Genetic Dissection of Salicylic Acid-Mediated Defense Signaling Networks in Arabidopsis

dc.contributor.authorNg, Gina
dc.contributor.authorSeabolt, Savanna
dc.contributor.authorZhang, Chong
dc.contributor.authorSalimian, Sasan
dc.contributor.authorWatkins, Timley A.
dc.contributor.authorLu, Hua
dc.date.accessioned2023-07-19T20:38:06Z
dc.date.available2023-07-19T20:38:06Z
dc.date.issued2011-11-01
dc.description.abstractProperly coordinated defense signaling networks are critical for the fitness of plants. One hub of the defense networks is centered on salicylic acid (SA), which plays a key role in activating disease resistance in plants. However, while a number of genes are known to affect SA-mediated defense, relatively little is known about how these gene interact genetically with each other. Here we exploited the unique defense-sensitized Arabidopsis mutant accelerated cell death (acd) 6-1 to dissect functional relationships among key components in the SA hub. We show that while enhanced disease susceptibility (eds) 1-2 and phytoalexin deficient (pad) 4-1 suppressed acd6-1–conferred small size, cell death, and defense phenotypes, a combination of these two mutations did not incur additive suppression. This suggests that EDS1 and PAD4 act in the same signaling pathway. To further evaluate genetic interactions among SA regulators, we constructed 10 pairwise crosses in the acd6-1 background among mutants defective in: SA INDUCTION-DEFICIENT 2 for SA biosynthesis; AGD2-LIKE DEFENSE 1, EDS5, and PAD4 for SA accumulation; and NONEXPRESSOR OF PR GENES 1 for SA signaling. Systematic analysis of the triple mutants based on their suppression of acd6-1–conferred phenotypes revealed complex and interactive genetic relationships among the tested SA genes. Our results suggest a more comprehensive view of the gene networks governing SA function and provide a framework for further interrogation of the important roles of SA and possibly other signaling molecules in regulating plant disease resistance.en
dc.description.sponsorshipWe thank members in the Lu laboratory for assistance in this work and Stephen Miller at University of Maryland Baltimore County for critical comments on the manuscript. We thank William LaCourse for sharing the usage of his HPLC instrument, Charles Bieberich for sharing the use of his dissecting microscope, and Tim Ford for taking pictures for this publication. This work was supported by startup funds from University of Maryland Baltimore County and a grant from the National Science Foundation (RIG-0818651) to H.L. and a scholarship from the China Scholarship Council to C.Z.en
dc.description.urihttps://www.ncbi.nlm.nih.gov/pmc/articles/PMC3213356/en
dc.format.extent12 pagesen
dc.genrejournal articlesen
dc.identifierdoi:10.13016/m2gq8n-kv7n
dc.identifier.citationGina Ng and others, Genetic Dissection of Salicylic Acid-Mediated Defense Signaling Networks in Arabidopsis, Genetics, Volume 189, Issue 3, 1 November 2011, Pages 851–859, https://doi.org/10.1534/genetics.111.132332en
dc.identifier.urihttps://doi.org/10.1534/genetics.111.132332
dc.identifier.urihttp://hdl.handle.net/11603/28785
dc.language.isoenen
dc.publisherOxford University Pressen
dc.relation.isAvailableAtThe University of Maryland, Baltimore County (UMBC)
dc.relation.ispartofUMBC Biological Sciences Department Collection
dc.relation.ispartofUMBC Faculty Collection
dc.relation.ispartofUMBC Student Collection
dc.rightsThis item is likely protected under Title 17 of the U.S. Copyright Law. Unless on a Creative Commons license, for uses protected by Copyright Law, contact the copyright holder or the author.en
dc.subjectsalicylic acid (SA)en
dc.subjectaccelerated cell death (acd)en
dc.subjectenhanced disease susceptibility (eds) 1-2en
dc.subjectphytoalexin deficient (pad) 4-1en
dc.subjectSA INDUCTION-DEFICIENT 2en
dc.subjectAGD2-LIKE DEFENSE 1, EDS5, and PAD4en
dc.subjectNONEXPRESSOR OF PR GENES 1en
dc.titleGenetic Dissection of Salicylic Acid-Mediated Defense Signaling Networks in Arabidopsisen
dc.typeTexten
dcterms.creatorhttps://orcid.org/0000-0002-7496-3200en

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