Upstream Open Reading Frame Mediated Translation of WNK8 Is Required for ABA Response in Arabidopsis

With no lysine (K) (WNK) kinases comprise a family of serine/threonine kinases belonging to an evolutionary branch of the eukaryotic kinome. These special kinases contain a unique active site and are found in a wide range of eukaryotes. The model plant Arabidopsis has been reported to have 11 WNK members, of which WNK8 functions as a negative regulator of abscisic acid (ABA) signaling. Here, we found that the expression of WNK8 is post-transcriptionally regulated through an upstream open reading frame (uORF) found in its 5′ untranslated region (5′-UTR). This uORF has been predicted to encode a conserved peptide named CPuORF58 in both monocotyledons and dicotyledons. The analysis of the published ribosome footprinting studies and the study of the frameshift CPuORF58 peptide with altered repression capability suggested that this uORF causes ribosome stalling. Plants transformed with the native WNK8 promoter driving WNK8 expression were comparable with wild-type plants, whereas the plants transformed with a similar construct with mutated CPuORF58 start codon were less sensitive to ABA. In addition, WNK8 and its downstream target RACK1 were found to synergistically coordinate ABA signaling rather than antagonistically modulating glucose response and flowering in plants. Collectively, these results suggest that the WNK8 expression must be tightly regulated to fulfill the demands of ABA response in plants.


Introduction
Protein kinases comprise a superfamily of enzymes that regulate a wide range of cellular processes through induced phosphorylation of downstream protein substrates in all living cells. WITH NO LYSINE (WNK) kinases belong to a superfamily of serine/threonine protein kinases uniquely characterized by the lack of a catalytic lysine residue in the kinase subdomain II, which is crucial for coordinating ATP and catalyzing phosphoryl transfers within other protein kinase superfamily and downstream targets [1].
WNK kinases have been identified in various eukaryotes. They were first discovered in mammals while screening for new members of the mitogen-activated protein, serine/threonine kinase (MAPK) family. Humans have four different WNK kinases, namely WNK1, WNK2, WNK3, and WNK4 [2]. Studies have reported four WNK members in mice, two in Xenopus, and a single WNK homolog member in Drosophila melanogaster, Caenorhabditis elegans, and Giardia lambia [3][4][5]. In animals, WNK kinases play critical roles in ion homeostasis by regulating numerous ion channels, including sodium chloride cotransporter (NCC) and sodium potassium chloride cotransporter (NKCC1), as well as in angiogenesis, tumor cell growth, and neuropathic disorders [6][7][8][9][10][11][12]. In plants, the WNK gene family is larger and more diverse than in animals. A total of 11 and 9 WNK members have been identified in the model plant Arabidopsis and Oryza sativa, respectively [13,14].
The plant hormone abscisic acid (ABA) is known to play important roles in development and stress responses. Some WNK family members have been found to be involved in ABA-signaling pathway. WNK8 and WNK9 from Arabidopsis have been shown to regulate salt and osmotic stress responses through an ABA-dependent pathway [23,24]. Studies have shown that AtWNK8 expression is enhanced under salt and sorbitol treatments and that the wnk8 mutant lines have higher proline content and exhibit significant catalase (CAT) and peroxidase (POD) activities, which lead to in high salinity and osmotic stress tolerance [23]. Furthermore, AtWNK8 has been proposed to negatively modulate ABA signaling by interacting with ABA-signaling core components, including the ABA receptor, PYR1, and type 2C protein phosphatase (PP2CA) [28]. In contrast, AtWNK9 positively regulates ABA signaling and enhances drought tolerance in transgenic plants [24]. Os-WNK9, a member of rice WNK gene family, has been functionally well characterized, and its overexpression in Arabidopsis has been shown to confer high tolerance to drought and salt stress in an ABA-dependent manner [25]. Moreover, a previous study showed that the soybean GmWNK1 gene reduces sensitivity to both ABA and mannitol treatment with increased endogenous ABA in Arabidopsis [15]. Furthermore, this study showed that GmWNK1 directly interacted with a crucial ABA catabolism enzyme, GmCYP707A1. Collectively, these findings revealed the diverse roles of plant WNKs in ABA response and the relevance of their interaction with ABA in both signaling pathways and ABA metabolic processes. However, many questions regarding the regulation of WNK kinases and their comprehensive interaction with ABA components remain to be explored.
In the present study, we investigated Arabidopsis WNK8 found that two individual T-DNA insertion lines of WNK8 showed similar ABA response phenotypes. However, no significant transcript regulation of WNK8 was observed under ABA treatment compared to the control. Further studies showed that a conserved peptide encoded by an upstream open reading frame (uORF), called uORF58, has been identified in the 5 -UTR of WNK8. We showed that the translation of WNK8 was repressed by CPuORF58 in vivo and that this element may act by a ribosome stalling mechanism, independently of the main open reading frame (mORF) downstream of the uORF. Moreover, we showed that such an ingenious regulation is necessary for plants to fulfill the demands of ABA response caused by the uncontrolled expression of WNK8. Finally, we found that WNK8 coordinates ABA signaling with RACK1, a downstream target of WNK8.

