The wild-type used in this study was the Arabidopsis thaliana (L.) Heynh. ecotype Columbia (Col-0). All Mediator mutants except med33b were previously described (Wang et al., 2015b). The med33b mutant (SALK_037472) and med15/nbr4-4 (SAIL_792_F02) were obtained from the Arabidopsis Biological Resource Center at The Ohio State University (Columbus, OH, USA). Homozygous mutant plants of SALK_037472 were confirmed with primers (forward: 5′GTACGAGGTTGCAACTACTG3′and reverse: 5′GCAGTGGAGAAAACAGCATG3′) that flank the T-DNA insertion and the left border primer LBa1 (Alonso et al., 2003). The med33a/b double mutant was created by crossing SALK_037472 with SALK_022477 (med33a) and identified in the F₂ generation by PCR. The Arabidopsis seeds were sown on autoclaved soil (Sunshine MVP; Sun Gro Horticulture, Agawam, MA, USA) and cold-treated at 4°C for 3 days. Plants were germinated and grown at 22–24°C under a 16-hr-light/8-hr-dark regime. Four-week-old soil-grown plants were used for pathogen infection.

Ten-day-old seedlings grown on one-half-strength Murashige and Skoog (½12 × MS) medium were treated with 0.5 mM SA, 0.1 mM MeJA, 0.1 mM ACC, or their combination. Seedlings for the negative control were treated with water. Aerial parts of the seedlings were collected and subjected to total RNA extraction.

The B. cinerea strain B05 was used in this study. B. cinerea inoculation and lesion size measurement were conducted as described in detail previously (Wang et al., 2015a).

Total RNA extraction, reverse transcription, and real-time quantitative PCR (qPCR) were performed as previously described (Defraia et al., 2010). Primers used for PR1, VSP1, and PDF1.2 were described previously (Defraia et al., 2010; Wang et al., 2015b). Primers used for HEL are forward: 5′GTGAGTGCTTATTGCTCCAC3′ and reverse: 5′ACATCCAAATCCAAGCCTCC3′, and for CHIB are forward: 5′GGTTCTGGATGACTGCTCAG3′ and reverse: 5′CTATACGATCGGCGACTCTC3′.

Statistical analyses were performed using the one-way ANOVA and the two-way ANOVA in Prism 5.0b (GraphPad Software, La Jolla, CA, USA). Lesion sizes measured in three independent experiments were combined and analyzed as a one-way ANOVA, blocked by experiment, using JMP 11 (JMP Software, Cary, NC, USA). All experiments were repeated three independent times with similar trends. Results from a representative experiment are presented.

To compare the function of different Arabidopsis Mediator subunits in the SA, JA, and ET signaling pathways, we tested SA-induced expression of the SA pathway marker gene PATHOEGNESIS-RELATED GENE1 (PR1), MeJA-induced expression of the wound-responsive marker gene VEGATATIVE STORAGE PROTEIN1 (VSP1) and the defense marker gene PLANT DEFENSIN1.2 (PDF1.2), and ACC-induced expression of PDF1.2 in the previously described 13 Mediator subunit mutants except that a med33a/b double mutant was used to replace the med33b single mutant (Wang et al., 2015b). Ten-day-old seedlings of the wild-type Col-0 and the 13 Mediator mutants grown on ½12 × MS medium were treated with SA, MeJA, or ACC. We also included the med15/nrb4-4 mutant in the experiment, as MED15 is essential for SA signaling (Canet et al., 2012). Since homozygous med15 plants are sterile, we used seeds from heterozygous plants. Three weeks after germination in soil, the small and chlorotic homozygous med15 plants were transplanted and allowed to grow for four more weeks. As med15 mutant plants grow very slowly compared with Col-0, 3-week-old soil-grown Col-0 plants with a size similar to that of the med15 plants were used for comparison. As shown Figure 1A, SA-induced PR1 expression was significantly blocked in med14, med15, and med16, MeJA-induced VSP1 expression was significantly reduced only in med25, MeJA-induced PDF1.2 expression was significantly decreased in med8, med14, med15, med16, med18, med20a, med25, med31, and med33a/b, and ACC-induced PDF1.2 expression was significantly inhibited in med8, med14, med15, med16, med25, and med33a/b. Note that the observation that MeJA-induced PDF1.2 expression was significantly decreased in med18 is in contrast to the previous report (Lai et al., 2014). This discrepancy is probably due to different growth conditions. Nevertheless, these results indicate that, among the 14 Mediator subunits, MED14, MED15, and MED16 are required for SA-activated PR1 expression, MED25 is required for MeJA-induced VSP1 expression, MED8, MED14, MED15, MED16, MED18, MED20a, MED25, MED31, and MED33A/B are required for MeJA-induced PDF1.2 expression, and MED8, MED14, MED15, MED16, MED25, and MED33A/B are required for ACC-induced PDF1.2 expression.

