Identification of WRKY gene family members in amaranth based on a transcriptome database and functional analysis of AtrWRKY42-2 in betalain metabolism

Introduction WRKY TFs (WRKY transcription factors) contribute to the synthesis of secondary metabolites in plants. Betalains are natural pigments that do not coexist with anthocyanins within the same plant. Amaranthus tricolor (‘Suxian No.1’) is an important leaf vegetable rich in betalains. However, the WRKY family members in amaranth and their roles in betalain synthesis and metabolism are still unclear. Methods To elucidate the molecular characteristics of the amaranth WRKY gene family and its role in betalain synthesis, WRKY gene family members were screened and identified using amaranth transcriptome data, and their physicochemical properties, conserved domains, phylogenetic relationships, and conserved motifs were analyzed using bioinformatics methods. Results In total, 72 WRKY family members were identified from the amaranth transcriptome. Three WRKY genes involved in betalain synthesis were screened in the phylogenetic analysis of WRKY TFs. RT-qPCR showed that the expression levels of these three genes in red amaranth ‘Suxian No.1’ were higher than those in green amaranth ‘Suxian No.2’ and also showed that the expression level of AtrWRKY42 gene short-spliced transcript AtrWRKY42-2 in Amaranth ‘Suxian No.1’ was higher than that of the complete sequence AtrWRKY42-1, so the short-spliced transcript AtrWRKY42-2 was mainly expressed in ‘Suxian No.2’ amaranth. Moreover, the total expression levels of AtrWRKY42-1 and AtrWRKY42-2 were down-regulated after GA3 treatment, so AtrWRKY42-2 was identified as a candidate gene. Therefore, the short splice variant AtrWRKY42-2 cDNA sequence, gDNA sequence, and promoter sequence of AtrWRKY42 were cloned, and the PRI 101-AN-AtrWRKY42-2-EGFP vector was constructed to evaluate subcellular localization, revealing that AtrWRKY42-2 is located in the nucleus. The overexpression vector pRI 101-AN-AtrWRKY42-2-EGFP and VIGS (virus-induced gene silencing) vector pTRV2-AtrWRKY42-2 were transferred into leaves of ‘Suxian No.1’ by an Agrobacterium-mediated method. The results showed that AtrWRKY42-2 overexpression could promote the expression of AtrCYP76AD1 and increase betalain synthesis. A yeast one-hybrid assay demonstrated that AtrWRKY42-2 could bind to the AtrCYP76AD1 promoter to regulate betalain synthesis. Discussion This study lays a foundation for further exploring the function of AtrWRKY42-2 in betalain metabolism.


Introduction
Amaranth (Amaranthus tricolor L.) is an annual plant with beneficial health effects.It is cultivated in many countries.It is native to India (Parveen et al., 2018) and distributed in southern Asia (Wang et al., 2019), Central Asia, Japan, and other places.Amaranth is rich in betalains, characteristic pigments in Amaranthaceae (Chang et al., 2021), and betalain structure in the species differs from that of betalain in beet.Amaranth is an important resource for betalain extraction and research (Zheng et al., 2016).
We have identified genes involved in betalain metabolism in amaranth, such as AtrCYP76AD1, AtrDODA, AtrDOPA5-GT, AtrB5-GT, and AtrB6-GT, by transcriptomics analyses (Zheng et al., 2016).However, the specific WRKY TFs in amaranth involved in betalain synthesis and the underlying regulatory mechanisms have not been determined.In this study, we identified WRKY TFs and demonstrated that AtrWRKY42-2 interacts with the promoter of AtrCYP76AD1, thereby regulating the betalain synthesis in amaranth.These findings provide new insight into betalain synthesis.1).The leaves (functional leaves) of 'Suxian No.1' from potted seedlings at about one month were used for transient transformation and virus-induced gene silencing (VIGS).All samples were frozen in liquid nitrogen immediately and stored at −80°C for further analyses.Briefly, 1 mg/L GA 3 and 2 mg/L paclobutrazol (PP 333 ) were added into MS medium supplemented with sucrose (30 g/L) and agar (7 g/L) (Pan et al., 2018;Zhao et al., 2019;Xiao et al., 2021).The sterilized seeds of 'Suxian No.1' and 'Suxian No.2' were inoculated in the medium.Medium without hormones was used as a control.Each treatment was evaluated with 15 bottles and three biological replicates.After 7 days of culture, the hypocotyl at the amaranth seedling stage was collected.