WNK8 Negatively Regulates ABA Response in Seed Germination and Post-germination Development
A previous study showed that different T-DNA insertion mutants of WNK8 led to opposite ABA responses during seed germination [28]. To learn more about the roles of WNK8 in response to ABA, two T-DNA insertion mutants, SALK_206987C (wnk8-1) and SALK_103318C (wnk8-2), were used in this study ( Figure 1A). The T-DNA insertions were confirmed to be present in the fourth exon of the WNK8 gene by genotyping and sequencing ( Figure 1B). An RT-PCR analysis using region-specific primers detected no WNK8 transcript in either allele ( Figure 1B).
We further carried out a seed germination assay for each genotype following ABA treatment. The germination rates of the different genotypes were similar in the absence of ABA. In the presence of 1.5 µM ABA, both wnk8-1 and wnk8-2 seeds showed higher ABA sensitivity with much lower germination rates than the wild-type seeds ( Figure 1C). In addition, the wnk8-1 and wnk8-2 mutants showed significantly lower cotyledon greening rates after germination in the medium with ABA for 7 days ( Figure 1D). Taken together, these results suggest that WNK8 negatively regulates the ABA response during seed germination and post-germination development.

WNK8 Has a Conserved Open Reading Frame in Its 5 -UTR
To study the expression pattern of WNK8 in the presence of ABA, we quantified WNK8 mRNA accumulation under high ABA concentration (50 µM) and found only slightly increase ofWNK8 mRNA levels ( Figure S1). This indicated that the regulatory mechanism of WNK8 at high ABA concentrations is unlikely to be involved in transcription.
To learn more about the expression of WNK8, transcription and translation were further investigated using the ATHENA database (http://athena.proteomics.wzw.tum.de accessed on 16 August 2021), a collection of many protein and transcript expression profiles from Arabidopsis thaliana (Col-0) plants [29]. The ATHENA search analysis showed that similar transcription levels of WNK8 in different organs or tissues, except for higher transcriptional expression in pollen ( Figure S2A). Consistent with the data from ATHENA, the qRT-PCR results confirmed higher expression levels of WNK8 in open flowers and mature pollens ( Figure S2B). In contrast, the translation levels of WNK8 varied greatly among the organs or tissues, in which it was almost undetectable, such as in cotyledons (CT), hypocotyl (HY), rosette leaf (LFs), and carpel (CP). This suggests a post-transcriptional regulation mechanism for WNK8.
The presence of an encoded peptide in the 5 -UTR of WNK8 upstream of its mORF has been previously reported [30]. We further analyzed the published ribosome profiling data for the distribution of ribosomes along the WNK8 sequence [31][32][33]. The data clearly indicated that the uORF had a high frequency of ribosome occupancy, with an average higher ribosome density compared to that of the mORF (Figure 2A). We further performed an in silico analysis of WNK8 homologs within representative plant species to determine the functionality of such a peptide. The basic local alignment search tool BLASTP retrieved 12 nucleotide sequences encoding WNK8 homologs from both monocots and dicots, using the WNK8 protein sequence as the query. These homologous sequences were further analyzed for the presence of ORFs, and this analysis led to the identification of 12 uORFs ( Figure 2B). Further alignment of these sequences showed a certain degree of conservation in both monocots and dicots ( Figure 2C). More peptide conservation was observed in monocots than in dicots (Figures 2D,E and S3).

