Sir2‐mediated cytoplasmic deacetylation facilitates pathogenic fungi infection in host plants

乙酰化 生物 灰葡萄孢菌 生物发生 细胞质 丝氨酸 毒力 细胞生物学 核糖体生物发生 遗传学 核糖体 磷酸化 基因 植物 核糖核酸
作者
Ning Zhang,Jicheng Hu,Zhishan Liu,Wenxing Liang,Limin Song
出处
期刊:New Phytologist [Wiley]
卷期号:241 (4): 1732-1746 被引量:3
标识
DOI:10.1111/nph.19438
摘要

Summary Lysine acetylation is an evolutionarily conserved and widespread post‐translational modification implicated in the regulation of multiple metabolic processes, but its function remains largely unknown in plant pathogenic fungi. A comprehensive analysis combined with proteomic, molecular and cellular approaches was presented to explore the roles of cytoplasmic acetylation in Fusarium oxsysporum f.sp. lycopersici ( Fol ). The divergent cytoplasmic deacetylase FolSir2 was biochemically characterized, which is contributing to fungal virulence. Based on this, a total of 1752 acetylated sites in 897 proteins were identified in Fol via LC–MS/MS analysis. Further analyses of the quantitative acetylome revealed that 115 proteins representing two major pathways, translational and ribosome biogenesis, were hyperacetylated in the ∆Folsir2 strain. We experimentally examined the regulatory roles of FolSir2 on K271 deacetylation of FolGsk3, a serine/tyrosine kinase implicated in a variety of cellular functions, which was found to be crucial for the activation of FolGsk3 and thus modulated Fol pathogenicity. Cytoplasmic deacetylation by FolSir2 homologues has a similar function in Botrytis cinerea and likely other fungal pathogens. These findings reveal a conserved mechanism of silent information regulator 2‐mediated cytoplasmic deacetylation that is involved in plant‐fungal pathogenicity, providing a candidate target for designing broad‐spectrum fungicides to control plant diseases.
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