Fine mapping links the FTa1 flowering time regulator to the dominant spring1 locus in Medicago

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dc.contributor.author Yeoh, CC en
dc.contributor.author Balcerowicz, M en
dc.contributor.author Zhang, Lulu en
dc.contributor.author Vista, Mauren en
dc.contributor.author Brocard, L en
dc.contributor.author Ratet, P en
dc.contributor.author Putterill, Joanna en
dc.coverage.spatial United States en
dc.date.accessioned 2016-08-14T23:45:47Z en
dc.date.issued 2013 en
dc.identifier.citation PLoS One 8(1):Article number e53467 2013 en
dc.identifier.uri http://hdl.handle.net/2292/29987 en
dc.description.abstract To extend our understanding of flowering time control in eudicots, we screened for mutants in the model legume Medicago truncatula (Medicago). We identified an early flowering mutant, spring1, in a T-DNA mutant screen, but spring1 was not tagged and was deemed a somaclonal mutant. We backcrossed the mutant to wild type R108. The F1 plants and the majority of F2 plants were early flowering like spring1, strongly indicating that spring1 conferred monogenic, dominant early flowering. We hypothesized that the spring1 phenotype resulted from over expression of an activator of flowering. Previously, a major QTL for flowering time in different Medicago accessions was located to an interval on chromosome 7 with six candidate flowering-time activators, including a CONSTANS gene, MtCO, and three FLOWERING LOCUS T (FT) genes. Hence we embarked upon linkage mapping using 29 markers from the MtCO/FT region on chromosome 7 on two populations developed by crossing spring1 with Jester. Spring1 mapped to an interval of ∼0.5 Mb on chromosome 7 that excluded MtCO, but contained 78 genes, including the three FT genes. Of these FT genes, only FTa1 was up-regulated in spring1 plants. We then investigated global gene expression in spring1 and R108 by microarray analysis. Overall, they had highly similar gene expression and apart from FTa1, no genes in the mapping interval were differentially expressed. Two MADS transcription factor genes, FRUITFULLb (FULb) and SUPPRESSOR OF OVER EXPRESSION OF CONSTANS1a (SOC1a), that were up-regulated in spring1, were also up-regulated in transgenic Medicago over-expressing FTa1. This suggested that their differential expression in spring1 resulted from the increased abundance of FTa1. A 6255 bp genomic FTa1 fragment, including the complete 5' region, was sequenced, but no changes were observed indicating that the spring1 mutation is not a DNA sequence difference in the FTa1 promoter or introns. en
dc.language eng en
dc.relation.ispartofseries PLoS One en
dc.rights Items in ResearchSpace are protected by copyright, with all rights reserved, unless otherwise indicated. Previously published items are made available in accordance with the copyright policy of the publisher. Details obtained from http://www.sherpa.ac.uk/romeo/issn/1932-6203/ en
dc.rights.uri https://researchspace.auckland.ac.nz/docs/uoa-docs/rights.htm en
dc.rights.uri https://creativecommons.org/licenses/by/4.0/ en
dc.subject Arabidopsis en
dc.subject Chromosome Mapping en
dc.subject Chromosomes, Plant en
dc.subject DNA, Bacterial en
dc.subject Flowers en
dc.subject Gene Expression Regulation, Plant en
dc.subject Medicago truncatula en
dc.subject Microarray Analysis en
dc.subject Mutation en
dc.subject Phenotype en
dc.subject Plant Proteins en
dc.subject Promoter Regions, Genetic en
dc.subject Quantitative Trait Loci en
dc.subject Time Factors en
dc.subject Transcription Factors en
dc.title Fine mapping links the FTa1 flowering time regulator to the dominant spring1 locus in Medicago en
dc.type Journal Article en
dc.identifier.doi 10.1371/journal.pone.0053467 en
pubs.issue 1 en
pubs.volume 8 en
dc.description.version VoR - Version of Record en
dc.identifier.pmid 23308229 en
pubs.publication-status Published en
dc.rights.accessrights http://purl.org/eprint/accessRights/OpenAccess en
pubs.subtype Article en
pubs.elements-id 371877 en
pubs.org-id Science en
pubs.org-id Biological Sciences en
dc.identifier.eissn 1932-6203 en
dc.identifier.pii PONE-D-12-23895 en
pubs.number e53467 en
pubs.record-created-at-source-date 2016-08-15 en
pubs.dimensions-id 23308229 en


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