seems to play an essential role in its infection process, sharing crucial functions with the conventional secretion pathways. |