Genome-Wide Identiﬁcation and Characterization of the Polyamine Uptake Transporter (Put) Gene Family in Tomatoes and the Role of Put2 in Response to Salt Stress

: The polyamine uptake transporter (Put), an important polyamines-related protein, is involved in plant cell growth, developmental processes, and abiotic stimuli, but no research on the Put family has been carried out in the tomato. Herein, eight tomato Put were identiﬁed and scattered across four chromosomes, which were classiﬁed into three primary groups by phylogenetic analysis. Protein domains and gene structural organization also showed a signiﬁcant degree of similarity, and the Put genes were signiﬁcantly induced by various hormones and polyamines. Tissue-speciﬁc expression analysis indicated that Put genes were expressed in all tissues of the tomato. The majority of Put genes were induced by different abiotic stresses. Furthermore, Put2 transcription was found to be responsive to salt stress, and overexpression of Put2 in yeast conferred salinity tolerance and polyamine uptake. Moreover, overexpression of Put2 in tomatoes promoted salinity tolerance accompanied by a decrease in the Na + /K + ratio, restricting the generation of reactive oxygen and increasing polyamine metabolism and catabolism, antioxidant enzyme activity (SOD, CAT, APX, and POD), and nonenzymatic antioxidant activity (GSH/GSSG and ASA/DHA ratios, GABA, and ﬂavonoid content); loss of function of put2 produced opposite effects. These ﬁndings highlight that Put2 plays a pivotal role in mediating polyamine synthesis and catabolism, and the antioxidant capacity in tomatoes, providing a valuable gene for salinity tolerance in plants.


Introduction
Polyamines, one of the organic polycations, are abundant in various plant organisms and are involved in various cellular processes such as cell growth, nucleic acid stability, and protein synthesis [1,2]. The most abundant polyamines in plant cells, diamine putrescine, triamine spermidine, and tetraamine spermine, are strongly associated with plant responses to biotic and abiotic cues [3,4]. Manipulation of putrescine, spermidine, and spermine by chemical or genetic means is essential for many developmental processes [5,6]. The crucial roles of polyamine synthesis and metabolism in response to numerous stresses have been demonstrated by genetic manipulation [7]. Intracellular polyamine pools are critical for the intermediary part of nitrogen metabolism, and also crosstalk with other metabolic pathways, such as hormones, small molecule signals, and stress-response complexes [8,9].
Besides, increasing evidence indicates that the uptake of polyamine plays essential functions in coordinating the response of plants to a variety of environmental stresses. A salt-sensitive cultivar of rice supplied with putrescine in roots exhibited an increased grain

Plant Material and Treatments
Three-week-old tomato (Solanum lycopersicum L. cv. Ailsa Craig) seedlings were treated with different exogenous polyamines, hormones, and oxidative stress, or abiotic stresses. Briefly, 2.0 mM Put, 1.0 mM Spd, or 2.0 mM Spm were sprayed over the seedlings; for hormone treatments and oxidative stress, 100 µM ABA, 2 mM SA, 100 µM GA 3 , 40% ethylene (ETH), 100 µM paraquat, and water were also sprayed onto the tomato plants, respectively. For RNA extraction, at 0, 30 min, 1, 3, 6, and 12 h, samples of leaves were taken, accordingly. The control was the water treatment at 0 h.
We then investigated Put genes response to different abiotic stresses. Salt and drought stress were initiated by irrigating the plants with 200 mM NaCl or 20% PEG6000 solution, respectively. Tomato seedlings were subjected to 42 • C (high temperature), and 4 • C (low temperature) for heat and cold stress, respectively. After, the treated samples were respectively collected after 0, 30 min, 1, 3, 6, and 12 h; the samples at 0 h were used as the control. In addition, tissues (root, stem, leaf, bud, flower, and fruit) were harvested for investigation of tissue-specific expression. After each treatment, leaves from different plants (three biological replicates) were quickly frozen in liquid nitrogen and kept at −80 • C for further analysis.

