Abstract
BackgroundNuclear endosperm development is a common mechanism among Angiosperms, including Arabidopsis. During nuclear development, the endosperm nuclei divide rapidly after fertilization without cytokinesis to enter the syncytial phase, which is then followed by the cellularized phase. The endosperm can be divided into three spatial domains with distinct functions: the micropylar, peripheral, and chalazal domains. Previously, we identified two putative small invertase inhibitors, InvINH1 and InvINH2, that are specifically expressed in the micropylar region of the syncytial endosperm. In addition, ectopically expressing InvINH1 in the cellularized endosperm led to a reduction in embryo growth rate. However, it is not clear what are the upstream regulators responsible for the specific expression of InvINHs in the syncytial endosperm.ResultsUsing protoplast transient expression system, we discovered that a group of type I MADS box transcription factors can form dimers to activate InvINH1 promoter. Promoter deletion assays carried out in the protoplast system revealed the presence of an enhancer region in InvINH1 promoter, which contains several consensus cis-elements for the MADS box proteins. Using promoter deletion assay in planta, we further demonstrated that this enhancer region is required for InvINH1 expression in the syncytial endosperm. One of the MADS box genes, AGL62, is a key transcription factor required for syncytial endosperm development. Using promoter-GFP reporter assay, we demonstrated that InvINH1 and InvINH2 are not expressed in agl62 mutant seeds. Collectively, our data supports the role of AGL62 and other type I MADS box genes as the upstream activators of InvINHs expression in the syncytial endosperm.ConclusionsOur findings revealed several type I MADS box genes that are responsible for activating InvINH1 in the syncytial endosperm, which in turn regulates embryo growth rate during early stage of seed development.
Highlights
Nuclear endosperm development is a common mechanism among Angiosperms, including Arabi‐ dopsis
Our data indicated that AGL62 and AGL37 form a dimer in the protoplast that directly activates the invertase inhibitor 1 (InvINH1) promoter
Since InvINH1 expression is higher in the micropylar region and absent in the chalazal region of the syncytial endosperm [33], we investigated whether this spatial specificity is due to the selective activation of InvINH1 by C2 AGLs that are preferentially expressed in the micropylar endosperm
Summary
Nuclear endosperm development is a common mechanism among Angiosperms, including Arabi‐ dopsis. Ectopically expressing InvINH1 in the cellularized endosperm led to a reduction in embryo growth rate. It is not clear what are the upstream regulators responsible for the specific expression of InvINHs in the syncytial endosperm. The syncytial program is negatively regulated by a chromatin repressive complex, the FIS-PRC2 (Polycomb Repressive Complex 2) complex. In fis mutants such as mea, fis, fie, and msi, the endosperm fails to cellularize, which in turn leads to embryo abortion [8,9,10,11]. The transition from syncytial to cellularized endosperm is likely achieved through the FIS-PRC2-mediated suppression of AGL62
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