Since MED14, MED15, and MED16 function in the SA pathway (Canet et al., 2012; Wathugala et al., 2012; Zhang et al., 2012, 2013), they might also be involved in SA-mediated suppression of JA signaling. To test this hypothesis, we treated med14, med15, med16, and Col-0 plants with MeJA or MeJA plus SA and examined the induction of the MeJA-induced wound-responsive gene VSP1. As shown in Figure 1B, SA significantly inhibited MeJA-induced expression of VSP1 in the Col-0 plants, but the inhibition was significantly alleviated in med14 and med16, and completely blocked in med15, indicating that MED14, MED15, and MED16 are all required for SA-mediated suppression of JA-mediated wound-responsive gene expression. Moreover, MED14, MED15, and MED16 also function in the ET-mediated defense pathway. As MED16 is required for ET-activated suppression of JA-mediated wound signaling (Wang et al., 2015b), MED14 and MED15 might also be required for this process. To test this, we treated med14, med15, and Col-0 plants with MeJA or MeJA plus ACC and tested the induction of VSP1. As shown in Figure 1C, ACC significantly inhibited MeJA-induced expression of VSP1 in the Col-0 plants, but the inhibition was dramatically relieved in med14 and completely blocked in med15. Therefore, as MED16 (Wang et al., 2015b), MED14 and MED15 are also required for ET-mediated suppression of JA-induced wound-responsive gene expression. Finally, since MED25 functions in JA-mediated pathogen and wound responses (Kidd et al., 2009; Chen et al., 2012), it might modulate JA-mediated suppression of SA signaling. To test this hypothesis, we treated med25 and Col-0 plants with SA and SA plus MeJA and examined the induction of the SA-responsive genes PR1, PR2, and PR5. As shown in Figure 1D, MeJA inhibited SA-induced PR gene expression to similar extents in the Col-0 and med25 plants, indicating that MED25 is not involved in JA-mediated suppression of SA signaling.

PDF1.2 is a marker gene of the JA/ET-mediated defense signaling, which is central in resistance to necrotrophic pathogens. The Mediator subunits MED8, MED14, MED16, MED18, and MED25 are required for MeJA- and/or ACC-induced PDF1.2 expression and contribute to resistance to necrotrophic fungal pathogens (Kidd et al., 2009; Wathugala et al., 2012; Zhang et al., 2012; Lai et al., 2014; Wang et al., 2015b). Since MED20a, MED31, and MED33A/B are also required for full induction of PDF1.2 by MeJA and/or ACC, we examined B. cinerea-induced expression of three JA/ET-responsive genes PDF1.2, HEVEIN-LIKE (HEL), and BASIC CHITINASE (CHIB) in med20a, med31, and med33a/b and tested resistance of these mutants to B. cinerea. We did not include the med15 mutant in the experiment due to its extremely delayed growth. As shown in Figure 2A, B. cinerea-induced expression of PDF1.2, HEL, and CHIB was significantly reduced only in the med33a/b double mutant. Consistently, med33a/b also exhibited enhanced susceptible to B. cinerea (Figures 2B,C). These results indicate that MED33A/B plays a positive role in defense against this necrotrophic fungal pathogen.