Abstract
Key message
BnaIAA7 crosstalk with BR signaling is mediated by the interaction between BnaARF8 and BnaBZR1 to regulate rapeseed plant morphogenesis.
Abstract
Auxin (indole-3-acetic acid, IAA) and brassinosteroids (BRs) are essential regulators of plant morphogenesis. However, their roles in rapeseed have not been reported. Here, we identified an extremely dwarf1 (ed1) mutant of rapeseed that displays reduced stature, short hypocotyls, as well as wavy and curled leaves. We isolated ED1 by map-based cloning, and found that it encodes a protein homologous to AtIAA7. ED1 acts as a repressor of IAA signaling, and IAA induces its degradation through its degron motif. A genomic-synteny analysis revealed that ED1 has four homologs in rapeseed, but two were not expressed. Analyses of transcriptomes and of various mutant BnaIAA7s in transgenic plants revealed that the three expressed BnaIAA7 homologs had diverse expression patterns. ED1/BnaC05.IAA7 predominantly functioned in stem elongation, BnaA05.IAA7 was essential for reproduction, while BnaA03.IAA7 had the potential to reduce plant height. Physical interaction assays revealed that the three BnaIAA7 homologs interacted in different ways with BnaTIRs/AFBs and BnaARFs, which may regulate the development of specific organs. Furthermore, BnaARF8 could directly interact with the BnaIAA7s and BnaBZR1. We propose that BnaIAA7s interact with BR signaling via BnaARF8 and BnaBZR1 to regulate stem elongation in rapeseed.
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Introduction
Plant height (PH) is under the integrated control of plant hormones and environmental factors (Salas Fernandez et al. 2009). Among the former, the brassinosteroid (BRs) and gibberellin (GAs) biosynthetic and signaling pathways are the crucial control factors, and mutants with defects in these processes display dwarf phenotypes (Sun 2008; Clouse 2011). In addition, BRs are also involved in the regulation of root growth and the morphological development of leaves and flowers (Zhu et al. 2013). The strigolactones and auxins are other families of plant hormones that affect PH and the outgrowth of axillary buds (Zhao 2010; Ruyter-Spira et al. 2013). Although these mechanisms are well-established in model species (Arabidopsis and rice), the identities of these signals are not known in rapeseed.
The plant growth regulator auxin (indole-3-acetic acid, IAA) plays a crucial role in plant growth and development, including lateral root formation, stem elongation, apical dominance, gravitropism, and vascular development (Woodward and Bartel 2005). Active auxins are synthesized in shoot apical meristems, young leaves, and root meristems (Ljung et al. 2001), and are then transported in or out of the cell by auxin carriers, such as AUX1, PINs, and ABCB/PGPs (Blakeslee et al. 2005). After decades of work, an auxin-signaling pathway has been elucidated (Gray et al. 2001; Dharmasiri et al. 2005; Wang and Estelle 2014). Auxin signal transduction begins with specific binding of auxin receptors TRANSPORT INHIBITOR RESPONSE 1/AUX SIGNALING F-BOX PROTEINS (TIR1/AFBs), and Auxin/Indole-Acetic Acid (Aux/IAAs) transcriptional repressors (Dharmasiri et al. 2005; Calderon Villalobos et al. 2012; Salehin et al. 2015). The Auxin-Response Factors (ARFs) are the downstream targets of Aux/IAAs that bind auxin-response elements (AuxRE) in the promoters of auxin-response genes to regulate their transcription (Weijers et al. 2005).
Most Aux/IAA repressor proteins have four conserved domains (I–IV) (Abel et al. 1996). Domain I is an L × L×L motif, with a transcriptional repression activity, and it recruits the co-repressor protein, TOPLESS (TPL), to inactivate the ARFs (Tiwari et al. 2004). The C-terminal domain (III/IV) is required for homo-dimerization between Aux/IAA repressors or hetero-dimerization between Aux/IAAs and ARF regulators (Kim et al. 1997; Ulmasov et al. 1999). Domain II is related to the instability of Aux/IAA repressors in the presence of auxin, and it can directly interact with TIR1 and auxin (Worley et al. 2000). A mutation of the conserved motif (GWPPV) in domain II abolishes the interactions between TIR1/AFBs and Aux/IAAs, which prevents their degradation and thus alters the auxin response (Ramos et al. 2001; Dharmasiri et al. 2005). In Arabidopsis, dominant missense mutations in domain II produce a series of gain-of-function mutants, such as shy2/iaa3, axr2/iaa7, bdl/iaa12, slr/iaa14, axr3/iaa17, msg2/iaa19, and iar2/iaa28; these mutants display diverse defects in growth and development, including slowed root growth, few lateral roots, curled leaves, dwarfism, and decreased gravitropism (Nagpal et al. 2000; Reed 2001). Conversely, most of the single copy loss-of-function ARF mutants fail to show any obvious growth defects, except for hss/arf2, ett/arf3, mp/arf5, and nph4/arf7 (Hardtke and Berleth 1998; Harper et al. 2000; Nemhauser et al. 2000). Double ARF mutants also display strong auxin phenotypes, suggesting that there are unique and overlapping functions among the ARFs in Arabidopsis (Nagpal et al. 2005; Okushima et al. 2005).
