Genome-wide identification of Aux/IAA gene family in white clover ( Trifolium repens L.) and functional verification of TrIAA18 under different abiotic stress

Background White clover ( Trifolium repens L.) is an excellent leguminous cool-season forage with a high protein content and strong nitrogen-fixing ability. Despite these advantages, its growth and development are markedly sensitive to environmental factors. Indole-3-acetic acid (IAA) is the major growth hormone in plants, regulating plant growth, development, and response to adversity. Nevertheless, the specific regulatory functions of Aux/IAA genes in response to abiotic stresses in white clover remain largely unexplored. Results In this study, we identified 47 Aux/IAA genes in the white clover genome, which were categorized into five groups based on phylogenetic analysis. The TrIAAs promoter region co-existed with different cis-regulatory elements involved in developmental and hormonal regulation, and stress responses, which may be closely related to their diverse regulatory roles. Collinearity analysis showed that the amplification of the TrIAA gene family was mainly carried out by segmental duplication. White clover Aux/IAA genes showed different expression patterns in different tissues and under different stress treatments. In addition, we performed a yeast two-hybrid analysis to investigate the interaction between white clover Aux/IAA and ARF proteins. Heterologous expression indicated that TrIAA18 could enhance stress tolerance in both yeast and transgenic Arabidopsis thaliana . Conclusion These findings provide new scientific insights into the molecular mechanisms of growth hormone signaling in white clover and its functional characteristics in response to environmental stress.

repressors in the auxin signaling pathway [4,5].The first Aux/IAA family member was isolated from soybeans (Glycine max) and subsequently identified in wheat (Triticum aestivum L.), rice (Oryza sativa L.), tomato (Solanum lycopersicum), and other crops [6][7][8][9].Generally, the Aux/IAA protein consists of four protein-conserved domains, I, II, III, and IV, of which domain I contains the conserved motif 'LxLxL' , which can interact with the TPL family of co-suppressors (TOPLESS) to form a co-repressor [10][11][12].Domain II contains a conserved "GWPPV" motif that plays a role in the ubiquitination and degradation of Aux/IAA proteins by interacting with SCF TIR1 [13].Domains III and IV are homologous to PB1, the C-terminal domain of the ARF protein, and can interact with ARFs to repress the expression of auxin-responsive genes [14].In addition, there are truncated Aux/IAA proteins that do not have domain III or domain IV, such as the CpIAA11, CpIAA19, CpIAA27, and CpIAA31 proteins in papaya (Carica papaya L.) [15].
In the auxin signaling pathway, auxin receptor TIR1/ AFB (Transport Inhibitor Resistant/Auxin Signaling F-Box), transcriptional repressor Aux/IAA, and plant auxin response factor (Auxin Response Factor, ARF) are the three types of regulators [16,17].In the absence or at low auxin concentrations, the Aux/IAA protein interacts with the ARF protein through a homologous structural domain at the C-terminus, thus hinders the direct transcriptional regulatory effects of ARF on auxinresponsive genes [18][19][20].Under high auxin levels, auxin binds to the receptor TIR1/AFBs, which makes it easy for TIR1 to bind with Aux/IAA proteins, and induces SCF TIR1 -mediated ubiquitination degradation of Aux/ IAA proteins [21,22].As a consequence, ARF proteins are released which turn on the transcriptional regulation of downstream genes [23].However, the interaction between Aux/IAA and ARF proteins during the auxinsignaling pathway could regulate the expression of downstream genes has remained uninvestigated so far.
The functional characterization of Aux/IAA-encoding genes has been substantiated through mutants and overexpression studies in Arabidopsis thaliana.For example, the loss of function of atiaa3/shy2 and atiaa28 mutations results in defective lateral root formation [24,25].AtIAA12 and AtIAA18 can regulate embryo apical conformation and root meristem formation by inhibiting AtARF5 activity [26,27].In addition, SlIAA27 controls the biosynthesis of strigolactone through the regulation of NODULATION SIGNALING PATHWAY1 (NSP1), therefore complementing the defective phenotype of mycorrhizal roots [28].Recent studies have indicated that Aux/IAA genes are extensively involved in plants' responses to abiotic stress.For instance, it has been discovered that the expression level of the sorghum SbIAA1 gene is significantly induced under salt and drought stress [29].In Arabidopsis, loss of AtIAA5/6/19 resulted in reduced Glucosinolates (GLS) levels, thus resulting in reduced drought tolerance.In addition, all three single mutants, as well as the iaa5/6/19 triple mutant, were hypersensitive to drought when compared to the Wild Type (WT) [30].Auxin has been reported to negatively regulate Aluminum (Al) resistance by altering the expression and distribution of Al-sensitive protein 1 in Arabidopsis root cells, where co-treatment of IAA with Al significantly reduced Al content in root tips [31].In rice, OsIAA6 may trigger an auxin-mediated drought response by regulating the expression of auxin synthesis genes, thereby improving drought tolerance [32].Under drought and salt stress, the expression level of the OsIAA20 gene was enhanced, and overexpression of the gene significantly improved drought and salt tolerance in rice [33].The TaIAA15-1A gene in wheat enhanced drought tolerance in brachypodium by regulating ABA-related genes and increasing antioxidant stress capacity [34].Therefore, the identification of Aux/IAA genes and their functions is highly indispensible for growth and development, as well as improvement of crop resistance under different environmental conditions.
White clover (Trifolium repens L.) is an important forage legume and excellent lawn plant with high nutritional value and palatability.The lack of validated molecular markers and genetic maps for the white clover genome makes it difficult to perform genetic analysis and functional annotation [35][36][37].However, whether Aux/IAA family members are involved in different biological processes of white clover has remained unclear so far.In this study, we identified and characterized 47 Aux/IAA genes in the white clover genome and analyzed their gene structure, phylogenetic relationships, chromosomal localization, motif patterns, cis-acting elements, and expression patterns under Al, drought, and salt stresses.Finally, we verified that TrIAA18 interacted with TrARF5 using a yeast two-hybrid.We also examined the positive effects of heterologous yeast expression and overexpression of TrIAA18 in Arabidopsis under Al, drought and salt stress.These findings will provides better understand about the role and evolution of Aux/IAA genes and further supporting the study of other herbaceous Aux/IAA genes.