CPuORF58 Is Essential for the Translational Suppression of the WNK8
5 -UTRs play a significant role in translational regulation [33]. We presumed that the CPuORF58 peptide located in the 5 -UTR could play a translational regulatory role in controlling the expression of WNK8. To address this hypothesis, we generated mutations to replace the start codon (ATG) of CPuORF58 with AAG. Two different genetic constructs were generated with the expression of the GUS reporter gene controlled by the WNK8 promoter including its 5 -UTR with the native (pWNK8:GUS) or mutated CPuORF58 (pWNK8m:GUS). These constructs were transformed into Col-0 Arabidopsis plants. Several independent lines were generated for both constructs, and homozygous lines were established. Subsequently, the lines showing similar GUS transcript levels were selected ( Figure S4) and assayed histochemically for GUS expression in the same tissues (cotyledons, rosette leaves, inflorescence, and anthers). The results showed that weak GUS expression was detected in the plants transformed with pWNK8:GUS, whereas a strong GUS color was detected in all selected tissues and organs of the plants transformed with pWNK8m:GUS (in which CPuORF58 was mutated) ( Figure 3A). The ribosome profiling data presented some peak distributions in the CPuORF58 peptide of WNK8, indicating ribosome stalling ( Figure 2A). A previous study showed that the nascent peptides encoded by uORFs cause ribosomal arrest during mRNA translation [34]. Therefore, we decided to examine the importance of the CPuORF58 sequence followed by the generation of several genetic constructs with the truncated or frameshift uORF. A schematic representation of these constructs presented in Figure 3B. In 35S:FS1-uORF58:GFP and 35S:FS2-uORF58:GFP, the C-terminus of uORF58 was truncated and shifted, respectively. In 35S:FS3-uORF58:GFP, the nucleotide sequence of uORF58 exhibited little change, whereas the deduced amino acid sequence was completely changed. These constructs were transformed into Col-0 Arabidopsis plants and homozygous lines were established. Stable transgenic lines with these constructs showing similar GFP transcript levels were selected ( Figure 3C). The GFP expression was analyzed by 'immunoblotting. The results showed that both truncated and frameshift mutations in uORF58 led to increased GFP levels, suggesting the involvement of uORF58 in translational suppression of WNK8 ( Figure 3D).

Two Independent Regions in the 5 -UTR of WNK8 Are Required for Gene Expression
A further analysis showed that the 5 -UTR of WNK8 contains two short open reading frames (here named uORF1 and CPuORF58) ( Figure 4A). Regarding the presence of the two uORFs, we constructed a list of site-mutated WNK8 5 -UTR to evaluate responsible role of these regions in gene expression regulation ( Figure 4B). The GUS expression driven by 35S CaMV promoter was applied as the control. The wild-type (UTR WT ) and site-mutated of WNK8 5 -UTR were inserted between the 35S promoter and the GUS reporter gene. All constructs were introduced into GV3101, and a transient expression assay of GUS expression was performed within tobacco leaves, and followed by GUS histochemistry. The result showed that GUS expression under 35S promoter was strong in control. In contrast, the wild-type of WNK8 5 -UTR (UTR WT ) significantly repressed GUS expression ( Figure 4C). The individual site-mutated of WNK8 5 -UTR was also able to repress GUS expression driven but less effect in compared with the wild-type 5 -UTR, similar to the inhibition seen from the CPuORF58 in transgenic Arabidopsis plants. Unexpectedly, the extent of repression in GUS expression was not enhanced in the double site-mutated UTR m1+m2 of WNK8 5 -UTR.