The two key transcription factors in the BR signaling pathway are BRASSINAZOLE-RESISTANT 1 (BZR1) and BRI1-EMSSUPPRESSOR (BES1). They positively mediate BR responses depending on their phosphorylation status (Sun et al. 2010). Recently, auxin and BR were reported to collaborate during some developmental processes (Wang et al. 2014). In Arabidopsis, ARF6 interacts with PIF4 and BZR1 to cooperatively regulate Arabidopsis hypocotyl elongation (Oh et al. 2014). In addition, ARF5 recruits BES1 to its target promoter when treated with IAA or BR (Walcher and Nemhauser 2012). BIN2 can directly phosphorylate ARF2 and ARF7, and, therefore, mediate hypocotyl elongation and lateral root development, respectively (Vert et al. 2008). In rice (Oryza sativa), OsARF19 controls leaf angles by positively regulating OsBRI1 expression (Zhang et al. 2015). Despite these significant advances, mutations in auxin-related genes have not yet been identified in rapeseed, which is allopolyploid. Therefore, the overall understanding of the molecular mechanisms controlling auxin- or BR-mediated plant growth and development remains limited in allopolyploid plants.
In this study, we identified a rapeseed semi-dominant gene extremely dwarf1 (ED1) that encoded an Aux/IAA7 protein, which acts as a transcriptional repressor in auxin signal transduction. In addition, the rapeseed genome has four other BnaIAA7 homologs. These BnaIAA7 homologs have redundant but divergent functions in rapeseed plant morphogenesis, where ED1/BnaC05.IAA7 predominantly functions in stem elongation. Furthermore, we found that BnaARF8 directly interacts with all three expressed BnaIAA7s and BnaBZR1. The rapeseed BnaIAA7–BnaARF8–BnaBZR1 interaction model enhances our understanding of the ways in which BnaIAA7 proteins participate in BR-mediated growth responses.
Materials and methods
Plant materials and growth
The ed1 mutant is a spontaneous mutant obtained from the field and back-crossed with the Ningyou 336 (NY336) strain to generate a homozygous line (from BC5F2) in the ‘NY336’ background. The wild-type (WT) rapeseed varieties used in this study were ‘NY336’ (semi-winter-type) and ‘862’ (spring-type) for transformation analyses. The rapeseed F2 population used for genetic mapping was grown in its natural growing season in Wuhan, China. The seedlings of WT, mutants, and transgenic plants were grown in the greenhouse (under 16 h of light/8 h of dark at 20–23 °C).
Histological analysis
For microscopy, rapeseed stem (five-leaf stage) and young leaf (three-leaf stage) segments were fixed in FAA (formalin–acetic acid–alcohol) solution overnight, followed by a series of dehydration and infiltration steps. The samples were then embedded in Paraffin Plus (Thermo Fisher). The tissues were sliced to reach a thickness of 8–10 μm (Leica RM2265) and then stained with 0.05% toluidine blue. These were observed under an Eclipse E80i light microscope (Nikon). The stem cell size and number were calculated using the Image J software.
The rapeseed leaves were cleaned with chloral hydrate solution (200 g of chloral hydrate, 20 g of glycerol, and 50 ml of dH2O) and photographed with a digital camera (Nikon).
Analysis of endogenous IAA and BR content
For IAA (total) and BR (24-epiBL and 24-epiCS) measurements, 200 mg or 1 g fresh leaves were ground to a fine powder in liquid nitrogen, and the samples were extracted, purified, and analyzed following the standard procedure for liquid chromatography–mass spectrometry (LC–MS) as previously described (Xin et al. 2013; Wang et al. 2015). Each sample was analyzed in triplicate.
Map-based cloning and complementation analysis
To map and identify the ED1 gene, the ed1 mutant was crossed with Y96 (Brassica napus) to generate the F2 population. Ninety-two individuals from the F2 population were genotyped using a 60-k SNP array for preliminary mapping. 750 F2 plants with normal phenotypes were then used for fine mapping with SNP markers (Supplementary Table 1). To confirm that mutation of ED1 resulted in the ed1 phenotype, we generated the Pro35S::ed1 and ProED1::ed1 constructs and introduced them into the hypocotyls of a WT variety ‘862’ (spring-type) via Agrobacterium-mediated transformation (Zhou et al. 2002).
qRT-PCR
Total RNA was extracted using RNA Prep Pure Plant Kits (Tiangen). The cDNA was synthesized using the First cDNA Transcriptase and Oligo (dT)18 primer (Takara). qRT-PCR was performed using a Fast Start Universal Probe Master Mix (Roche) in an ABI 7500 Fast PCR system with three biological replicates. The rapeseed TMA7 gene (BnaC05g11560D) was used as control. Primers for qRT-PCR are listed in Supplemental Table 6. Data were analyzed following the relative quantification method (\(2^{{ - \Delta \Delta C_{T} }}\)).