Identification of TrIAA members in T. repens
A total of 47 IAA genes were identified and confirmed in the white clover genome based on the Aux domain (PF02309).According to the location of these genes on the chromosome, they are tentatively named TrIAA1-TrIAA47.The amino acid lengths of all TrIAA genes were 135-942 aa.Relative Protein Isoelectric points (PI) ranged from 5.16 to 10.08.The Molecular Weight (MW) ranged from 15.20 kDa to 105.17 kDa.In addition, based on subcellular localization predictions, 38 TrIAA proteins were localized to the nucleus, 8 TrIAA proteins were localized to chloroplasts, and 1 TrIAA protein was localized to the cell membrane.The diversity of subcellular localization implies a variety of biological functions within members of the white clover IAA gene family [38].All details are shown in Table S1.

Phylogenetic analysis of IAA genes in T. repens
To explore the evolutionary relationships of TrIAA genes with IAAs of other species, a phylogenetic tree was constructed using 29 AtIAAs and 18 MtIAAs from Arabidopsis and Medicago truncatula (Fig. 1, Table S2).According Tr -IA A 37 At -IA A2 6 At-IA A18

Gene structure, motif, and cis-element analysis of TrIAA genes
We also established a phylogenetic tree of TrIAAs (Fig. 2A).Ten different conserved motifs were identified using the MEME tool.Among the 47 TrIAA, only motif 2 was common, indicating that this structural domain was highly conserved in the IAAs family (Fig. 2B).This was followed by motif 1, motif 3, and motif 4 being relatively conserved in the IAAs family.Furthermore, gene structure analysis showed that the number of introns in the 47 TrIAA genes ranged from 0 to 12, with no introns in TrIAA10.The number of exons was 1 to13, and genes clustered together generally contained similar structures (Fig. 2C).Interestingly, TrIAA23 has 5 exons and exhibited the longest gene length, possibly caused by a mutation in the gene [39].