Yeast Strain and Culture Conditions
The wild type (WT), G19 (∆ena1-4), failure to mediate Na + uptake; CY162, the K + uptake-deficient, and a yeast strain impaired in spermidine uptake, agp2∆ (strains obtained from open biosystems, http://www.openbiosystems.com/GeneExpression/Yeast/ORF/, accessed on 10 May 2022), were used to describe the potential transporter. The yeasts were grown in YPD media at 28 • C. The yeast cells were converted using lithium acetate. Put1-8 coding sequences were respectively cloned into the pYES2 expression vector.
Wild type-empty vector and agp2∆-Put1-8 transformants were grown in yeast extract peptone galactose (YPG) medium. Cell suspensions were serially diluted as OD 600 of 0.6 for growth tests, and 5 µL aliquots were spotted onto YPG plates containing 25 mM spermidine and 1.5 mM paraquat. After 3-4 days of incubation at 28 • C, the plates were photographed. For polyamine transport assays, the yeast cells were harvested at the midlogarithmic phase, washed with ddH 2 O, and suspended in the YPG media at a dose of 10 8 cells/mL. One-hundred-microliter aliquots cells were transferred to the Eppendorf tubes, and polyamine absorption was activated by the addition of Spermidine or Putrescine at 25 µM concentrations. The absorption was inhibited by adding 1.5 mL of ice-cold uptake buffer with excessive spermidine content at selected times, filtered by a 0.45 µm membrane, and washed with 2 mL ice-cold ddH 2 O (three times) to remove the exogenous polyamines. Polyamine determination in vivo was performed by an Agilent high-performance liquid chromatography 1200 series system (HPLC, Agilent Technologies, Santa Clara, CA, USA). Polyamines were obtained from Sigma-Aldrich (St Louis, MO, USA).
For salt tolerance assays, the final pYES2-empty and pYES2-Put1-8 vectors cultured in G19 and CY162 were performed on SD-U (Synthetic Dextrose Minimal Medium without Uracil) medium, and then diluted until the OD 600 value = 0.6. 5 µL. Aliquots were spotted onto YPG plates containing 100 mM NaCl and 0.1 mM KCl, respectively, and incubated at 28 • C. No treatment was added for the control. After 3-4 days of incubation, the plates were photographed. For Na + and K + uptake treatment, the empty and positive yeast were incubated to OD 600 = 1.0, the supporting was discarded, and 50 mL ddH 2 O was used to wash the yeast. The yeast cells were obtained by centrifugation, followed by starvation treatment with AP liquid medium without K + and Na + . After starvation treatment, the yeast cells were obtained by centrifugation and treated as follows: inoculating the yeast with an AP liquid medium including 200 µM NaCl and 200 µM KCl, respectively. Subsequently, the liquids were put on a 28 • C shaker (220 r/min), and 4 mL of bacterial solution was taken every 10 min, centrifuged, and the supernatant was collected for analysis of Na + and K + contents. Three biological replicates were made. The primers for vector construction are listed in Supplemental data S3 (Table S1).

Plasmid Construction and Plant Transformation
The Put2-overexpression vector (full-length coding sequence of Put2) was constructed as previously described [30]. Gene loss-function of put2 lines was generated through gene editing approaches. To generate the CRISPR/Cas9 vector, the two target sequences for put2 were designed using the online software CRISPR-GE (http://skl.scau.edu.cn/ targetdesign/, accessed on 22 January 2022), which were inserted into two single guide RNA (sgRNA) expression cassettes through overlap PCR, followed by cloning into the pYLCRISPR/Cas9Pubi-H vector via Golden Gate ligation method [31]. The confirmed pFGC1008-Put2-3HA vector and pYLCRISPR/Cas9Pubi-H-put2 binary vector were transformed into Agrobacterium tumefaciens strain GV3101 by electroporation after transgenic plants were generated with Agrobacterium-mediated cotyledon transformation of Solanum lycopersicum cv. Ailsa Craig via a method previously described [32]. Two separate homozygous T2 lines from mutation and overexpression lines were confirmed with Sanger sequencing and qRT-PCR. The put2 mutants and Put2-OE plants were used in this study. The primers for vector construction are listed in Supplemental data S3 (Table S1).

Salt Treatment and Salt Tolerance Assays
The tomato seedlings (WT, put2 mutants, and Put2 overexpression lines) were used for salt tolerance experiments. After seed germination and two cotyledons full expansion, the seedlings were cultured in 250 cm 3 plastic pots filled with a peat-vermiculite combination (2:1, v:v). The seedlings were placed in a greenhouse at 28 ± 2 • C/20 ± 2 • C (day/night) under a maximum photosynthetic photon flux density (PPFD) of approximately 1200 µmol m −2 s −1 and a relative humidity of 70-80%. They were watered daily using Hoagland nutrient solution. Three-week-old WT and transgenic tomatoes of uniform size and health growth status were selected and subjected to salt stress treatment. The seedlings were treated by watering the plants with 200 mL of 200 mM NaCl every other day for salt stress. The control treatment was replaced with an equal amount of water. The salt stress treatment lasted for 7 days, and pictures were captured. The maximum quantum yield of PSII (Fv/Fm) was examined with the Imaging-PAM system (IMAG-MAXI; Heinz Walz, Effeltrich, Germany), as previously described by Zhong et al. [30]. The relative electrolyte leakage (REL%), Na + , and K + analysis was performed as described previously by Zhong et al. [30]. The plants were enclosed in envelopes and placed in an oven at 105 • C for 30 min, and then the oven temperature was adjusted to 75 • C to obtain a permanent dry weight (DW).