Pro BnaIAA7s :: GUS reporter gene construction and GUS staining
The fragments’ upstream of the three BnaIAA7s ATG start codons (1967, 2387, and 1970 bp for ED1, BnaA03.IAA7, and BnaA05.IAA7, respectively) were cloned into the DX2181 vector to generate ProC05::GUS, ProA03::GUS, and ProA05::GUS. Primers for PCR amplification are listed in Supplemental Table 6. The three plasmids were transformed into 862 hypocotyls and were then selected using hygromycin (15 mg L−1). Two independent T2 positive transgenic lines were used for histochemical analysis, where GUS staining was performed, as described by Zheng et al. (2015).
Transient expression assays
The ED1 full-length cDNA was cloned into the vectors, pCAMBIA-1305 or pGreenII 0800-LUC, to generate GFP-ED1, ED1-LUC, and ed1-LUC plasmids for subcellular localization analysis or auxin-mediated degradation assays, respectively. The GFP-ED1 fusion proteins were transiently expressed in epidermal cells of Nicotiana benthamiana leaves, where the FIB2-mCherry was used as a nuclear marker (Zheng et al. 2016). The rapeseed protoplast isolation and transformation procedure was carried out as described by Zheng et al. (2018). For measurement of the luciferase activity, rapeseed protoplasts were transformed with ED1/ed1-LUC plasmids and incubated for 18 h; they were then treated with or without 1 or 10 μM IAA for 1 or 4 h, respectively. 40 μM MG132 was added to control samples and incubated for 1 h before IAA treatment to inhibit proteasomal degradation of ED1. The ratios of firefly luciferase (fLUC)/Renilla luciferase (rLUC) were detected using the Dual-Luciferase Reporter Assay System (Promega).
Generating defined mutations in BnaA03.IAA7 and BnaA05.IAA7
To determine whether the other BnaIAA7 copies have a similar function in auxin signal transduction, we constructed ProA03::A03D (P86L) and ProA05::A05D (P87L) that had the same amino acid substitution (P–L) in their GWPPV motifs as ed1. Full-length ed1 cDNA was then cloned into the binary vector under control of the BnaA03.IAA7 promoter to generate ProA03::ed1. The three plasmids were transformed into ‘862’ hypocotyls and selected using phosphinothricin (10 mg L−1). Two independent T2 positive transgenic lines of each construct were used in further phenotypic observation.
Y2H assay
For BnaTIRs/AFBs interaction assays, ED1, ed1, BnaA03.IAA7, and BnaA05.IAA7 full-length cDNAs were cloned into pB424AD (Clontech), while BnaTIRs/AFBs full-length cDNA were cloned into pLexA (Clontech). BnaIAA7/TIRs or AFBs were transformed into the EGY48A strain and selected on control media plates (SD/−Ura/−His/−Trp) for 3 days at 30 °C. Three single clones were then selected by spotting on a selective plate (SD/Gal/Raff/−Ura–His–Trp + X–Gal + BU salts) by incubation for 3 days. For BnaIAA7 and BnaARF interaction assays, the three BnaIAA7 full-length cDNAs were cloned into pGBKT7 (Clontech), and copies of BnaARF full-length cDNA were cloned into pGADT7 (Clontech). The BnaIAA7/ARF plasmids were then transformed into AH109 strain and selected on control media (SD/–Leu–Trp) plate by incubation for 3 days at 30 °C. The interactions were detected on the selective plate (SD/−Leu−Trp−His−Ade + X-a−Gal). Primers for PCR amplification are listed in Supplementary Table 6.
Bimolecular fluorescence complementation (BiFC) assay
The full-length cDNA of BnaBZR1 was cloned into the pVYN (Venus) vector to construct the NV-BnaBZR1 fusion protein and BnaARF8 cloned into the pVYC (Venus) vector was used to produce CV-BnaARF8 fusion proteins, respectively (primer sequences are listed in Supplementary Table 6). The BiFC analyses were performed in rapeseed protoplasts, and NV-bZIP63/CV-bZIP63 was used as positive control (Walter et al. 2004).
RNA-Seq analysis
Total RNA was extracted from 4-week-old 862 strain, 35S::ed1 and ProED1::ed1, leaves with two biological replicates using RNA Prep Pure Plant Kits (Tiangen). The libraries were constructed and sequenced using an Illumina HiSEquation 2000 (Benagen). ~ 25 million raw reads from each sample were collected and filtered. Clean reads were mapped to the reference genome (http://www.genoscope.cns.fr/brassicanapus/) using Hisat2. The gene expression levels were calculated by the FPKM method based on the number of uniquely mapped reads. Differential expression analysis was performed with the DESeq2 R package using |log2 (fold change)| ≥ 1 and a corrected P < 0.05 as the threshold for significant differential expression. P values were adjusted using the Benjamini and Hochberg approach to control for false discovery rates. Functional enrichment analyses, including Gene Ontology (GO) and KEGG, were performed on DEGs, which were compared to the whole genome background using the hypergeometric test with Benjamini and Hochberg’s false discovery rate correction at the significance threshold of 0.05.
