María Amalia Chiesa

Characterization of a variant of Xanthomonas citri subsp. citri that triggers a host-specific defense response.

Citrus is an economically important fruit crop that is severely afflicted by Asiatic citrus bacterial canker (CBC), a disease caused by the phytopathogen Xanthomonas citri subsp. citri (X. citri). To gain insight into the molecular epidemiology of CBC, 42 Xanthomonas isolates were collected from a range of Citrus spp. across 17 different orchards in Tucumán, Argentina and subjected to molecular, biochemical, and pathogenicity tests. Analysis of genome-specific X. citri markers and DNA polymorphisms based on repetitive elements-based polymerase chain reaction showed that all 42 isolates belonged to X. citri. Interestingly, pathogenicity tests showed that one isolate, which shares >90% genetic similarity to the reference strain X. citri T, has host range specificity. This new variant of X. citri subsp. citri, named X. citri A(T), which is deficient in xanthan production, induces an atypical, noncankerous chlorotic phenotype in Citrus limon and C. paradisi and weak cankerous lesions in C. aurantifolia and C. clementina leaves. In C. limon, suppression of canker development is concomitant with an oxidative burst; xanthan is not implicated in the phenotype induced by this interaction, suggesting that other bacterial factors would be involved in triggering the defense response.

Resistance to citrus canker induced by a variant of Xanthomonas citri ssp. citri is associated with a hypersensitive cell death response involving autophagy-associated vacuolar processes.

Xanthomonas citri ssp. citri (X. citri) is the causal agent of Asiatic citrus canker, a disease that seriously affects most commercially important Citrus species worldwide. We have identified previously a natural variant, X. citri AT , that triggers a host-specific defence response in Citrus limon. However, the mechanisms involved in this canker disease resistance are unknown. In this work, the defence response induced by X. citri AT was assessed by transcriptomic, physiological and ultrastructural analyses, and the effects on bacterial biofilm formation were monitored in parallel. We show that X. citri AT triggers a hypersensitive response associated with the interference of biofilm development and arrest of bacterial growth in C. limon. This plant response involves an extensive transcriptional reprogramming, setting in motion cell wall reinforcement, the oxidative burst and the accumulation of salicylic acid (SA) and phenolic compounds. Ultrastructural analyses revealed subcellular changes involving the activation of autophagy-associated vacuolar processes. Our findings show the activation of SA-dependent defence in response to X. citri AT and suggest a coordinated regulation between the SA and flavonoid pathways, which is associated with autophagy mechanisms that control pathogen invasion in C. limon. Furthermore, this defence response protects C. limon plants from disease on subsequent challenges by pathogenic X. citri. This knowledge will allow the rational exploitation of the plant immune system as a biotechnological approach for the management of the disease.

Differential expression of distinct soybean resistance genes interacting with Argentinean isolates of Diaporthe phaseolorum var. meridionalis

Soybean Stem Canker (SSC), caused by Diaporthe phaseolorum var. meridionalis (Dpm), is an important disease of soybean in Argentina. There are five known dominant genes that confer resistance to SSC, Rdm1 to Rdm5. Particularly, Rdm2 was identified in cv. Tracy-M and then it was stabilized in the breeding line T2. The Rdm4 gene was first identified in cv. Hutcheson. More recently it was found that this gene was linked to the Rdm5 gene, defining the Rdm4-5 resistance region in Hutcheson. The objective of this work was to analyze the behaviour of the dominant Rdm2, Rdm4 and Rdm5 genes interacting with the CE109 and CE112 local physiological races of Dpm, in different susceptible backgrounds (genotypes RA702 and J77-339). Rdm4 and Rdm5 segregated phenotypically as completely dominant genes in the specific interactions with the CE109 and CE112 isolates, respectively, in both susceptible backgrounds. Similarly, Rdm2 segregated as expected for a complete dominant gene in the specific interaction with the CE109 isolate, in both susceptible backgrounds. However, when interacting with the CE112 isolate, the Rdm2 gene did not segregate as expected for a completely dominant gene, neither in RA702 nor in J77-339 susceptible background. The distorted segregation of the Rdm2 gene was due to incomplete penetrance. To the best of our knowledge this is the first report documenting changes in the degree of penetrance of a soybean resistance gene (Rdm2) depending upon the physiological race of Dpm which interacts with and the genetic background in which the Rdm gene is being expressed.

Molecular mapping of the genomic region conferring resistance to soybean stem canker in Hutcheson soybean

Genetic resistance to soybean stem canker, caused by the fungus Diaporthe phaseolorum var. meridionalis (Dpm), is controlled by five major, dominant, nonallelic genes Rdm1 to Rdm5. A genomic region containing the Rdm4 and Rdm5 genes was first described in Hutcheson soybean, where they were found to confer specific resistance to Argentinean physiological races of Dpm. Here, we report the genetic mapping of Rdm4 and Rdm5 loci using two pheno- and genotypically characterized F2:3 populations derived from Hutcheson cultivar. The mapping populations were screened with amplified fragment length polymorphism (AFLP) markers using bulk segregant analysis, and with simple sequence repeat (SSR) markers. Linkage analysis indicated that the Rdm4 and Rdm5 resistance loci were located in a genomic region collinear with the molecular linkage group (MLG) A2 (chromosome 8) of the soybean genetic map. The linkage group contains two SSR markers, Sat_162 and Satt233, flanking the Rdm4 and Rdm5 loci. These SSR will be useful to increase the efficiency of selection in breeding programs aimed to incorporate Rdm4 and Rdm5 genes into soybean elite germplasm.