Analyses of conserved motifs and conserved domains of WRKY proteins
Conserved motifs of AtrWRKY proteins were identified using MEME (Multiple Expectation Maximization for Motif Elicitation) [http://meme-suite.org/tools/meme(accessed on October 29, 2022)].

RT-qPCR analyses
Total RNA was isolated from samples using MolPure Plant Plus RNA Kit (Yeasen, China) according to the manufacturer's instructions.First-strand cDNA was synthesized from 1 mg of total RNA using Recombinant M-MLV reverse transcriptase (TransGen Biotech, Beijing, China).Quantitative real time-PCR (qRT-PCR) was performed in optical 96-well plates using the Roche LightCycler 480 instrument (Roche, Sweden).The reactions were carried out in a 20 mL volume containing 10 mL of SYBR Premix Ex Taq, 0.8 mL of genespecific primers, 2 mL f diluted cDNA, and 6.4 mL of ddH 2 O.The PCR conditions were as follows: 30 s at 95°C, 45 cycles of 10 s at 95°C and 20 s at 59°C, followed by 12 s at 72°C.Three biological repeats were performed for each material.SAND (Xiao et al., 2021) was used as the internal reference gene.Excel 2016 was used for data analyses, SPSS 20 was used to evaluate the homogeneity of variances, and the 2 −DDCt method was used for quantitative analyses of gene expression.The primer pairs used for the qRT-PCR analysis of WRKY genes are listed in Supplementary Table S1.

Subcellular localization of AtrWRKY42-2
The full-length coding sequence of AtrWRKY42-2 was inserted into the pRI 101-AN-EGFP vector (primers are listed in Supplementary Table S1).Agrobacterium strain GV3101 cells carrying pRI 101-AN-AtrWRKY42-2-EGFP and pRI101-AN-EGFP were infiltrated into onion inner epidermis cells.Transient expression of EGFP was recorded using a laser confocal microscope (Olympus model: FV1200 4 laser) at 405 nm.Onion epidermis cells were stained with DAPI to evaluate nuclear localization, and the fluorescence signal was visualized by laser confocal microscopy at 473 nm.

Functional analysis of AtrWRKY42-2
pRI 101-AN-AtrWRKY42-2-EGFP and pRI 101-AN-EGFP were transformed into the Agrobacterium tumefaciens strain GV3101.The bacterial cells were resuspended to an OD600 of 0.8-1.0 using MMA buffer (10 mM MES, 10 mM MgCl 2 , 100 mM acetosyringone) at a 1:1 ratio.Subsequently, bacterial cells were infiltrated into amaranth leaves.Then these seedlings were cultured in the dark at 25°C for 1-2 days.These seedlings were then transferred to a culture room set to 16 h/8 h (light/dark) and 25°C.Plant phenotypes were observed.The transiently transformed plants were cultured for 1 week (including dark treatment for 2 days), and the 7th to 8th true leaves were collected to detect gene expression levels and determine the betalain content.
The gene fragment with the AtrWRKY42-2 conserved domain was cloned into the pTRV2 vector.pTRV1, pTRV2, and pTRV2-AtrWRKY42-2 were transformed into Agrobacterium tumefaciens strain GV3101.The bacterial cells were resuspended to an OD600 of 0.6~0.8 using an MMA buffer.pTRV2 (negative control) and pTRV2-AtrWRKY42-2 were separately infiltrated into amaranth leaves with pTRV1 in a ratio of 1:1.The culture conditions were the same as those described above.The leaves were collected for the detection of gene expression level and the determination of betalain contents.