Chromosomal distribution and synteny analysis of IAA genes in white clover
To better understand the distribution mechanism of TrIAA gene chromosomes, a chromosome map of TrIAA was constructed using TBtools.The results showed that all chromosomes had TrIAA gene except chromosome 7, which lacked TrIAA gene (Fig. 3).Among them, chromosomes 1, 3 and 9 had six TrIAA genes, while chromosome 6, 11, 12 and 13 exhibited only one TrIAA gene, respectively.

Expression patterns of TrIAA genes under abiotic stresses and subcellular localization
To further investigate the transcriptional changes of TrIAA in response to different abiotic stress treatments, we randomly selected 8 TrIAAs representing the three branches of TrIAAs in the phylogenetic tree.We analyzed their expression patterns in roots and leaves using qRT-PCR at different time intervals under various stress conditions (Fig. 6).Under Al (pH = 4.5) stress, TrIAA17 and TrIAA18 were expressed at significantly higher levels in roots than the control, especially at 24 h.TrIAA17 and TrIAA30 were highly expressed in leaves compared to the control.Under drought stress, TrIAA1, TrIAA17 and TrIAA18 were highly expressed at 24 h compared to the control, whereas TrIAA30, TrIAA35, TrIAA39 and TrIAA40 showed a gradual decrease in expression in leaves.However, the expression of most TrIAA was upregulated under salt treatment.Among them, TrIAA1 was significantly elevated in both roots and leaves, followed by TrIAA17 and TrIAA18.In addition, TrIAA9 was preferentially expressed in leaves.The results suggest that TrIAA gene family members can respond to different stress conditions.
According to the qRT-PCR results, TrIAA18 was selected for subcellular localization analysis because it was strongly induced by AlCl 3 , PEG and NaCl treatments.The full-length CDS of TrIAA18 was cloned from 'Ladino' and then used to construct the corresponding transient vector for injection into rice protoplasts.As shown in Fig. 7, the TrIAA18-GFP fusion protein was expressed in the transformed protoplasts and localized in the nucleus, demonstrating the role of TrIAA18 as a transcription factor regulating relevant biological processes.

TrIAA18 expression enhances abiotic stress tolerance in yeast and interacts with TrARF5
The coding sequence of TrIAA18 was cloned and expressed in Saccharomyces cerevisiae strains BY4741 and INVSC1, respectively.Positive BY4741 yeast cells were plated on Synthetic Galactose Minimal Medium without Uracil (SG-Ura) containing 2 mM AlCl 3 , and positive INVSC1 yeast cells were plated on SG-Ura containing 2 M D-Mannitol and 1.5 M NaCl.Yeast overexpressing TrIAA18 grew better than the wild type under Al, drought, and salt stress conditions (Fig. 9A).When the bacterial solution was diluted to 10 -threefold , wild-type yeast could not survive at 1.5 M NaCl, but transgenic yeast overexpressing TrIAA18 could grow well under these conditions (Fig. 9A).These results suggest that TrIAA18 may respond positively to abiotic stress.
To explore potential roles of TrIAA18, protein-protein interaction was predicted against the protein databases of a model plant (Arabidopsis) and a legume plant species (red clover) using STRING (https:// string-db.org/).As shown in Fig. 8A, AtIAA27 (a TrIAA18 homolog) may interact with three AUX/IAA proteins (IAA6, IAA31, and AUX1), six ARF proteins (ARF5, ARF7, ARF8, ARF9, ARF18, and ARF22), and the TIR1/AFB protein (TIR1).Similarly, interactions were predicted between homologs of TrIAA18 in red clover (L195_g015546) and seven ARF proteins.Since high protein identity exists between TrIAA18 and AtIAA27 as well as L195_g015546 (56.9% and 96.4%, respectively; Fig. 8B), TrIAA18 may be involved in abiotic stress response through interaction with ARF proteins.Here, we performed a yeast two-hybrid assay to verified that the TrIAA18 was not transcriptionally active and cotransformed AH109 yeast with TrARF5.As shown in Fig. 9B, the cotransformed positive yeast turned blue on the defective medium (SD-Trp-Leu-His-Ade) containing x-α-gal.The results showed that TrIAA18 interacted with TrARF5.

