MODD Mediates Deactivation and Degradation of OsbZIP46 to Negatively Regulate ABA Signaling and Drought Resistance in Rice

Ma, Siqi; Zong, Wei; Lv, Yan; Chun, Yung; Guo, Zilong; Li, Jie; Li, Xu; Xiang, Yong Bing; Song, Huazhi; Xiao, Jin-Long; Li, Xianghua; Xiong, Lizhong

doi:10.1105/tpc.16.00171

Cited by 132 publications

(93 citation statements)

References 80 publications

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“…The transcriptional activity of OsbZIP46 is suppressed by OsMODD by recruiting HADC to OsbZIP46 chromatin to reduce its acetylation level. The protein stability of OsbZIP46 is also regulated by OsMODD through recruitment of the U-box-type ubiquitin E3 ligase OsPUB7 (Tang et al, 2016). Consistent with this finding, we detected a lower CO protein level in the CO-HA/AFP2-ox line than in the CO-HA line during the night (Fig.…”

Section: Afp2 Delays Flowering Time Via Cosupporting

confidence: 88%

ABI5-BINDING PROTEIN2 Coordinates CONSTANS to Delay Flowering by Recruiting the Transcriptional Corepressor TPR2

et al. 2018

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ORCID ID: 0000-0002-8009-4419 (X.H.).ABI5-BINDING PROTEIN2 (AFP2) negatively regulates the abscisic acid signal by accelerating ABI5 degradation during seed germination in Arabidopsis (Arabidopsis thaliana). The abscisic acid signal is reported to delay flowering by up-regulating Flowering Locus C expression, but the role of AFP2 in regulating flowering time is unknown. Here, we found that flowering time was markedly delayed and CONSTANS (CO) expression was reduced in a transgenic Arabidopsis line overexpressing AFP2 under LD conditions. Conversely, the loss-of-function afp2 mutant showed slightly earlier flowering, with higher CO expression. These data suggest that AFP2 negatively regulates photoperiod-dependent flowering time by modulating the CO signal. We then found that AFP2 exhibited circadian expression rhythms that peaked during the night. Furthermore, the C-terminus of AFP2 interacted with CO, while its N-terminal ethylene response factor-associated amphiphilic repression motif interacted with the transcriptional corepressor TOPLESS-related protein2 (TPR2). Thus, AFP2 bridges CO and TPR2 to form the CO-AFP2-TPR2 complex. Biochemical and genetic analyses showed that AFP2 mediated CO degradation during the night. AFP2 also recruited histone deacetylase activity at Flowering Locus T chromatin through its interaction with TPR2. Taken together, our results reveal an elaborate mechanism by which AFP2 modulates flowering time through coordinating the activity and stability of CO.

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Section: Afp2 Delays Flowering Time Via Cosupporting

confidence: 88%

ABI5-BINDING PROTEIN2 Coordinates CONSTANS to Delay Flowering by Recruiting the Transcriptional Corepressor TPR2

et al. 2018

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“…Alternatively (or in parallel), it could fine-tune the production of Hd3a and RFT1 during photoperiodic induction (Gómez-Ariza et al, 2015;Ogiso-Tanaka et al, 2013). More data will be required to distinguish between these possibilities and validate them, but it is clear that reproductive commitment requires a tight balance between flowering promoting and repressive complexes, whose equilibrium could be controlled by modulating the expression levels of distinct bZIPs by developmental or environmental factors (Tang et al, 2016;Wu et al, 2014;Zhang et al, 2016) or by controlling their activity through phosphorylation (Kagaya et al, 2002;Choi et al, 2005;Furihata et al, 2006). Indeed, phosphorylation of OsFD transcription factors is required for binding to 14-3-3 proteins and is limiting to FAC function (Taoka et al, 2011).…”