Determination of Polyamine Content
The free polyamines content was analyzed by Agilent 1200 High-performance Liquid Chromatography (HPLC, Agilent Technologies, Santa Clara, CA, USA), as previously described in Zhong et al. [33] with slight modifications. Frozen plant tissue (leaves sample, 0.5 mg) was ground with liquid nitrogen, used 10:1 (v/w) of extraction buffer (5% cold aqueous perchloric acid (PCA), w/w). Samples were incubated for 1 h at 4 • C, then centrifuged at 15,000× g for 10 min at 4 • C. Volumes of 200 µL of collected supernatant were mixed with 15 µL benzoyl chloride and incubated for 1 h at 60 • C in darkness conditions. Four milliliters of saturation NaCl solution was used to quench the reaction and diethyl ether was added; 5 mL cold ethyl acetate was then added to extract polyamines. Then, organic layers were evaporated to dryness, redissolved in 100 µL methanol, and filtered with a 0.45 µm pore nylon filter. A volume of 25 µL extraction solution was used to determine the endogenous polyamines levels. The mobile phase was with 64% (v/v) methanol and had a flow rate of 0.8 mL min −1 . Putrescine, spermidine, spermine, and cadaverine (Sigma, St. Louis, MO 63178, USA) were chosen as standard samples and treated similarly.

Determination of PAO Enzymatic Activities and H 2 O 2 Content
Amine oxidase was determined as previously described by Su et al. [34] and Urra et al. [9]. Leaf samples (0.5 g) were ground with liquid nitrogen, homogenized 2:1 (v/w) in 100 mM sodium phosphate buffer (pH 6.5), and centrifuged at 12,000× g for 20 min at 4 • C. One-hundred-microliters of the recovered supernatant was mixed with the 3 mL reaction mix, which contained 2.5 mL sodium phosphate buffer (100 mM, pH 6.5), 200 µL 15 mM 4-aminoantipyrine/0.2% (v/v) N, N-dimethylaniline, 100 µL 250 U ml −1 peroxidase, and 100 µL 20 mM putrescine as a substrate. The CuAO Put , PAO Spm , and PAO Spd were determined using Putrescine, Spermine, and Spermidine as substrates, respectively. A 0.01 value of the changes in absorbance at 555 nm was assayed to one activity unit of the PAO enzyme after being incubated for 30 min at 22 • C. Control samples without polyamines were used to calculate these activities. Leaf H 2 O 2 content was determined by specific detection kits according to the manufacturer's instructions (Nanjing Jiancheng Bioengineering Institute, Jiangsu, China).

Antioxidant Assay
To assess the antioxidant enzyme activity, 0.5 g leaf samples were homogenized with 3 mL ice-cold 50 mM phosphate buffer (pH 7.8), which contained of 2 mM L-ascorbic acid, 2% (w/v) PVPP, and 0.2 mM EDTA. Then, the homogenates were centrifuged for 20 min at 12,000× g, and supernatants were collected to determine the enzyme activity. The activities of SOD, CAT, APX, and POD were assayed as previously described [30]. AsA/DHA and GSH/GSSG were measured as described by Zhong et al. [35]. The GABA content was determined by the Berthelot reaction with some modifications [36]. Leaf samples (0.5 g) were ground with methanol, centrifuged at 6000× g for 15 min, and the supernatant was discarded. The sediment was dissolved in 1.5 mL ddH 2 O and heated in a water bath at 50 • C for 2 h, followed by centrifugation for 15 min at 7000× g. A volume of 1 mL supernatant was mixed with 100 µL 2 mol L −1 AlCl 3 and oscillated, and then centrifuged for 10 min at 12,000× g. The supernatant was added with 300 µL KOH and incubated for 5 min, then centrifuged at 12,000× g for 10 min. The GABA content was measured according to the following procedure: 300 µL supernatant was mixed with the reaction mix, composed of 500 µL 0.1 mol L −1 sodium tetraborate (pH 10.0), 400 µL 6% phenol, and 600 µL 5% sodium hypochlorite. The solution was boiled for 10 min and then placed in an ice bath for 5 min. Finally, the absorbance at 645 nm was measured after shaking the solution with 2 mL 60% ethyl alcohol. The assessment of the total flavonoid concentration was determined by Zhishen et al. [37], with some modifications. Dried leaf samples (0.5 g) were homogenized with 2 mL 80% ethanol, and then added 300 µL 20 mol L −1 NaNO 2 ; 3 mL 1 mol L −1 AlCl 3 was added after 5 min, and after 6 min, 2 mL 1 mol L −1 NaOH was added and mixed well. Finally, the absorbance was measured at 510 nm.