TrIAA18 overexpression in Arabidopsis improves abiotic stress tolerance
To further investigate the function of TrIAA18 during stress response, three independent homozygous T3-generation transgenic Arabidopsis plants were studied under different stress treatments (Fig. 9C,   D).Phenotypic analysis indicated that under 0.2 mM Al treatment, the root lengths of all three TrIAA18-OE plants were significantly longer than those of WT plants (Fig. 9D).Under 100 mM D-Mannitol treatment, only TrIAA18-OE3 plants had significantly longer root lengths compared to WT plants (Fig. 9D).Under 100 mM NaCl treatment, TrIAA18-OE3 and TrIAA18-OE5 strains had significantly or highly significant root lengths than WT plants (Fig. 9D).These results indicate that transgenic plants are more resistant to Al, D-Mannitol and salt stresses compared to WT plants.

Disscussion
The Aux/IAA gene family is a family of plant-specific transcription factors that play important roles in growth factor signaling and various physiological processes [2,4].White clover is an excellent forage legume with high protein and good palatability, but its growth and development are often susceptible to various environmental adversities [36].While extensive research has been conducted on the Aux/IAA genes of model plants like Arabidopsis and rice, the exploration of these genes in white Arabidopsis thaliana Trifolium repens clover remains limited.Therefore, the study of the Aux/ IAA gene in white clover will not only help to reveal its growth hormone signaling mechanism but also help to explore its stress tolerance mechanism.In this study, using annotated files and newly released white clover genome data, 47 Aux/IAA genes were identified by homology comparison and structural domain analysis and designated as TrIAA1-TrIAA47 [42].Compared with 29 in Arabidopsis [43] and 18 in M. truncatula [44], the number of Aux/IAA genes was significantly increased in white clover and showed extensive variations in Open Reading Frame (ORF) length, predicted MW, and PI.These changes suggest that different TrIAA proteins may function in different microenvironments [5,45,46].According to phylogenetic analyses, most TrIAAs were closely related to AtIAAs and MtIAAs.AtIAA18 was found to be associated with lateral root formation in Arabidopsis.A previous study showed that the AtIAA5/6/19 deletion resulted in reduced GLS levels and decreased drought tolerance, suggesting that Aux/IAA proteins could regulate drought tolerance in Arabidopsis by regulating GLS levels [30].Taken together, these data suggest that the TrIAA genes, which are closely related to AtIAA and MtIAA, may also be involved in growth and development and response to abiotic stresses.AUX/IAA proteins typically have four conserved structural domains that define members of the gene family, referred to as I, II, III, and IV [10][11][12].A total of 16 TrIAA proteins contain four structural domains, while other proteins were missing at least one structural domain.Analysis of the exon/intron structure of the gene showed that the number of exons/introns in TrIAA was highly variable, ranging from 1 to 13, similar to Arabidopsis [44,47].Taken together, the structural features of TrIAA proteins within each subfamily are relatively conserved, and the structural variability among different TrIAA genes may contribute to the functional diversity of the AUX/ IAA gene family.In addition, cis-regulatory elements in the promoter region play important roles in plant growth and development, secondary metabolism and response to adversities [48,49].In this study, most TrIAA gene promoters contained growth hormone-responsive (AuxRE/ TGA-element) cis-elements or their variants [50].Some TrIAA gene promoters have been reported to contain ciselements involved in abiotic stress response, for example, LTR is involved in low temperature response [51], MBS plays a role in drought-inducibility [52,53], ARE is involved in anaerobic induction, and TC_rich_repeats are involved in defense and stress response [54].In conclusion, the different types of cis-elements on the promoters of the TrIAA gene family reflect the complexity and diversity of gene expression regulation and evolution.