Measurement of betalain contents
Betalain contents were determined as described by Hua et al. (Hua et al., 2016) The absorption peaks of betacyanin and betaxanthin at 538 nm and 465 nm were determined by ultraviolet-visible spectrum spectrophotometer (UV-900, Shanghai Yuan Analysis Instrument Co., Ltd.).The betacyanin and betaxanthin contents were calculated according to a molar extinction coefficient of betaxanthin of 5.66 × 10 4 .All determinations were performed in triplicate.

Yeast one-hybrid assay of AtrWRKY42-2 and the AtrCYP76AD1 promoter
The promoter of AtrCYP76AD1 (see Supplementary Text S2 for the sequence) was ligated to the pHis II yeast reporter vector to form a pPromoter-pHis II recombinant bait vector.AtrWRKY42-2 was ligated into the expression vector pGADT7 to construct the pGADT7-AD recombinant vector and the pGADT7-AtrWRKY42-2 vector plasmid was used to transform the positively verified AtrCYP76AD1-pHis II (primers are listed in Supplementary Table S1).The bait yeast strain Y187 was cultured at 30°C for 3 days.Two deficient media, SD/-Leu-Trp and SD/-Leu-Trp-His-Ade, were used to detect the interaction between AtrWRKY42-2 and the AtrCYP76AD1 promoter based on yeast growth.

Identification and physical parameters of WRKY gene family members in amaranth
A total of 72 putative WRKY genes were screened by a systematic analysis of the transcriptome of A. tricolor.These WRKY genes were termed AtrWRKY1 to AtrWRKY72.The fulllength CDS of the AtrWRKY genes ranged from 818 bp (AtrWRKY12 and AtrWRKY31) to 5459 bp (AtrWRKY15) with deduced proteins of 178-1093 amino acids.Furthermore, the computed molecular weights of these WRKY proteins ranged from 19517.74 to 124261.7 Da.The theoretical pI of the deduced AtrWRKY proteins ranged from 5.11 to 9.96.The detailed sequences and annotation are listed in Supplementary Table S3.

Conserved motifs and domains of AtrWRKYs
A total of 15 conserved motifs were detected from AtrWRKYs using the MEME tool.Each motif contained 15-50 amino acids, and each sequence included 2-12 motifs.Motifs 1 and 3 formed the main structure of the WRKY domain (WRKYGQK), and Motifs 2, 10, and 13 contained a zinc-finger motif.The most frequent motifs of AtrWRKYs were Motif 1, Motif 5, and Motif 2, which showed high amino acid sequence conservation and represent the AtrWRKY domain (Figure 2).AtrWRKY6, AtrWRKY72, AtrWRKY10, and AtrWRKY43 all had Motif 14.However, Motif 9 was only identified in AtrWRKY63.

Phylogenetic analysis and structural classification of WRKY genes in A. tricolor
At the amino acid sequence level, the family motifs were well conserved (Figures 3A, B).To evaluate the evolutionary history of the WRKY gene family in A. tricolor and to uncover their classification and function in betalain synthesis, 72 WRKY proteins from A. tricolor, Beta vulgaris (betalain), and 'Guan Huahong'pitaya (betalain) were used to construct a phylogenetic tree using the NJ method implemented in MEGA11.Among the selected AtrWRKY7, AtrWRKY40, and AtrWRKY42-2 proteins, WRKY homologs in the same group/subgroup as those in sugar beet and pitaya may have similar functions.AtrWRKY7 and AtrWRKY40 were homologous to AtWRKY25 and HmoWRKY40, respectively.In particular, AtrWRKY42-2 was homologous to HpWRKY44, AtWRKY44, and BvWRKY44.We predicted that AtrWRKY7, AtrWRKY40, and AtrWRKY42-2 might be involved in betalain synthesis (Figure 3C).
An un-rooted phylogenetic tree was constructed based on the alignments of the WRKY motif and zinc-finger motif from amaranth using the NJ method (Figures 2, 3C).The AtrWRKYs were divided into four groups (Groups I-IV).Group I contained two WRKY domains and C 2 H 2 type zinc finger protein domains, including 19 AtrWRKYs.Group II contained one WRKY domain and C 2 H 2 type zinc finger protein domain, including 48 AtrWRKYs.Group III only contained one zinc finger motif of type C 2 HC and one protein domain (Huang et al., 2012;Wang et al., 2014), including four AtrWRKYs (AtrWRKY65, AtrWRKY38, AtrWRKY58, and AtrWRKY26).AtrWRKY43 belonged to Group IV, which contained one WRKY domain and an incomplete C 2 H 2 type zinc finger protein domain (Eulgem et al., 2000).