The Absence of a Strictly Regulated Expression of WNK8 Altered ABA Sensitivity
Two different genetic constructs were generated to study the role of CPuORF58 in vivo. In the first construct, WNK8 expression was controlled by a 2.3-kb region upstream of the start codon, including its 5 -UTR (pWNK8:WNK8), and in the second construct, a point mutation (G→C) was introduced in the start codon ATG of CPuORF58 (pWNK8m:WNK8). In both constructs, the Myc tag was directly attached to the mORF of WNK8. These constructs were used to transform wnk8-1 mutant plants. As stated above, independent transgenic lines were generated for these constructs, after which homozygous lines were established. The WNK8 protein was rarely detected in plants transformed with pWNK8:WNK8, which was used as the complementation material hereafter ( Figure 5A). This was similar to the weak expression of GUS driven, by the WNK8 promoter. In contrast, strong WNK8 expression was detected in plants transformed with pWNK8m:WNK8 ( Figure 5B). These lines were further selected to evaluate the role of WNK8 in the ABA response. As expected, the complementation of WNK8 in wnk8-1 (Comp) showed a phenotype similar to that of the wild-type phenotype. However, plants transformed with pWNK8m:WNK8 exhibited much lower sensitivity to ABA ( Figure 5C). We further investigated the expression patterns of the ABA response genes RD29B and COR47 in these genetic backgrounds. Under normal conditions, the expression levels of the two ABA response genes were similar in all selected plants, but slightly lower in plants transformed with pWNK8m:WNK8 ( Figure 5D,E). After ABA treatment, the transcription levels of both RD29B and COR47 were significantly increased, with the highest in the wnk8 mutant. The expression of the two ABA response genes was also induced in plants transformed with pWNK8m:WNK8 but was lower than their expression in Col-0 and wnk8 mutant plants. This suggested that WNK8 negatively affected the expression of ABA response genes, which is consistent with a previous study [28].

WNK8 and RACK1 Coordinate ABA Signaling
Receptor for activated C kinase1 (RACK1) has been suggested to act downstream of WNK8 to regulate flowering and glucose responsiveness as well as to play a negative role in ABA signaling [17,35]. Hence, we examined whether WNK8 and RACK1 function together in coordinating ABA signaling. Seed germination analysis showed that both wnk8-1 and rack1a-2 were more sensitive to ABA than Col-0 plants ( Figure 6A). This was different from the opposing flowering and glucose phenotypes of rack1a-2 and wnk8-1 single mutants [17]. Interestingly, the double mutant rack1a-2 wnk8-1 was even more sensitive to ABA in seed germination than the single mutant. This suggests that WNK8 and RACK1 function in the same pathway to regulate the ABA response. WNK8-mediated phosphorylation negatively affects the stability of the RACK1 protein [17]. Thus, we examined the expression of RACK1 in different genetic backgrounds related to WNK8. The results showed that transcription of RACK1A was constant in Col-0, wnk8-1 mutant, and plants transformed with pWNK8m:WNK8 ( Figure 6B). The protein levels of RACK1A were also similar in Col-0 and wnk8-1 mutant plants ( Figure 6C). However, the accumulation of RACK1A was higher in plants with high WNK8 expression. This indicated the occurrence of other kinds of posttranslational modifications that may contribute to the stability of the RACK1A protein and counteract the effect of WNK8-mediated phosphorylation.