Gene duplication events promote rapid expansion and evolution of species gene families by doubling chromosomes.A total of 8 gene pairs with gene duplication events (7 segmental duplication gene pairs and 1 tandem duplication gene pair) were identified in white clover, suggesting that the expansion of the TrIAA gene family may have occurred primarily through segmental duplication [40,41].The covariance of IAA genes in white clover, Arabidopsis, red clover, M. truncatula, and soybean was analyzed using TBtools (v2.019,Chengjie Chen, Guangzhou, China) software.A total of 15 TrIAA-AtIAA pairs, 34 TrIAA-MtIAA pairs, 37 TrIAA-TpIAA pairs, and 79 TrIAA-GmIAA pairs were observed in the Aux/IAA family.The results showed that white clover was phylogenetically more related to soybean than to Arabidopsis.Previous studies have shown that AUX/IAA genes have regulatory functions in abiotic stresses.For example, OsIAA20 confers drought and salt tolerance to transgenic rice by increasing proline and chlorophyll content via ABA signaling pathway [33].OsIAA6 is involved in the downward growth of the rice root system, thereby enhancing drought tolerance [32].In this study, TrIAA genes showed different expression patterns in different tissues and under different stress treatments.Among them, the expression levels of TrIAA17 and TrIAA18 were highly expressed at different time points under Al, drought, and salt stresses, indicating the potential multiple functions of this gene.It was further verified by yeast heterologous expression and transgenic Arabidopsis that TrIAA18 could enhance its stress tolerance.Our research provides insights into the expression spectrum of TrI-AAI8 under various stress conditions, but further studies are needed to elucidate the stress response mechanisms in white clover and to confirm its potential as a target for enhancing plant stress tolerance.
In addition, it has been demonstrated that AUX/IAA proteins can interact with ARF proteins to regulate the expression of downstream target genes.In wheat, TaIAA8 was localized in the nucleus and responded to growth hormone signaling, thereby regulating lateral root growth by interacting with TaARF21 [55].In apple (Malus domestica), MdARF13 affects anthocyanin synthesis by interacting with MdIAA121, which is characterized by growth hormone-induced degradation of MdIAA121 and release of MdARF13, which negatively regulates anthocyanin metabolic pathways [56].However, the regulation of plant responses to abiotic stresses by Aux/IAA and ARF through specific interactions has rarely been reported.In this study, we confirmed that TrIAA18 could interact with TrARF5 by yeast two-hybrid assay.It is hypothesized that TrIAA18 may enhance stress tolerance by affecting TrARF5, but its regulatory function needs to be further explored in future studies.However, current research has preliminarily elucidated the response of the TrIAA18 to abiotic stress, and it is important to recognize the potential role of other Aux/ IAA genes in mediating stress responses.Future research could benefit from a broader examination of the Aux/IAA gene family, exploring the synergistic effects and regulatory networks that contribute to the plant's resilience.Such an inclusive approach would not only enhance our understanding of the gene family's collective response to environmental challenges but also pave the way for developing more robust stress-tolerant crops.