Section: The Rice Florigens Act In Leaves To Regulate Their Own Exprementioning

confidence: 99%

Antagonistic Transcription Factor Complexes Modulate the Floral Transition in Rice

et al. 2017

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Plants measure day or night lengths to coordinate specific developmental changes with a favorable season. In rice (Oryza sativa), the reproductive phase is initiated by exposure to short days when expression of HEADING DATE 3a (Hd3a) and RICE FLOWERING LOCUS T 1 (RFT1) is induced in leaves. The cognate proteins are components of the florigenic signal and move systemically through the phloem to reach the shoot apical meristem (SAM). In the SAM, they form a transcriptional activation complex with the bZIP transcription factor OsFD1 to start panicle development. Here, we show that Hd3a and RFT1 can form transcriptional activation or repression complexes also in leaves and feed back to regulate their own transcription. Activation complexes depend on OsFD1 to promote flowering. However, additional bZIPs, including Hd3a BINDING REPRESSOR FACTOR1 (HBF1) and HBF2, form repressor complexes that reduce Hd3a and RFT1 expression to delay flowering. We propose that Hd3a and RFT1 are also active locally in leaves to fine-tune photoperiodic flowering responses.

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Section: Methodsmentioning

confidence: 99%

“…For subcellular localization, the full‐length coding sequence of BnaA9.WRKY47 amplified from ‘Westar 10’ was cloned into the pM999‐33 vector driven by the CaMV35S promoter (Tang et al , ) using the In‐Fusion HD Cloning kit (Takara Bio). The fused construct 35S:BnaA9.WRKY47:GFP was cotransformed with 35S:Ghd7:CFP , a nuclear marker (Tang et al , ), into Arabidopsis protoplasts. After transformation for 12 to 16 h, a confocal laser‐scanning microscope (Leica SP8) was used for capturing the fluorescence signal with the setting of excitation/detection wavelengths: GFP (488 nm/505–540 nm) and CFP (448 nm/460‐490 nm).…”

Section: Methodsmentioning

confidence: 99%

Transcription factor BnaA9.WRKY47 contributes to the adaptation of Brassica napus to low boron stress by up‐regulating the boric acid channel gene BnaA3.NIP5;1

Feng

Cui

Wang

et al. 2019

Plant Biotechnology Journal

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Summary Boron (B) deficiency is one of the major causes of growth inhibition and yield reduction in Brassica napus (B. napus). However, the molecular mechanisms of low B adaptation in B. napus are largely unknown. Here, fifty‐one BnaWRKY transcription factors were identified as responsive to B deficiency in B. napus, in which BnaAn.WRKY26, BnaA9.WRKY47, BnaA1.WKRY53 and BnaCn.WRKY57 were tested in yeast one‐hybrid assays and showed strong binding activity with conserved sequences containing a W box in the promoters of the B transport‐related genes BnaNIP5;1s and BnaBOR1s. Green fluorescent protein fused to the target protein demonstrated the nuclear localization of BnaA9.WRKY47. CRISPR/Cas9‐mediated knockout lines of BnaA9.WRKY47 in B. napus had increased sensitivity to low B and lower contents of B than wild‐type plants. In contrast, overexpression of BnaA9.WRKY47 enhanced the adaptation to low B with higher B contents in tissues than in wild‐type plants. Consistent with the phenotypic response and B accumulation in these transgenic lines, the transcription activity of BnaA3.NIP5;1, a B efficiency candidate gene, was decreased in the knockout lines but was significantly increased in the overexpressing lines under low B conditions. Electrophoretic mobility shift assays, transient expression experiments in tobacco and in situ hybridizations showed that BnaA9.WRKY47 directly activated BnaA3.NIP5;1 expression through binding to the specific cis‐element. Taken together, our findings support BnaWRKYs as new participants in response to low B, and BnaA9.WRKY47 contributes to the adaptation of B. napus to B deficiency through up‐regulating BnaA3.NIP5;1 expression to facilitate efficient B uptake.

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MODD Mediates Deactivation and Degradation of OsbZIP46 to Negatively Regulate ABA Signaling and Drought Resistance in Rice

Cited by 132 publications

References 80 publications

ABI5-BINDING PROTEIN2 Coordinates CONSTANS to Delay Flowering by Recruiting the Transcriptional Corepressor TPR2

ABI5-BINDING PROTEIN2 Coordinates CONSTANS to Delay Flowering by Recruiting the Transcriptional Corepressor TPR2

Antagonistic Transcription Factor Complexes Modulate the Floral Transition in Rice

Transcription factor BnaA9.WRKY47 contributes to the adaptation of Brassica napus to low boron stress by up‐regulating the boric acid channel gene BnaA3.NIP5;1

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