Sequence comparison of transcript
AtrWRKY42-1 and AtrWRKY42-2 As shown in Figure 4, the complete transcript sequence was named AtrWRKY42-1 (CL2645.Contig1_All), and short splice transcript was one of the transcripts of the AtrWRKY42 gene, named AtrWRKY42-2 (CL2645.Contig2_All).AtrWRKY42-2 had only one conserved domain, which was one fewer domain than the complete protein-coding gene, and it could be confirmed as a member of Group II according to the WRKY classification criteria.
A sequence alignment of WRKY44 homologues in beet, pitaya, and Arabidopsis (see Supplementary Text S4 for sequence details) showed that the other four proteins were clearly different from the AtWRKY44 protein motif (Figure 4).We further analyzed the AtrWRKY42-2 conserved domains.WRKY proteins involved in betalain synthesis from pitaya, B. vulgaris, Arabidopsis, and amaranth revealed that AtrWRKY42-2 had the same domain and zinc finger structure as those of the WRKY44 cluster.Except for AtWRKY44, the other three genes had special amino acid sequence fragments (Figure 4).

Expression patterns under treatment with plant growth regulators
To further identify betalain-related WRKY genes from A. tricolor, the expression patterns of AtrWRKY7\40\42 genes in the leaves of 'Suxian No.1' and 'Suxian No.2' were determined by RNA-seq.We have previously found that GA 3 , 2,4-D, and 6-BA promote the growth of amaranth, the accumulation of betacene in amaranth is inhibited by GA 3 and 2,4-D, and PP 333 promotes the synthesis of betacene (Liu et al., 2018;Pan et al., 2018).Therefore, we determined the expression patterns of AtrWRKY7\40\42 genes under treatment with 1 mg/L GA 3 and 2 mg/L paclobutrazol to verify the expression of the putative WRKY TFs.As shown in Figure 4, the expression levels of AtrWRKY7\40\42 were altered in the 'Suxian No.1' leaves.In particular, AtrWRKY40 was upregulated under GA 3 treatment, AtrWRKY42-2 was downregulated, and AtrWRKY7 expression did not differ between treatment and control groups.AtrWRKY40 was upregulated under paclobutrazol treatment, AtrWRKY7 was downregulated, and AtrWRKY42 was upregulated (Figure 5).Based on these results, we selected AtrWRKY42 as a candidate gene for further analyses.However, the total expression levels of AtrWRKY42-1 and AtrWRKY42-2 in 'Suxian No.1' and'Suxian No.2' were always higher than the expression levels of AtrWRKY42-1, so the short splicing transcript AtrWRKY42-2 expressed mainly in the plants of the two varieties.
A 1891 bp promoter region (see Supplementary Text S2 for the sequence) was successfully amplified.In this region, a transcription start site (TSS), a TATA-box 1000 bp upstream of the TSS (Figure 6C), and a large number of other cis-acting elements (Supplementary Table S5) were predicted based on a PlantCARE database analysis.

Subcellular localization of AtrWRKY42-2
The full-length CDS of AtrWRKY42-2 was fused with the EGFP gene to analyze its subcellular localization.Ater the transient expression of constructs in the inner epidermis of onion, green fluorescence of AtrWRKY42-2 was detected exclusively in the nuclei (as evaluated by 4',6-diamidino-2-phenylindole (DAPI) staining); however, in the positive control, the EGFP signal was observed around the cytoplasm, cell membrane, and nuclei (Figure 7).