Conclusion
In conclusion, 47 IAA gene family members were identified from the white clover genome and categorized into five classes based on their phylogenetic relationships with Arabidopsis and M. truncatula IAA.Structural analyses, including gene structure, motif composition, and homologous protein modeling, indicated that TrIAA proteins in specific subfamilies were relatively conserved.The coexistence of different cis-regulatory elements involved in developmental regulation, hormones, and stress responses in their promoter regions may be closely related to the multiple regulatory roles of TrIAAs.Collinearity analyses indicated that the expansion of the TrIAA gene family might have occurred primarily through segmental duplication, whereas many other duplicate gene pairs exhibited different expression profiles, suggesting their functional diversity.Finally, TrIAA18 was shown to be involved in the positive regulation of Al, drought, and salt stress, as well as interaction with TrARF5, indicating that TrIAA18 may regulate abiotic stress responses by affecting TrARF5.These results will provide foundation for future studies about the regulatory functions of IAA proteins in forage legumes exposed to abiotic stresses.

Plant materials and treatments
The white clover cultivar 'Ladino' used in this study was purchased from Evergeen International Co., Ltd.Seeds of Ladino were first germinated in plastic containers with quartz sand and sterile ddH 2 O (22/20 ℃, 16/8 h, light/ dark).After one week, seedlings were allowed to grow in Hoagland's nutrient solution for the next 23 days.Later, one-month-old white clover seedlings were subjected to Al stress (2 mM AlCl 3 ), drought stress (15% PEG), and salt stress (100 mM NaCl), respectively.Leaves and root samples were collected at 0, 3, 6, 12, and 24 h after stress treatments.Samples for all time points were taken with three independent biological replicates, frozen in liquid nitrogen, and stored at -80 ℃.

Gene structure, motif and cis-element analysis
The exons and introns of each TrIAA gene were obtained from the white clover genome annotation file.Conserved protein motifs were predicted using the MEME Suite web server (https:// meme-suite.org/) with a maximum number of 10 motif sets and an optimal width of 5 to 200 amino acids [66].The exons and introns of the TrIAA gene, as well as the conserved motifs and structural domains of the TrIAA protein, were visualized and analyzed using TBtools software.Finally, the PlantCARE database (http:// bioin forma tics.psb.ugent.be/ webto ols/ plantcare/html/) was used to analyze cis-acting elements in genomic DNA sequences 2000 bp upstream of the transcription start site of each TrIAA gene [67].

Chromosomal locations, gene duplication, and syntenic analysis
The chromosomal location of each TrIAA gene was retrieved from the GFF3 file of the white clover genome and visualized using TBtools.The Multiple Covariance Scanning Toolkit (MCScanX, default parameters) was utilized to analyze the duplication events of the TrIAA gene [68].TBtools software was used to construct synchronization maps of white clover with four other plants (Arabidopsis, red clover, M. truncatula, and soybean).

RNA extraction and qRT-PCR analysis
Total RNA was extracted from leaf and root samples using the HiPure Plant RNA Mini Kit (Magen, Guangzhou, China).cDNA was synthesized using the Monad MR00101 kit (Monad, Suzhou, China).cDNA was then analyzed on a CXF Connect ™ Real-Time System (Bio-RAD) using the ABM ® Evagreen 2 × QPCR Master Mix (ABM, Canada), following the manufacturer's protocol.qRT-PCR analyses were performed according to the manufacturer's protocol.The ACTIN gene was used as an internal reference.Gene expression was quantified using the 2 −∆∆CT method [69].Three biological replicates were used for each data point.The primers used in this study are listed in Table S6.

Subcellular localization analysis of TrIAA18-GFP protein
The CDS of TrIAA18 was fused to the PAN580 subcellular localization vector, with Green Fluorescent Protein (GFP) at the N-terminus.Rice protoplasts were prepared and transformed as described previously [70], and then stained using a confocal laser scanning microscope (ZESS LSM880) to observe the green fluorescence signals.