Discussion
Plants have developed diverse environmental adaptation strategies for their development and survival. In general, they adapt to alterations in environmental conditions by controlling their gene expression profiles through both transcriptional regulation and post-transcriptional regulation. It is widely known that different regulatory elements are present in the 5 -UTR of mRNAs. uORFs appear in the 5 -UTR as translational control elements, which generally attenuate the translation of the downstream mORF in most cases [36][37][38][39]. uORFs have been found in approximately 20% to 50% of eukaryotic transcripts. Approximately 50% of protein-encoding genes possess one or more uORFs in humans [39]. In plants, 24-30% of the 5 -UTR of mRNAs contains uORFs; however, only a few uORFs have been identified and characterized [40,41]. Therefore, it is necessary to further explore uORFs in plants and investigate their translational control mechanisms, which could provide a deeper understanding of plant development and adaptations to changing environments.
uORFs have been identified in many transcripts responsible for plant development, including transcription factors (TFs) and RNA processing factors [42]. In particular, genes encoding TFs are over-represented. Several studies have demonstrated that uORFs play important roles in the translational regulation of many pathways in plants including metabolic, plant morphogenesis, disease resistance, and nutrient absorption pathways [43][44][45][46][47]. For instance, several enzymes, such as S-adenosylmethionine decarboxylase (AdoMetDC) and flavin-containing polyamine oxidases (PAO), are controlled by uORFs in a small metabolite-dependent manner, which are important for the biosynthesis of polyamine (PA) and phosphocholine (PCho), respectively [48][49][50][51][52]. Some proteins are tightly regulated by uORFs, though other signals including light and plant hormones. Both Arabidopsis TFs AtHB1 (HOMEOBOX 1) and PHYTOCHROME-INTERACTING FACTOR 3 (AtPIF3) are light-dependent and regulated by uORFs [53][54][55]. One uORF in the 5 -UTR of the Brassinosteroid receptor protein AtBRI1 (Brassinosteroid insensitive 1) has been to be essential for the stability of BR (Brassinosteroid) levels in vivo [56]. Here, we demonstrated that CPuORF58, a highly conserved genetic element in the 5 -UTR of WNK8, is important for ABA-signaling response in plants. Our results showed that the protein level of WNK8 is closely related to the ABA response in Arabidopsis. The two T-DNA insertion lines wnk8-1 and wnk8-2, which lacked WNK8 transcripts, were more ABA-sensitive (Figure 1). In contrast, high expressed WNK8 expression conferred significantly less ABA sensitivity when CPuORF58 was mutated in plants ( Figure 5). Thus, WNK8 expression must be tightly regulated to fulfill the demands of ABA signaling in plants.
Although uORFs are distributed in a considerable number of mRNAs, only a small number of these regulatory elements are conserved between species. Here, we showed that in all retrieved DNA sequences encoding WNK8 homologs from both monocot and dicot species that contain known 5 -UTRs, and CPuORF58 was predicted ( Figure 2B). Although the conservation of the total amino acids is not very high due to the unusual longer size (ranging from 55 aa-84 aa), it is important to note that higher conservation in some specific amino acids is species-specific ( Figure 3C-E). Clear coverage peaks upstream of the uORF stop codon for the 5 -UTR of WNK8 were observed with ribosome footprinting analyses, indicating ribosome stalling in this region (Figure 2A). Here, we demonstrated the role of CPuORF58 in translational repression in vivo, which is most likely due to ribosome stalling. With frameshift mutations, the repressive activity of CPuORF58 was lost in plants, although little change was observed in the RNA sequence ( Figure 3B-D). In addition, another uORF (uORF1) was identified in the 5 -UTR of WNK8 overlapping with CPuORF58 ( Figure 4A). The transient expression assay showed that either of the two uORFs was effective in triggering the translation repression of the downstream mORF, while the extent of the reduction was stronger with CPuORF58. As uORF1 partially overlapped with CPuORF58, the translated uORF1 prevented the translation of CPuORF58. Thus, the extent of suppression of reporter expression was not enhanced when both uORFs were mutated, but when they acted as mimics of the mutated uORF1 ( Figure 4B-D). This indicates that at least two post-transcriptional regulatory mechanisms contribute to tight control of the WNK8 accumulation in vivo.
RACK1A has been suggested to act downstream of WNK8 and play a negative role in ABA responses [17,35]. Here, we found that the double mutant rack1a-2 wnk8-1 was more sensitive to ABA than either of the single mutants ( Figure 6A). This indicated that WNK8 and RACK1A coordinate the ABA-signaling pathway differently from the glucose response pathway and flowering. The enhanced ABA activity in the wnk8 mutant may lead to the repression of the RACK1 expression of, as ABA treatment resulted in rapid downregulation of RACK1 [35]. However, no significant change in the transcription of RACK1A was detected in either the control or wnk8 mutant plants ( Figure 6B). A similar expression of RACK1A was also found in plants with high WNK8 expression. It has been suggested that WNK8 affects the protein stability of RACK1 by phosphorylation modification [17]. However, no difference in RACK1A protein abundance was observed in either wnk8 mutant or the wild-type plants, which is consistent with the results of a previous study. Instead, more RACK1A proteins were detected under high WNK8 expression. It is possible that the dominant effect of certain modifications contributes to stable RACK1A expression, even under high WNK8 expression. ABA represses RACK1 at the transcriptional level, but also enhances the sumoylation of RACK1, which increases the stability of RACK1 in vivo [57]. As the ABA core receptor, PYR1 could be phosphorylated by WNK8 at several residues close to the ABA-binding site and may affect the ABA-affinity, leading to more ABA accumulation in cells [28]. It has also been suggested that WNK proteins are helpful in maintaining ABA homeostasis. GmWNK1 interacts with the putative ABA 8 -hydroxylase protein GmCYP707A1, and enhanced levels of endogenous ABA were observed in transgenic lines [22]. We suspected an accumulation of ABA when WNK8 proteins were highly expressed, therefore enhancing the protein stability of RACK1A. It remains to be investigated whether RACK1 sumoylation increases with increase in WNK8 expression. Moreover, it would be interesting to examine the ABA levels in these genetic lines in future studies.