Overexpression of AtrWRKY42-2 in amaranth
As shown in Figure 8A, when compared with expression in the control and empty plasmid group, the overexpression of AtrWRKY42-2 was visualized as dark red in the scales of 'Suxian No.1' amaranth.There were no significant differences in the betaxanthin content among transgenic plants, blank control group, and positive control group.However, the betacyanin content in transgenic plants was significantly higher (P < 0.05) than that in the control (Figure 8B).Results from the RT-qPCR analyses showed that AtrWRKY42-2, CYP76AD1, TyDC, MYB1, B5-GT, and B6-GT (Download ID and primer sequences are shown in Supplementary Table S1), key genes involved in betalain metabolism, were upregulated in plants overexpressing AtrWRKY42-2 (Figure 8C).These findings were consistent with the leaf phenotype and betacyanin content.

VIGS analysis of AtrWRKY42-2
The silencing of AtrWRKY42-2 resulted in new green leaves (although not completely green) after 2-3 weeks of transformation (Figure 9A).There was no significant difference in the betaxanthin content between plants with gene silencing and the control; however, the betacyanin content in leaves was significantly lower in plants with gene silencing than in the control (Figure 9B).The RT-qPCR analysis showed that the expression levels of key genes in betalain synthesis were significantly decreased by gene silencing (Figure 9C).These results indicate that AtrWRKY42-2 plays an important role in the betacyanin biosynthetic pathway of amaranth, and silencing AtrWRKY42-2 inhibited the synthesis of betacyanin.sequence).A typical W-box motif was identified in the AtrCYP76AD1 promoter, which is a cognate binding site for WRKY TFs, suggesting that WRKY TFs are involved in the regulation of AtrCYP76AD1.Therefore, the interaction between AtrWRKY42-2 and the promoter of AtrCYP76AD1 was evaluated using a yeast one-hybrid assay.Yeast cells carrying only pHis II-AtrCYP76AD1-Pro could not grow on SD/-Leu-Trp-His-Ade medium (Figure 10).Yeast cells containing pHis II-AtrCYP76AD1-Pro+pGADT7-AtrWRKY42-2 were grown on SD/-Leu-Trp-His-Ade medium (Figure 10).These results suggest that AtrWRKY42-2 binds directly to the promoter of AtrCYP76AD1 and may be involved in the biosynthesis of amaranth betalains.