Results
ed1 is a semi-dominant mutant and is insensitive to exogenous IAA and brassinolide (BL)
We obtained the ed1 mutant from the field and back-crossed it with the Ningyou 336 (NY336, wild-type) strain to generate a homozygous line. Compared with wild-type (WT), the ed1 mutant showed reduced stature throughout its life cycle and displayed weaker apical dominance (Fig. 1). At the seedling stage, root elongation and lateral root outgrowth were inhibited in ed1 (Fig. 1a, i–iii). At the vegetative stage, the most obvious phenotypes of ed1 were the wavy and curled leaves (Fig. 1b). At flowering, the flowers and pollen grains were smaller than those of WT (Fig. 1c, d). At maturity, the ed1 mutant displayed dwarfism, with shorter siliques (Fig. 1e, f). Briefly, all of the yield-related traits decreased (Table 1). The phenotypes of F1 plants were intermediate between the parental plants, indicating that the ed1 mutation acted in a semi-dominant manner (Fig. 1; Table 1). Genetic analysis of an F2 population generated from a cross between WT and ed1 showed that the curled leaf and dwarfism traits were linked and were controlled by a single semi-dominant gene (Supplementary Fig. 1).
The ed1 mutant displayed curled and dark-green leaves, and had shorter hypocotyls than WT in the light (Fig. 1a, b; Supplementary Fig. 2a), suggesting that ed1 might be defective in IAA or BR biosynthetic or signaling pathways (Reed 2001; Clouse 2011). We, therefore, treated WT and ed1 seedlings (3 days after germination) with several concentrations of either IAA or BL added to their hydroponic culture solution for 4 days or 7 days, respectively, and measured the effect on hypocotyl lengths. The results showed that ed1 is less sensitive to IAA or BL than WT plants (Supplementary Fig. 2b). Moreover, measurements of endogenous IAA and BR showed that ed1 accumulates markedly higher levels of IAA than WT (Supplementary Fig. 2c). Therefore, we hypothesized that ed1 is an IAA/BR-insensitive mutant that is involved in IAA signaling.
Cell elongation or expansion is defective in ed1
To understand the cellular basis of the ed1 dwarfism and small leaf phenotypes, we performed a comparative histological analysis of the stems and leaves of WT and ed1 plants at the four-leaf stage. Examination of cross sections revealed that cell radii in the ed1 stems were significantly reduced, and differentiation of the primary phloem and xylem was repressed. In addition, the sizes of pith and parenchymal cells (PCs) decreased (Fig. 2a, b). Longitudinal sections of the stem showed that the cell lengths and sizes of the pith and PCs significantly decreased in ed1 (Fig. 2c–g). In addition, the pith cells showed an irregular arrangement in ed1 (Fig. 2f).
Whole-mount clearing of WT and ed1 plants at the four-leaf stage revealed that the number of lateral veins was significantly reduced in ed1 plants (Fig. 2h, i). Cross sections of midribs showed that their diameters decreased, but the numbers of PCs did not (Fig. 2j, k). In addition, the sizes of the vascular bundles in the midribs significantly decreased (Fig. 2l, m). Scanning the leaves showed that the sizes of the lower epidermal and mesophyll cells decreased (Fig. 2n–r).
Thus, the cells in ed1 plants displayed a defect in cell elongation or expansion, which led to the plants’ smaller stature.
ED1 encodes a protein homologous to AtIAA7
To isolate the ED1 gene, 92 individuals from the ed1 × Y96 F2 population were genotyped using a 60-k SNP array. The major locus related to the dwarfism phenotype was located on chromosome C05 (Supplementary Fig. 3). We further narrowed the location of ED1 to a 350-kb region between SNP markers ZS-7 and ZS-9 using 750 recessive plants (Fig. 3a; Supplementary Table 1). Twenty-seven open reading frames were predicted to be present in this region, according to the “Darmor-bzh” database (http://www.genoscope.cns.fr/brassicanapus/), including two Aux/IAA genes (BnaC05.IAA2/BnaC05g29330D and BnaC05.IAA7/BnaC05g29300D) (Supplementary Table 2). We sequenced the two candidate genes in ed1 and found a missense mutation (C–T) in the second exon of BnaC05.IAA7 that converted a conserved Pro (position 87) to a Leu in domain II (GWPPV) (Fig. 3b).
