A Role for the GCC-Box in Jasmonate-Mediated Activation of the <i>PDF1.2</i> Gene of Arabidopsis

Brown, Raymond Albert Joseph; Kazan, Kemal; McGrath, Ken; Maclean, D. J.; Manners, John M.

doi:10.1104/pp.102.017814

Cited by 393 publications

(283 citation statements)

References 65 publications

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“…In the case of AtERF2, its role as a positive regulator of MeJA response was confirmed, as had previously been suggested in plants overexpressing AtERF2 (Brown et al, 2003). Additionally, a reduction in disease symptoms relative to wild type after inoculation with F. oxysporum was observed, supporting a role for AtERF2 as a positive regulator of disease resistance.…”

Section: What Was Shownsupporting

confidence: 62%

Ethylene Response Factors in Jasmonate Signaling and Defense Response

Grennan

2008

Plant Physiology

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Section: What Was Shownsupporting

confidence: 62%

Ethylene Response Factors in Jasmonate Signaling and Defense Response

Grennan

2008

Plant Physiology

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“…The activation of defense responses by ethylene has previously been associated with the activity of transcription factors binding the GCC box in defense promoters, resulting in the induction of antimicrobial genes such as PDF1.2 and chitinases in Arabidopsis (Ohme-Takagi and Fujimoto et al, 2000;Brown et al, 2003). When transgenic hairy roots containing the 43GCC::luciferase construct were challenged with R. solani, an early induction of the reporter gene suggested that an ethylene-mediated response was induced at the initial stages of infection, while an additional induction peaking at 14 h suggested a secondary phase of activity of the GCC element.…”

Section: Discussionmentioning

confidence: 99%

The B-3 Ethylene Response Factor MtERF1-1 Mediates Resistance to a Subset of Root Pathogens inMedicago truncatulawithout Adversely Affecting Symbiosis with Rhizobia

et al. 2010

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The fungal necrotrophic pathogen Rhizoctonia solani is a significant constraint to a range of crops as diverse as cereals, canola, and legumes. Despite wide-ranging germplasm screens in many of these crops, no strong genetic resistance has been identified, suggesting that alternative strategies to improve resistance are required. In this study, we characterize moderate resistance to R. solani anastomosis group 8 identified in Medicago truncatula. The activity of the ethylene-and jasmonateresponsive GCC box promoter element was associated with moderate resistance, as was the induction of the B-3 subgroup of ethylene response transcription factors (ERFs). Genes of the B-1 subgroup showed no significant response to R. solani infection. Overexpression of a B-3 ERF, MtERF1-1, in Medicago roots increased resistance to R. solani as well as an oomycete root pathogen, Phytophthora medicaginis, but not root knot nematode. These results indicate that targeting specific regulators of ethylene defense may enhance resistance to an important subset of root pathogens. We also demonstrate that overexpression of MtERF1-1 enhances disease resistance without apparent impact on nodulation in the A17 background, while overexpression in sickle reduced the hypernodulation phenotype. This suggests that under normal regulation of nodulation, enhanced resistance to root diseases can be uncoupled from symbiotic plant-microbe interactions in the same tissue and that ethylene/ERF regulation of nodule number is distinct from the defenses regulated by B-3 ERFs. Furthermore, unlike the stunted phenotype previously described for Arabidopsis (Arabidopsis thaliana) ubiquitously overexpressing B-3 ERFs, overexpression of MtERF1-1 in M. truncatula roots did not show adverse effects on plant development.