Discussion
The WRKY TFs are a universal gene family in higher plants, controlling plant growth and development under normal and stress conditions (Jiang et al., 2017;Gangola and Ramadoss, 2020;Li et al., 2020;Jia et al., 2022).However, WRKY gene family members in A. tricolor have not been identified and characterized.We screened 72 AtrWRKY genes from the A. tricolor transcriptome database, which was more than 70 genes reported in pitaya (Chen et al., 2022) and 2 genes in Beta vulgaris (Wu et al., 2019).AtrWRKYs were divided into four subfamilies according to their domain and zinc finger structure, consistent with the previous classification of WRKY TFs (Eulgem et al., 2000;Huang et al., 2012;Wang et al., 2014).
Betalains are a unique lineage in anthocyanin evolution (Alfonso et al., 2019;Li et al., 2019).However, they cannot coexist within the same plant.Betalains have only been detected in Caryophyllales species, with the exception of Caryophyllaceae and Molluginaceae species, as well as some higher fungi.The WRKY TFs has important roles in higher plants, including roles in plant growth and development and secondary metabolite synthesis under the normal and stress conditions (Peng et al., 2019;Hu et al., 2021;Chen et al., 2022).Recent studies have also shown that WRKY TFs are involved in betalain metabolism in pitaya (Gangola and Ramadoss, 2020;Hu et al., 2021;Chen et al., 2022).In pitaya, HmoWRKY40 and HpWRKY44 promote the synthesis of betalains (Cheng et al., 2017;Zhang et al., 2021), while HmoWRKY42 inhibits the synthesis of betalains (Chen et al., 2022).A phylogenetic analysis revealed that AtrWRKY42-2 was homologous to HmoWRKY44 and BvWRKY44.However, the amino acid sequences of BvWRKY44, AtrWRKY42-2, and HpWRKY44 in betalain-producing differed from AtWRKY44 in Arabidopsis (Figure 3C).Some studies have found that AtWRKY44 only regulates the biosynthesis of phenylpropyl and indole alkaloids (Johnson et al., 2002;Mao et al., 2011), no one studied the role of AtWRKY44 in betalain synthesis, so we speculated that amino acid substitutions are involved in the regulation of betalain synthesis.Therefore, we speculated that the amino acid substitutions are involved in the regulation of betalain synthesis.Further studies are needed to verify whether the transfer of AtWRKY44 into A. thaliana mediated by A. tumefaciens regulates anthocyanin synthesis and increases the anthocyanin content, similar to the other three WRKY homologues.
Betalain accumulation could make the amaranth leaves red ( Barba-Espin et al., 2018;Fan et al., 2020), which is determined by environmental conditions and transcription factors (Erika et al., 2018;Preczenhak et al., 2019;Guerrero-Rubio et al., 2020;Sakuta et al., 2021;Sokolova et al., 2022).Our previous studies have indicated that various environmental factors and hormones (GA 3 and 2,4-D) influence betalain biosynthesis (Xiao et al., 2021).The predicted cis-acting elements of AtrWRKY42-2 contain TC-rich repeats, STREs, and so on based on a PlantCARE database analysis (Supplementary Table S5).Therefore, we speculated that these factors affect betalain synthesis via WRKY TFs.We found that the function of AtrWRKY42-2 in amaranth is similar to those of HpWRKY44 and HmoWRKY40 in pitaya (Cheng et al., 2017;Zhang et al., 2021), and all of these loci promote the accumulation of betalains.When the WRKY domain and zinc finger structure of AtrWRKY42-2 were silenced by VIGS technology, betacyanin synthesis was inhibited.In contrast, betacyanin accumulation in amaranth was promoted by AtrWRKY42-2 overexpression.In analyses of the relative expression of AtrWRKY42-2 and key genes involved in betalain synthesis, we observed that the gene expression levels were associated with the betacyanin content.
These results indicated that AtrWRKY42-2 promotes betacyanin synthesis.However, there was no difference in the betaxanthin content between transgenic plant and the control.These results content showed that AtrWRKY42-2 was not involved in betaxanthin synthesis.Perhaps it was synthesis by other CYP76AD members and transcription factors.Previous studies have shown that the synthesis of betacyanin mainly depends on the action of CYP76AD1 to synthesize cyclo-DOPA, and maintaining the ratio of CYP76AD1 and CYP76ADb (CYP76AD5, 6, 15) can regulate the synthesis ratio of betacyanin and betaxanthin.(Sunnadeniya et al., 2016).However, the regulation of AtrWRKY42-2 in this study only led to the differential expression of key genes involved in the synthesis of betacyanin such as CYP76AD1, and it did not affect the expression of CYP76ADb subfamily members (CYP76AD5, 6, 15) to exercise hydroxylation.Further functional studies of AtrWRKY7 and AtrWRKY40 are in progress.
WRKY TFs recognize and bind to the TTGAC(C/T) W-box in the promoter regions of target genes (Chen et al., 2019).WRKY TFs can bind not only upstream promoters (Brand et al., 2013;Madhunita and Ralf, 2014) but also to upstream promoters of other genes regulated by WRKY TFs (Cheng et al., 2017;Li et al., 2020;Zhang et al., 2021;Chen et al., 2022;Zheng et al., 2022).The AtrWRKY42-2 promoter sequence contained six W-box elements that specifically bind WRKY TFs.These results indicated that AtrWRKY42-2 binds to itself or other WRKY TFs.In addition, the AtrCYP76AD1 promoter sequence contains a W-box element of WRKY TFs.AtrWRKY42-2 could activate AtrCYP76AD1, a key gene involved in betalain synthesis, by binding to its promoter responsible for betalain biosynthesis in amaranth.HpWRKY44 and HmoWRKY40 could activate HmoCYP76AD1 expression by binding to its promoter responsible for betalain biosynthesis of pitaya (Cheng et al., 2017;Zhang et al., 2021).A yeast one-hybrid assay showed that AtrWRKY42-2 interacts with the AtrCYP76AD1 AtrWRKY42-2 and AtrCYP76AD1 promoter yeast one-hybrid assay.The experiment was repeated independently three times.SD/-Leu-Trp and SD/-Leu-Trp-His-Ade indicate yeast single defect medium.
promoter (Figure 10), providing evidence that AtrWRKY42-2 activates the transcription of AtrCYP76AD1, involved in amaranth betalain biosynthesis (Figure 11).AtrWRKY42-2 transcript factor could regulate downstream gene transcription by binding W-box elements of target gene AtrCYP76AD1 promoter, and then participate in betalain synthesis.The expression level of the key genes in the betalain synthesis pathway was up-regulated or down-regulated in accordance with overexpression or silencing expression of .