Plant Materials and Growth Conditions
All plants used for transformation in this study are with the Arabidopsis ecotype Columbia-0 (Col-0). The mutants wnk8-1 (SALK_206987C) and wnk8-2 (SALK_103318C) in the Col-0 ecotype background, were supported by the Arabidopsis Biological Resource Center (http://www.arabidopsis.org accessed on 16 August 2021). The mutant rack1a-2 (SALK_073786C) was the gift from Jiafu Jiang in Nanjing Agricultural University. Seeds were surfaced sterilized and grown in Murashige and Skoog (MS) medium with 1% sucrose and 0.8% phyto agar. Plates were kept for 3 days at 4 • C in the dark before moved to a culture room with 22 • C under a long-day (16/8 h light/dark) photoperiod. Seven-day-old seedlings were grown in the culture room with same conditions as previously stated. The wnk8-1 was crossed with rack1a-2 for generation of the double mutant wnk8-1 rack1a-2.
For the seed germination assay, seeds were surfaced sterilized and placed on the half strength MS medium in the absence or presence of various concentrations of ABA, and transferred to the culture room. The seed germination was calculated after stratification, and cotyledon expansion and greening were scored at the indicated time intervals.

RNA/DNA Extraction and Analysis
For genotyping of the T-DNA insertion mutants, leaves from two-week-old seedlings were harvested for DNA extraction. Edwards buffer (20 mM Tris-HCl (pH 7.5), 250 mM NaCl, 25 mM EDTA, and 0.5% SDS) was applied for quick one-step DNA extraction following the protocol. The genotyping PCR using gene-specific primers and a T-DNA primer LBa1 for mutant lines were performed using PCR mix (Vazyme, Nanjing, China). The insertion site was confirmed by DNA sequencing.
For quantitative reverse transcription-PCR (qRT-PCR), the total RNA was extracted from the Arabidopsis seedlings or different organs and tissues using ReliaPrep™ RNA Miniprep System (Promega, Madison, WI, USA). For cDNA synthesis, the first-strand cDNA was synthesized using 2 µg total RNA with NovoScript ® Plus All-in-one 1st Strand cDNA Synthesis SuperMix (Novoprotein, Shanghai, China) following the instructions. The qRT-PCR was carried out with SYBR Green Master Mix (YEASEN, Shanghai, China) on Step-one Plus TM (Applied Biosystems, Carlsbad, CA, USA). The 2 −∆∆CT method was applied to quantify the gene expression levels [58]. Actin2 was used as an internal control. All primers used are listed in Table S1.

pWNK8:GUS and pWNK8m:GUS
The native version of the WNK8 promoter (2.3 kb upstream of WNK8 translation start site) was amplified and the mutated version was assembled by overlapping PCR amplification using specific oligonucleotides (Supplemental Table S1). The PCR products were cloned into the HindIII and NcoI sites of pCAMBIA1301, replacing the 35S CaMV. The correct insertion was verified by sequencing.

pWNK8:WNK8 and pWNK8m:WNK8
To generate the plasmid for the native expression of WNK8, the genomic region including 2.3 kb upstream of ATG plus introns and exons were cloned with nuclear sequence (GAGCAGAAACTCATCTCTGAAGAGGATCTG) for Myc tag (EQKLISEEDL) included in the reverse primer. The mutated version of the WNK8 was assembled overlapping PCR. Both PCR products were cloned into pDONOR221 using Gateway™ BP Clonase™ Enzyme Mix (Thermo Scientific, Waltham, MA, USA), and further cloned into the pGWB4 plant expression vector using Gateway™ LR Clonase™ II Enzyme mix (Thermo Scientific, Waltham, MA, USA). The WNK8 5 -UTR was amplified, and the indicated mutations were introduced by overlapping using specific oligonucleotides. All the PCR products were introduced into pDONOR221 using Gateway™ BP Clonase™ Enzyme Mix, and further cloned into the pGWB405 to produce C-terminal GFP-tagged fusion proteins under the control of the 35S promoter using Gateway™ LR Clonase™ II Enzyme mix. All the constructs were confirmed by sequencing.
For plasmids construction, all genes were amplified using Tks Gflex™ DNA polymerase (Takara, Shiga, Japan) with corresponding primers listed in Table S1. The plant expression constructs were introduced into the Agrobacterium tumefaciens GV3101 strain. Plant transformation was applied with the floral dipping method [59]. Further selection of transformed plants was performed in petri dishes with MS medium supplemented with the appropriate selector chemical (50 mg L −1 kanamycin or 25 mg L −1 hygromycin). Three or four homozygous T3 and T4 independent lines for each construct were further reproduced and used to analyze the gene expression levels and phenotypes.