To determine whether this mutation in BnaC05g29300D caused the curled leaf and dwarf phenotypes, we generated transgenic plants independently expressing WT and ed1 under the control of CaMV35S (35S) and its native promoter in Arabidopsis or B. napus ‘862’ (spring-type). As expected, the Arabidopsis transgenic plants that expressed ed1 under the control of 35S displayed the dwarf phenotype, which was a phenocopy of the axr2/iaa7 mutant (Gray et al. 2001) (Supplementary Fig. 4a). The ed1 transgenic lines driven by both the 35S and the native promoters displayed curled leaves and dwarfism that phenocopied the original ed1, but the phenotype of the 35S-driven transgenic line was more severe (Fig. 3c; Supplementary Fig. 4b). Therefore, we concluded that the BnaC05.IAA7 (BnaC05g29300D) gene was actually ED1 (Zhao et al. 2019).
ED1 acts as a repressor of IAA signaling and is degraded in response to IAA
Quantitative RT-PCR (qRT-PCR) analyses revealed that ED1 was expressed in various organs, including roots, leaves, axillary buds, and the reproductive organs, but at much higher levels in stems and siliques (Fig. 4a). The β-glucuronidase (GUS) gene driven by the ED1 promoter was transformed into 862 (spring-type) to more precisely detect the expression levels. Consistent with the qRT-PCR results, GUS activity was detected in all organs, but predominately in the stem (Fig. 4b). Further examination of stem cross- and longitudinal sections revealed that GUS was predominately expressed in the vascular bundles (Fig. 4b, ii). In addition, high levels of GUS activity were observed in both the mesophyll and leaf veins (Fig. 4b, iii). Thus, ED1 was constitutively expressed and might play important roles in regulating the normal growth of cells and vascular bundles.
To determine the subcellular localization of ED1, the C-terminal region of GFP was fused to the N-terminus of ED1, and the fusion gene was transiently expressed in epidermal cells of Nicotiana benthamiana leaves. GFP-ED1 co-localized to the nucleus with the nuclear marker FIB2-mCherry (Zheng et al. 2016) (Fig. 4c). In addition, the N-terminal region of ED1 contains an EAR motif (L × L × L), which is involved in transcriptional repression (Tiwari et al. 2004). We fused the GAL4-DNA binding domain to the N-terminus of ED1 or VP16 (a transcriptional activator) to construct effector proteins. The effector and GAL4–UAS–LUC or DR5–LUC reporter were then co-transfected into rapeseed protoplasts in the presence or absence of IAA. ED1 repressed the expression of LUC and DR5–LUC, and this repression was partially alleviated by IAA treatment, indicating that ED1 was a repressor in the auxin-signaling pathway (Fig. 4d).
We further evaluated whether ED1 and ed1 proteins could be degraded in response to auxin. We, therefore, compared the luciferase activities in rapeseed protoplasts 4 h after transfection with ED1–LUC, ed1 (P87L)–LUC, and ed1 (P87S)–LUC in the presence of 0, 1, or 10 µM IAA, IAA treatment induced the rapid degradation of the ED1-LUC but not the mutant ed1 (P87L)–LUC fusion proteins (Fig. 4e). This suggested that auxin rapidly destabilized the ED1 protein and that the P87L substitution in the ed1 protein affected the normal degradation rate. In addition, auxin showed no observable effects on the P87S substitution in domain II, even under high IAA concentrations (Fig. 4e).
P-to-L substitutions in the GWPPV motifs of three BnaIAA7 homologs result in different morphologies
Genomic-synteny and BLASTP (protein–protein BLAST) analyses identified four rapeseed ED1 homologs (Supplementary Table 3; Supplementary Fig. 5). We studied whether these BnaIAA7 homologs had similar spatio-temporal expression patterns to those of ED1 in rapeseed by qRT-PCR analyses. These showed that two BnaIAA7 homologs (C01 and C07) were barely expressed in the tested tissues (data not shown), while BnaA03.IAA7 had higher expression levels in roots and stems than in other tissues, BnaC05.IAA7 showed significant expression in stems and siliques, and BnaA05.IAA7 was predominately expressed in stems, flower buds, and siliques (Fig. 5a). This indicated that the expression of these homologs varied greatly between tissues. To analyze the expression of each BnaIAA7 in more detail, we constructed ProBnaIAA7s::GUS plasmids and transformed them into ‘862’. Histochemical GUS staining of the seedlings showed high expression of BnaA03.IAA7 in young roots, whereas expression of the other homologs was low (Fig. 5b). At the bolting stage, strong GUS signals were detected in the stem of the ProC05::GUS line, but other lines showed weaker signals (Fig. 5b). Thus, the expression analyses and histochemical GUS staining indicated that the three BnaIAA7 homologs might have diverse functions in rapeseed.