Heterologous expression of TrIAA18 in yeast
The CDS sequence of the TrIAA18 was amplified using homology arm primers with restriction endonuclease cleavage sites NdeI and BamHI.The TrIAA18 was then ligated into the pYES2 vector using the MonClone ™ Single Assembly Cloning Mix (Monad, Suzhou, China) and transformed into Escherichia coli DH5α using heat excitation.Saccharomyces cerevisiae strains, BY4741 and INVSC1 were further transformed with the pYES2-TrIAA18 recombinant vector using the Yeast Transformation Kit (Coolaber, Beijing, China).Yeast cells were transformed in the presence of uracil-free glucose (SD-Ura) agar medium for growth.SG-Ura agar medium without and containing 2 mM AlCl 3 (pH = 4.5), 2 M D-Mannitol, and 1.5 M NaCl was prepared as described in the literature [71].Positive transformants were identified and incubated with SG-Ura liquid medium containing galactose until OD 600 = 1, then serially diluted (OD 600 = 1, 10 -1 , 10 -2 , 10 -3 , 10 -4 ). 8 μL of each dilution was dropped into a different medium and incubated at 30 °C for 3-5 days.

Yeast two-hybrid assay
The TrIAA18 protein sequence was submitted to the STRING website (http:// string-db.org).Direct homologs of Arabidopsis and red clover were selected as references for constructing the reciprocal network [72].Yeast two-hybrid assays were performed using the Yeastmaker Yeast Transformation System 2 (Clontech, San Francisco, CA, USA).The coding sequences of TrARF5 and TrIAA18 were cloned into the pGADT7 and pGBKT7 vectors, respectively.The pGADT7-TrARF5 and pGBKT7-TrIAA18 plasmids were transformed into Saccharomyces cerevisiae strain AH109 using the lithium acetate method [73].Yeast cells were cultured on defective (-Leu/-Trp) medium according to the manufacturer's instructions.Positive yeast cells were plated onto defective (-Leu/-Trp/-His/-Ade) medium containing X-gal to verify their interaction.

Fig. 1
Fig.1Phylogenetic analysis representing the relationship between IAA proteins in white clover, Arabidopsis, and M. truncatula.IAA subgroups (classifications I, II, III, IV, V) are marked with different colors.The phylogenetic tree was drawn using the neighbor-joining (NJ) method with a bootstrap value of 1000

Fig. 2
Fig. 2 Phylogenetic relationships, motif patterns and gene structures of the white clover IAA gene family.A Phylogenetic tree of the white clover IAA gene family; B The 10 conserved IAA protein motifs are represented by different colored squares; C The structures of introns and exons are indicated by black lines and green boxes, respectively; D Characterization of cis-acting elements in the promoter region of the TrIAA genes

Fig. 3
Fig. 3 Distribution of the 47 TrIAA genes on 16 chromosomes.Vertical bars indicate chromosome density, and the scale on the left indicates chromosome length

Fig. 4
Fig. 4 Distribution and covariance analysis of IAA in the white clover genome.The red line represents the covariance between TrIAA

Fig. 5 Fig. 6
Fig. 5 Collinearity analysis of IAA genes between white clover, Arabidopsis, red clover, M. truncatula and soybean.Gray lines represent blocks of covariance within the white clover and other plant genomes, and red lines represent covariant IAA gene pairs

Fig. 9
Fig. 9 Overexpression of TrIAA18 increases aluminum, drought, and salt tolerance in yeast and Arabidopsis.A Growth of BY4741 and INSVC1 yeast transformed with TrIAA18-containing pYES2 and the empty vector pYES2.B Yeast two-hybrid assay of TrIAA18 and TrARF5.Transcriptional activity assay of TrIAA18 was measured on selection medium, and then TrIAA18 fused with GAL4-BD and co-transformed with TrARF5 fused with GAL4-AD into AH109 and grown on selection medium.C Root length phenotypes of Wild-Type (WT) and TrIAA18-OE plants under normal conditions (CK), 0.2 mM AlCl 3 , 100 mM D-Mannitol, and 100 mM NaCl treatments.D Total root length of seedlings of WT and TrIAA18-OE plants.The asterisks indicate the significant differences compared with the WT plants (Student's test, * P < 0.05; ** P < 0.01)