Conclusions
In summary, WRKY family members were screened using HMM in the amaranth transcriptome.A total of 72 WRKY family members were obtained, and these were divided into four groups according to the domain and zinc finger structure.These WRKY TFs were located in the nuclei, with the exception of AtrWRKY50.There were no significant differences in the expression levels of AtrWRKY7\40\42 in the leaves of 'Suxian No.1', which may be explained by the complex factors involved in gene expression regulation, such that changes in any single factor do not cause substantial changes in expression.The expression level of AtrWRKY42-2 in 'Suamaranth 1' was significantly higher than that of AtrWRKY42-1.A transient overexpression experiment and VIGS assay showed that AtrWRKY42-2 promoted betalain synthesis.A yeast one-hybrid assay demonstrated that AtrWRKY42-2 could bind to the AtrCYP76AD1 promoter to regulate betalain synthesis.

FIGURE 2
FIGURE 2 Analysis of conserved motifs and conserved domains of AtrWRKYs.Motif1-15 represents the conserved sequence of AtrWRKYs members.WRKY and WRKY superfamily represent the conservative domain of AtrWRKYs members.LRR superfamily; NB-ARC superfamily represents the LRR and NB-ARC domains; Plant_zn_clust represent plant zinc cluster.(AtrWRKYs:Amaranth WRKY transcription factor family).
FIGURE 3 Conserved amino acid sequence analysis and WRKY phylogenetic tree analysis.(A) Comparison of the conserved domain (WRKY-a) of AtrWRKY family members; (B) Comparison of the WRKY-b conserved domain (The higher the bit value in the log map of the domain, the more conserved the corresponding amino acid; WRKY-a: upstream domain of the gene sequence; WRKY-b: downstream domain of gene sequence); (C) WRKY phylogenetic tree (Red circle represents amaranth, blue triangle represents pitaya, and yellow star represents sugar beet.The green circle represents the WRKY members classified in group IV).
features Complementary DNA and genomic DNA of AtrWRKY42-2 were cloned from both 'Suxian No.1' and 'Suxian No.2'.There was no difference in the cDNA sequence of AtrWRKY42-2 between

FIGURE 7
FIGURE 7 Subcellular localization of pRI 101-AN and AtrWRKY42-2 proteins in onion.Red arrows indicate the location of EGFP and DAPI fluorescence signals in cells.Bars=100mm.
FIGURE 9 Silencing of AtrWRKY42-2 inhibits betalain production.(A) Positive control plants (left) and VIGS transgenic positive plants (right) Phenotype.(B) Betalain content in leaves of positive control plants and VIGS transgenic plants.(C) Relative expression levels of key genes related to betalain synthesis in transgenic plants with gene silencing.Three biological replicates were performed for each sample (a, b and c indicate significant differences at p < 0.01; Bar = 1 cm).

FIGURE 10
FIGURE 10 Seeds of 'Suxian No.1' and 'Suxian No.2' were provided by Suzhou Academy of Agricultural Sciences.'Suxian No.1' was dark red and rich in betalains.'Suxian No.2' was light green and did not contain betalains (Figure