To confirm the defective phenotypes of other two BnaIAA7 copies, we next created variants of the BnaIAA7s that mimicked the ed1 mutation by replacing P with L in the GWPPV motif and expressed them in rapeseed using native promoters. In addition, we constructed a plasmid that expressed mutant ed1 controlled by the BnaA03.IAA7 promoter. We then compared the architecture of the homozygous transgenic plants with WT. ProC05::ed1 displayed the shortest stems, ~ 16.5% of the WT stem length, while both ProA03::A03D (P86L) and ProA03::ed1 were semi-dwarf compared with WT (Fig. 5c). Thus, the different expression levels of BnaC05.IAA7 and BnaA03.IAA7 in stems might be responsible for the distinct differences in PH (Supplementary Fig. 6). Notably, all eight of the ProA05::A05D (P87L) T0 positive lines displayed sterility and had decreased PH. This was consistent with the expression analyses, showing that BnaA05.IAA7 was most highly expressed in floral buds (Fig. 5a).
We, therefore, hypothesized that the three homologs of BnaIAA7 might have redundant and divergent functions in regulating rapeseed PH, where BnaC05.IAA7 predominately regulates stem elongation.
IAA affects interactions between BnaIAA7s and BnaTIR1/AFBs
The TIR1/AFB family members function as auxin receptors (Dharmasiri et al. 2005). We, therefore, used yeast two-hybrid (Y2H) assays to analyze interactions between various BnaTIR1/AFB-BnaIAA7 pairs. After eliminating the pairs that showed no interactions, we tested the interactions between seven BnaTIR1/AFBs and the BnaIAA7s across an auxin concentration gradient. Different dose responses were observed for each pair. In the absence of auxin, BnaA03.IAA7 and, to a lesser extent, BnaA05.IAA7, interacted strongly with BnaTIR1, BnaAFB1, and BnaAFB2. In contrast, BnaC05.IAA7 showed a slightly stronger interaction with BnaAFB5 in the absence of auxin (Fig. 6a). As the IAA concentration increased, the strength of the interactions between the BnaIAA7s and most BnaTIR1/AFBs increased, with the exception of BnaAFB2 (BnaA02g28290D) which interacted increasingly weakly with all three BnaIAA7s with increasing auxin concentration (Fig. 6a). In contrast, the interaction of BnaAFB2 (BnaC02g36370D) with the BnaIAA7 homologs did not significantly vary with auxin concentration (Supplementary Fig. 7).
The interactions between the BnaIAA7s and both BnaTIR1 and BnaAFB1 were particularly strong, and BnaC05.IAA7 showed the most obvious increase in interaction with auxin concentration (Fig. 6a; Supplementary Fig. 7). Conversely, BnaAFB3 only interacted with the BnaIAA7s at high auxin levels. Moreover, the mutant ed1 did not interact with any BnaTIR1/AFB1 (Fig. 6a; Supplementary Fig. 7). Thus, each BnaIAA7 homolog appeared to interact differently with the auxin receptors, and the mutation in ED1 domain II might have abolished the interactions between this domain and auxin receptors in yeast.
The three BnaIAA7s interact in different ways with BnaARFs
The Aux/IAAs regulate auxin-response genes by repressing the ARFs (Weijers et al. 2005). In this study, we aimed to determine which BnaARFs interacted with the BnaIAA7s using Y2H assays. We chose products of BnaARF5, BnaARF6, BnaARF8, BnaARF18, and BnaARF19 as the candidate interactors, because these genes are involved in cell elongation or vascular development (Nagpal et al. 2005; Wilmoth et al. 2005; Donner et al. 2009), which are related to the phenotypes of the ed1 plants. All of the tested BnaARFs, except for BnaARF18, exhibited interaction with the BnaIAA7s or ed1 in yeast (Supplementary Fig. 8b). After 4 days on selective plates, BnaA03.IAA7 interacted strongly with BnaARF7s (BnaC08g19040D and BnaA07g11660D), as compared with BnaA05.IAA7 and BnaC05.IAA7 (Fig. 6b). BnaA05.IAA7 had the strongest interaction with BnaARF5 (BnaA06g14040D), while BnaC05.IAA7 showed the strongest interaction with BnaARF5 (BnaC05g15390D) (Fig. 6b). In addition, BnaC05.IAA7 weakly interacted with BnaARF6 (BnaA08g17390D), whereas the other two BnaIAA7s did not. Furthermore, BnaC05.IAA7 interacted more weakly with BnaARF8 (BnaC06g27170D) and BnaARF19 (BnaA06g13320D) than BnaA03.IAA7 and BnaA05.IAA7, but more strongly than the other two BnaIAA7s with BnaARF8 (BnaC03g59640D) (Fig. 6b).
