4.7 Article

Identification by Tn-seq of Dickeya dadantii genes required for survival in chicory plants

期刊

MOLECULAR PLANT PATHOLOGY
卷 20, 期 2, 页码 287-306

出版社

WILEY
DOI: 10.1111/mpp.12754

关键词

Dickeya dadantii; glycosylation; metabolism; motility; phytopathogen; soft-rot disease; Tn-seq

资金

  1. Centre National de la Recherche Scientifique (CNRS)
  2. Institut National des Sciences Appliquees (INSA)
  3. University Lyon I
  4. Ministere de l'Enseignement Superieur, de la Recherche et de l'Innovation

向作者/读者索取更多资源

The identification of the virulence factors of plant-pathogenic bacteria has relied on the testing of individual mutants on plants, a time-consuming process. Transposon sequencing (Tn-seq) is a very powerful method for the identification of the genes required for bacterial growth in their host. We used this method in a soft-rot pathogenic bacterium to identify the genes required for the multiplication of Dickeya dadantii in chicory. About 100 genes were identified showing decreased or increased fitness in the plant. Most had no previously attributed role in plant-bacterium interactions. Following our screening, inplanta competition assays confirmed that the uridine monophosphate biosynthesis pathway and the purine biosynthesis pathway were essential to the survival of D. dadantii in the plant, as the mutants Delta carA, Delta purF, Delta purL, Delta guaB and Delta pyrE were unable to survive in the plant in contrast with the wild-type (WT) bacterium. This study also demonstrated that the biosynthetic pathways of leucine, cysteine and lysine were essential for bacterial survival in the plant and that RsmC and GcpA were important in the regulation of the infection process, as the mutants Delta rsmC and Delta gcpA were hypervirulent. Finally, our study showed that D.dadantii flagellin was glycosylated and that this modification conferred fitness to the bacterium during plant infection. Assay by this method of the large collections of environmental pathogenic strains now available will allow an easy and rapid identification of new virulence factors.

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