Arabidopsis Mitogen-Activated Protein Kinase Kinases MKK1 and MKK2 Have Overlapping Functions in Defense Signaling Mediated by MEKK1, MPK4, and MKS1

Hormone levels and growth phenotypes of mkk1/2/sid2 and mkk1/2/ein2 triple mutants. A and B, Free SA (A) and ET (B) levels. Error bars represent se of the mean. C and D, Phenotypes of mkk1/2/sid2 (C) and mkk1/2/ein2 triple mutants (D). E, Venn diagram showing overlapping gene expression signatures between BTH- or ACC-treated wild-type plants and the mkk1/2 double mutant. Overlap is between the top 500 most significantly differentially expressed genes as measured by the ATH1 Affymetrix GeneChip.

Defense gene expression in the mutants. PR1 (A) and PDF1.2 (B) mRNA levels were monitored by real-time RT-PCR after treatment of the mutants with BTH or JA, respectively. Means ± sd are shown.

Disease resistance in mutants. A, Response to infection by P. syringae of wild-type Col-0, mkk1, mkk2, and mkk1/2 compared to nahG transgenic. B, Response to P. syringae of mkk1/2 compared to mkk1/2/ein2 and mkk1/2/sid2 triple mutants, atgsnor1-3, and mpk4. C and D, Growth of H. parasitica detected by trypan blue staining (C) and corresponding conidial counts/milligram tissue (D). E, Growth of B. cinerea in mutants assayed as the number of outgrowing lesions developed 3 d after inoculation. Experiments were repeated three times with similar results and error bars represent se.

MKK1 and MKK2 function upstream of MPK4. A and B, MPK4 kinase activity in single and double mutants. MPK4 protein was immunoprecipitated out of total protein extracts from plants treated for 30 min with 10 μm flg22 (A) or 100 μm BTH (B) and used in an in vitro kinase assay with myelin basic protein as substrate. Duplicate gels were subjected to western blotting to monitor MPK4 protein levels. C, Phenotype of mkk1/2/mks1 triple mutant in comparison to mkk1/2 and wild type.