BnaIAA7s affect BR signaling via the interaction between BnaARF8 and BnaBZR1
The ed1 mutant had an abnormal plant architecture that was similar to BR-related phenotypes, including short stems and curled and dark-green leaves. We, therefore, performed an RNA-Seq analysis in which WT was compared separately with ProED1::ed1 and 35S::ed1 homozygous plants to determine whether the ed1 mutation affected the BR-response pathway. The transcriptome analysis identified 397 genes that had decreased expression levels (> 1.5-fold) compared to wild type in both ProED1::ed1 and 35S::ed1 and 1247 genes that had increased expression (> 1.5-fold) relative to wild type in both transgenic lines (Fig. 7a; Supplemental Datasheet). A gene ontology (GO) analysis showed that some of these genes responded to auxin or BR, or were involved in hormone biogenesis, while other genes involved in cell wall organization were highly enriched (Fig. 7b). In addition to the differentially expressed genes that were related to auxin or BR biosynthesis and signaling, we identified differentially expressed genes related to cell elongation/expansion that had previously been reported to be downstream targets of BZR1 (Sun et al. 2010) (Table 2; Supplementary Table 4).
Notably, no change in the expression level of either BnaBZR1 or BnaBES1 was detected, and expression levels of BnaARFs were unchanged in the two transgenic lines. The BnaARFs are the downstream targets of BnaIAAs, and we hypothesized that some BnaARFs might interact with BnaBZR1 in rapeseed. Y2H assays revealed that BnaARF8 directly interacted with BnaBZR1 (Fig. 7c). Similarly, BiFC assays showed that BnaARF8 interacted with BnaBZR1 in the nuclei of rapeseed protoplasts, and even in ed1 protoplasts, indicating that the domain II of ED1/BnaC05.IAA7 does not mediate these interactions (Fig. 7d). These results indicated that the interaction between BnaARF8 and BnaBZR1 might act as a bridge between auxin and BR signaling in rapeseed growth and development.
Discussion
In this study, we identified an ed1 mutant in rapeseed that displayed extreme dwarfism, a curled leaf phenotype and short hypocotyls. These phenotypes were similar to those of some Arabidopsis mutants deficient in auxin/BR biosynthesis or signaling (Clouse 2011; Reed 2001). Exogenous hormonal treatments showed that, compared with WT, hypocotyl elongation of the ed1 mutant was insensitive to IAA and BL. This observation was consistent with previous studies of the Arabidopsis iaa7/axr2 mutant (Nemhauser et al. 2004; Nakamura et al. 2006). Significantly, the changes caused by the two treatments on ed1 plants were the same (Supplementary Fig. 2b). In addition, the RNA-Seq analysis revealed that several genes related to IAA and BR synthesis or signaling were aberrantly expressed in ProED1::ed1 and 35S::ed1 plants (Table 2). The finding that the expression of IAA biosynthesis genes increased implies that there is a negative feedback loop controlling auxin levels in the ed1 mutant. Thus, the IAA- and BR-signaling pathways may be simultaneously deficient in the ed1 mutant, and auxin might mediate growth responses through BR signaling or the two hormones may have overlapping target genes that regulate cell elongation or expansion.
Our study showed that ed1, which has a mutation in domain II (GWPPV motif), is a gain-of-function mutant. In Arabidopsis, most Aux/IAAs repressor mutants have a mutation in either of the two Pro residues in domain II, which causes them to exhibit severe phenotypes (Reed 2001). Domain II is a degron motif that directly contacts TIR1 and auxin; therefore, a mutation in domain II can abolish the interaction between Aux/IAA repressors and TIR1/AFBs (Tan et al. 2007; Calderon Villalobos et al. 2012). Our interaction assays showed that the mutant ed1 protein lost its ability to bind BnaTIR1/AFBs, but could still interact with BnaARFs (Fig. 6; Supplementary Fig. 8b). Therefore, the mutation in ed1 probably abolished the interaction with the SCFTIR1/AFBs (auxin) complexes in yeast. Conversely, degradation assays in rapeseed protoplasts revealed that the P87L substitution in domain II decreased the degradation rate compared with WT, and the protein with the P87S substitution could not be degraded after IAA treatment. Thus, variation at residue 87 might result in different degradation rates. Therefore, the mutant ed1 (P87L) might have a weak interaction with the SCFTIR1/AFBs (auxin) complexes, at least in rapeseed (Fig. 4e).
