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Race nonspecific resistance of barley against the barley powdery mildew fungus (Blumeria Graminis f.sp. Hordei, Speer, Bgh ) is mediated by recessive mlo alleles and is controlled by at least two additional genes ‘required for ml o‐specified disease resistance’ (Ror1 and Ror2 ). The pathogenesis‐related accumulation of hydrogen peroxide (H2O2) was comparatively analysed in a susceptible barley line (Hordeum vulgare L. Cv Ingrid, genotype Mlo Ror1, Ror2 ), a resistant Ingrid backcross line carrying the mutant allele mlo5 (BCIngrid‐mlo5, genotype mlo5 Ror1 Ror2 ), and in the moderately susceptible mutants A44 and A89 (genotypes mlo5 Ror1 ror2 and mlo5 ror1‐2 Ror2, respectively). In situ localization of H2O2 was performed by microscopic detection of 3,3‐diaminobenzidine (DAB) polymerization. In BCIngrid‐mlo5 , penetration resistance against Bgh attack was closely correlated to H2O2 accumulation in cytoplasmic aggregates and cell wall appositions beneath the appressorium. In contrast, H2O2 accumulation was almost completely absent in susceptible Ingrid. Lines with mutations in Ror genes showed less H2O2 accumulation beneath appressoria, but more interaction sites with whole cell H2O2 accumulation and hypersensitive cell death response than resistant BCIngrid‐mlo5 . Thus, mutations in Ror1 or Ror2 genes influence the cellular pattern of H2O2 accumulation in mlo plants attacked by Bgh . The data support the hypothesis that H2O2 accumulation is involved in resistance to fungal penetration.
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The pathogenesis-related accumulation of superoxide radical anions (O·− 2) and hydrogen peroxide (H2O2) was comparatively analyzed in a barley line (Hordeum vulgare L. cv Sultan-5) carrying the powdery mildew (Blumeria graminis f.sp. hordei, Speer, Bgh) resistance gene Mla12, and in susceptible mutants defective in Mla12 or in genes “required for Mla12-specified disease resistance” (Rar1 and Rar2). In-situ localization of reactive oxygen intermediates was performed both by microscopic detection of azide-insensitive nitroblue tetrazolium (NBT) reduction or diaminobenzidine (DAB) polymerization, and by an NBT-DAB double-staining procedure. The Mla12-mediated hypersensitive cell death occurred either in attacked epidermal cells or adjacent mesophyll cells of wild-type plants. Whole-cell H2O2 accumulation was detected in dying cells, while O·− 2 emerged in adjacent cells. Importantly, all susceptible mutants lacked these reactions. An oxalate oxidase, which is known to generate H2O2 and has been implicated in barley resistance against the powdery mildew fungus, was not differentially expressed between the wild type and all mutants. The results demonstrate that the Rar1 and Rar2 gene products, which are control elements of R-gene-mediated programmed cell death, also control accumulation of reactive oxygen intermediates but not the pathogenesis-related expression of oxalate oxidase.