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“…Two kilobases of sequence upstream of the predicted start codon of each of the VvHT1 to -5 and VvcwINV genes was obtained from the published grapevine PN40024 genome sequence (Jaillon et al, 2007) and analyzed for putative regulatory motifs associated with stress-induced transcription using the PLACE database (Higo et al, 1999). A number of motifs were identified: GCC box (Brown et al, 2003), MYC recognition (Abe et al, 1997), T/G box (Boter et al, 2004), wound response element (Palm et al, 1990), and abscisic acid response elements (ABREs; Choi et al, 2000;Hattori et al, 2002). Figure 3 also shows the presence of Suc-responsive motifs (SURE1, Suc box 3) shown previously by Cakir et al (2003) to be involved in the transcriptional regulation of VvHT1.…”

Section: Identification Of Aba Regulatory Motifs In the Vvht5 Promotermentioning

confidence: 99%

“…The presence of regulatory motifs associated with stress-induced transcription in a 2-kb promoter region from the published grapevine PN40024 genome sequence is shown. Recognition sequences are as follows: GCC box (GCCGCC; Brown et al, 2003), T/G box (AACGTG; Boter et al, 2004), MYC (CACATG; Abe et al, 1997), ABRE (ACGTGG/TC; Hattori et al, 2002), and wound response element (WRE; AAA/TGTATCC/GA; Palm et al, 1990). Also shown are the Suc-responsive motifs SURE (ATA-GAAA) and Suc box 3 (AAATCA----AA), identified by Cakir et al (2003) to be involved in the transcriptional regulation of VvHT1.…”

Section: Biotrophic Pathogen Infection and Wounding Induce The Aba Bimentioning

confidence: 99%

Involvement of Abscisic Acid in the Coordinated Regulation of a Stress-Inducible Hexose Transporter (VvHT5) and a Cell Wall Invertase in Grapevine in Response to Biotrophic Fungal Infection

2010

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Biotrophic fungal and oomycete pathogens alter carbohydrate metabolism in infected host tissues. Symptoms such as elevated soluble carbohydrate concentrations and increased invertase activity suggest that a pathogen-induced carbohydrate sink is established. To identify pathogen-induced regulators of carbohydrate sink strength, quantitative real-time polymerase chain reaction was used to measure transcript levels of invertase and hexose transporter genes in biotrophic pathogen-infected grapevine (Vitis vinifera) leaves. The hexose transporter VvHT5 was highly induced in coordination with the cell wall invertase gene VvcwINV by powdery and downy mildew infection. However, similar responses were also observed in response to wounding, suggesting that this is a generalized response to stress. Analysis of the VvHT5 promoter region indicated the presence of multiple abscisic acid (ABA) response elements, suggesting a role for ABA in the transition from source to sink under stress conditions. ABA treatment of grape leaves was found to reproduce the same gene-specific transcriptional changes as observed under biotic and abiotic stress conditions. Furthermore, the key regulatory ABA biosynthetic gene, VvNCED1, was activated under these same stress conditions. VvHT5 promoter::b-glucuronidase-directed expression in transgenic Arabidopsis (Arabidopsis thaliana) was activated by infection with powdery mildew and by ABA treatment, and the expression was closely associated with vascular tissue adjacent to infected regions. Unlike VvHT1 and VvHT3, which appear to be predominantly involved in hexose transport in developing leaves and berries, VvHT5 appears to have a specific role in enhancing sink strength under stress conditions, and this is controlled through ABA. Our data suggest a central role for ABA in the regulation of VvcwINV and VvHT5 expression during the transition from source to sink in response to infection by biotrophic pathogens.

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A Role for the GCC-Box in Jasmonate-Mediated Activation of the PDF1.2 Gene of Arabidopsis

Cited by 393 publications

References 65 publications

Ethylene Response Factors in Jasmonate Signaling and Defense Response

Ethylene Response Factors in Jasmonate Signaling and Defense Response

The B-3 Ethylene Response Factor MtERF1-1 Mediates Resistance to a Subset of Root Pathogens inMedicago truncatulawithout Adversely Affecting Symbiosis with Rhizobia

Involvement of Abscisic Acid in the Coordinated Regulation of a Stress-Inducible Hexose Transporter (VvHT5) and a Cell Wall Invertase in Grapevine in Response to Biotrophic Fungal Infection

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