Auxin and BR interact in some plant growth and developmental process, including hypocotyl and root elongation in Arabidopsis and leaf angle regulation in rice (Vert et al. 2008; Oh et al. 2014; Zhang et al. 2015). In Arabidopsis, the bzr1-1D mutant exhibits reduced PH, and bes1 and bzr1 mutants have defects in phloem and xylem differentiation (Saito et al. 2018). Transcriptome analyses revealed that the expression levels of BZR1 downstream targets involved in cell elongation or expansion decreased in the axr2/iaa7 mutant and ProED1::ed1 plants (Table 2; Supplementary Table 5). In addition, the arf6-2 or arf6-2 arf8-3 mutants display decreased internodes or infertile flowers (Nagpal et al. 2005). In our study, BnaARF8 directly interacted with BnaIAA7s and BnaBZR1. Notably, the differentiation of the primary phloem and xylem was arrested, and the vascular bundle size was reduced in ed1 mutant leaves (Fig. 2j–m). A recent study revealed that the mutation of the degron motif of PtoIAA9 significantly repressed secondary xylem development in poplar via interaction with PtoARF5s (Xu et al. 2018). ARF5 could recruit BES1 to its target promoter when treated with IAA or BR in Arabidopsis (Walcher and Nemhauser 2012). Our study also found that three BnaIAA7s interact with BnaARF5s to different extents (Fig. 6b). Therefore, the BnaIAA7 proteins might be involved in BR-mediated growth responses via BnaBZR1 in rapeseed. In Arabidopsis, the bzr1 and bes1 single- or double-deficient mutants did not display obvious phenotypes in plant architecture, which may be the result of the presence of four additional BES-like homologs in the Arabidopsis genome (Saito et al. 2018). Similarly, both BnaARFs and BnaBZRs have many homologs in the rapeseed genome making it difficult to obtain mutants with obvious phenotypes. Intriguingly, bes1-RNAi lines that show decreased expression of several BZR/BES-like genes exhibit defects in stem elongation, indicating that simultaneously knocking down these functional redundant genes will obtain expected phenotypes (Wang et al. 2013). In the future, loss-of-function mutants of BnaBZR1/BES1-like homologs will be created by CRISPR/Cas9-mediated mutagenesis for genetic analysis between bnabzr/bes1 and bnaiaa7s to illuminate the roles of BZR1/BES1 genes in vascular development.
Most duplicated genes diverge in their expression levels (Blanc and Wolfe 2004; Zheng et al. 2016). Our expression pattern analyses showed that the expression of the three BnaIAA7 homologs varied between organs (Fig. 5a). Promoter sequence comparisons also showed that there were major differences between the three BnaIAA7s (Supplementary Fig. 9). Variants with substitutions in domain II revealed that ED1/BnaC05.IAA7 was a major factor in stem and silique elongation during rapeseed growth and development, while BnaA05.IAA7 was essential for rapeseed reproduction. In Arabidopsis, the overexpression of a poplar IAA14 (PtrIAA14) which had many amino acid differences with AtIAA14 resulted in reduced fertility (Liu et al. 2015). Acetic acid magenta staining assays revealed that the pollen of ProA05::A05D (P87L) transgenic plants was normal (data not shown); thus, the BnaA05.IAA7 mutation might affect the embryo sac. In addition, there was only a slight difference between ProA03::ed1 and ProA03::A03D (P86L) plants in PH, but an obvious difference in leaf morphology (Fig. 5c; Supplementary Fig. 10), suggesting that ED1 and BnaA03.IAA7 had functional differences. The interaction assays in yeast also showed that the three BnaIAA7s interacted differently with BnaARF5/19, whose Arabidopsis homologs play roles in regulating vascular development and leaf expansion (Wilmoth et al. 2005; Donner et al. 2009). Meanwhile, the three BnaIAA7 proteins also had several amino acid differences (Supplementary Fig. 5), indicating that the BnaIAA7s had functional differences in repressing BnaARF activity levels (Muto et al. 2007).
Recently, a G-to-E mutation in the GWPPV motif of BnaA3.IAA7 was found to contribute to yield heterosis by improving plant architecture with decreased PH and branch angle (Li et al. 2018). Notably, in our study, the ProA03::A03D (P86L) homozygous plants exhibited a semi-dwarf phenotype with major changes in leaf morphology but no change in branch angle (Supplementary Fig. 10), The phenotypic differences between the two mutant forms in the BnaA03.IAA7 degron motif might be due to the protein conformation changes resulting from the different properties of these residues, as Gly (G) affects the flexibility of Aux/IAAs, while the first Pro (P) is involved in packing auxin into the TIR1 pocket (Tan et al. 2007). Significantly, the semi-dominant BnaA03.IAA7 (P86L) mutation also has the potential application to breed decreased PH in rapeseed, and further studies will be performed to detect whether it can increase the yield.
Author contribution statement
MZ, MH, JZ, HP, and WH designed the experiments; MZ, MH, HY, MT, LZ, XL, and JL performed the experiments; HL analyzed the RNA-Seq data; XS and SF characterized the agronomic traits; MZ and MH wrote the manuscript, and WT revised the manuscript. All authors read and approved the final manuscript.
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Acknowledgements
We thank CK. Q. for providing the ed1 mutant that introduced from G. Buza. We also thank the support from Jiangsu Collaborative Innovation Centre for Modern Crop Production, China. This research was supported by the grants from the National Natural Science Foundation of China (31801402), the National Key Basic Research Program of China (2015CB150200), the National Key Research and Development Program of China (2016YFD0101300), and the China Agricultural Research System (CARS-13).
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Zheng, M., Hu, M., Yang, H. et al. Three BnaIAA7 homologs are involved in auxin/brassinosteroid-mediated plant morphogenesis in rapeseed (Brassica napus L.). Plant Cell Rep 38, 883–897 (2019). https://doi.org/10.1007/s00299-019-02410-4
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DOI: https://doi.org/10.1007/s00299-019-02410-4