Histochemical GUS Staining and GUS Activity Measurement
GUS staining was performed with commercial kit by following the protocol (Coolaber, Beijing, China). In brief, young seedlings, mature leaves, and flowers were immersed into fresh prepared GUS staining buffer, further with vacuum for 5 min, and then plants were kept at 37 • C for 24 h. Chlorophyll was removed from the plant tissues with 70% ethanol.
To examine the GUS activity, a plant-GUS ELISA kit was applied following the protocol (Abmart, Shanghai, China). The fresh plant tissue samples were grinded with 0.75% NaCl solution. After centrifuge for 10 min with 3000 rpm, the supernatant was collected and further incubated with reagents provided in kit. The OD values from the standard and test samples were measured with a wavelength of 450 nm. The GUS activity in each sample can be normalized per unit tissue weight.

Immunoblotting
Seedlings of stable transgenic lines expressed the corresponding GFP or Myc fusions were freeze grounded into powder and homogenized in total protein buffer (20 mmo1/L Tris-HCl (pH 7.5), 150 mmol/L NaCl, 2 mmol/L EDTA) with protease inhibitor cocktail in DMSO (YEASEN, Shanghai, China). Lysates were incubated on ice for 20 min and clarified by centrifugation at 15,000 g for 15 min at 4 • C. For immunoblotting, samples were separated on 12% SDS polyacrylamide gel and transferred to PVDF membranes. The membranes were then blocked with 5% (g/v) defatted milk in TBST buffer (10 mM Tris-HCl (pH 7.4), 150 mM NaCl, 0.05% Tween 20) and probed with using appropriate antibodies including 1:6000 dilution α-GFP conjugated with HRP (MBL, Nagano, Japan), 1:5000 dilution of α-RACK1 (PhytoAB, SAN JOSE, CA, USA), α-Myc (MBL, Nagano, Japan) and α-Actin2 (Sangon, Shanghai, China) overnight at 4 • C. Then the samples were washed with TBST buffer for three times and visualized using the ECL (Amersham™, Boston, MA, USA). Actin protein was used as the internal control. Image J2 was applied for quantification the intensity of signals [60].

Database Screening Analysis
The BLASTP program was applied for a search for Arabidopsis WNK proteins on the whole genome sequences from the Phytozome database (https://phytozome.jgi.doe.gov accessed on 16 August 2021), with AtWNK8 as the query sequence. Corresponding genomic DNA (gDNA) and coding DNA (cDNA) sequences of the WNK8s from the selected plant genome were retrieved. The uORF nucleotides and predicted amino acid sequences were aligned using the ClustalW software (version 2.0.12) [61]. The sequence logos were generated with MEME (https://meme-suite.org/meme/tools/meme accessed on 16 August 2021) with default setting. The GWIPS-viz (https://gwips.ucc.ie/ accessed on 16 August 2021) was applied to visualize the RNA-seq and ribosome profiling data of WNK8. The data exploration tool ATHENA (http://athena.proteomics.wzw.tum.de: 5002/master_arabidopsisshiny/ accessed on 16 August 2021) was used for comparing the proteome and transcriptome data of WNK8.

Conclusions
In this study, we found that tArabidopsis WNK8 is post-transcriptionally regulated by the conserved peptide (CPuORF58) located in its 5 untranslated region (5 -UTR). Together with another uORF, CPuORF58 represses WNK8 expression to fulfill the demands of ABA response in plants. Moreover, WNK8 and its downstream target RACK1 synergistically coordinate ABA signaling rather than antagonistically modulating plant glucose response and flowering. This study provides a better understanding of the role of uORFs in plant development and adaptation to changing environments.