Analysis of Gene Expression
Total RNA was extracted with the RNAsimple Total RNA Kit (Tiangen, DP419) and reverse transcribed with the HiScript TM qRT SuperMix for qPCR (+gDNA wiper) kit (Vazyme, Nanjing, China). The qPCR reaction was performed by the ABI VII7 real-time PCR system (Applied Biosystems, Waltham, MA, USA). Actin was used as the tomato reference gene. The qRT-PCR primers are listed in Supplemental data S3 (Table S2).

Statistics
The data are presented as the means ± SDs and were analyzed using SPSS 20 statistical software. The experimental data were analyzed with Duncan's multiple range test at p < 0.05.

Identification of Tomato Put Family Genes
To analyze Put proteins, a query search against the tomato genome database was accomplished using Arabidopsis and rice Put protein as the control search (Table 1). Eight potential Put proteins with high sequence similarity to AtPut and OsPut were identified and called Put1-8. They had CDs sizes ranging from 1077 bp (Put6) to 1605 bp (Put3), with polypeptides of 359-535 amino acids. The theoretical isoelectric points (pI) of Put varied from 5.41 (Put3) to 9.37 (Put8). The molecular weights (MW) of Put ranged from 40.28 (Put6) to 58.8 (Put3) ( Table 1). Additionally, all Puts were predicted to contain transmembrane domains ( Figure S1). To better study the evolutionary relationships among the tomato Put protein sequences and those of other plants, a phylogenetic tree was performed through the Neighbour-Joining method. By comparing the protein sequences of the Put genes, three main groupings could be distinguished. Two Put genes, Put4 and Put6, were included in Group I; Group II only included Put5, and the remaining five genes (Put1, Put2, Put3, Put7, and Put8) were classified into Group III ( Figure 1A). According to their location, the chromosomal positions of the Put genes were analyzed. Among these Put genes, three (Put4, Put6 and Put7) were mapped to chromosome 1, and three (Put1, Put2 and Put3) were located on chromosome 8, while Put5 and Put8 were located in chromosomes 9 and 10, respectively. These results suggest an uneven distribution of these genes on chromosomes ( Figure 1B).
To better analyze the evolutionary relationships in Put genes, the phylogenetic tree was also constructed. Put1, Put2, and Put3 were observed to have a close evolutionary relationship. A close evolutionary relationship was also found in Put7 and Put8, and Put4 and Put6, respectively. Interestingly, Put5 has a separate evolutionary branch. In addition, their structural domains are highly conserved and contain the polyamine transport protein PotE structural domain ( Figure 1C). The Put family gene structure analysis was carried out to learn more about their intron/exon structures. One intron was present in Put2 and Put5, two in Put3, while the other five (Put1, Put7, Put8, Put4, and Put6) were intron deletion genes ( Figure 1D). To investigate the feasible roles of Put family genes in different abiotic stress and developmental steps, we used the PlantCARE database to estimate the presence of cis-acting elements in the promoter regions of the Put family. We obtained cis-acting elements that are associated with stress, hormone, and light responsiveness. Surprisingly, we only found five typical ethylene responsive motifs (ERE, GCC-box motifs) in the promoter of Put2, but not in that of other Puts ( Figure 1E).

Responsiveness of Put Gene Expression under Hormone, Polyamine, and PQ Treatment
The hormones in the plant kingdom play crucial roles in plant growth and development. Therefore, four different hormone-induced Put transcript-level changes were analyzed. After ABA treatment, the expression of all Puts was induced at 30 min, while that of Put2 and Put5 was induced after 6 h ( Figure 2A). The expression of all Puts was induced at 30 min after SA treatment, which were also upregulated in the later time points, except for Put4 and Put6 (Figure 2A). In contrast, the transcripts of Put6, Put7, and Put8 were reduced initially following GA 3 and ETH treatments, and ETH also reduced the Put4 and Put5 expression, a GA 3 induced both. Put2 and Put3 were reduced after GA 3 treatment, and then induced after 6 h of treatment, Put1 was induced after GA 3 and ETH treatments ( Figure 2A).
To examine the possible roles of Put genes in the tomato, transcripts of Puts after three treatments with polyamines, including Spermidine, Putrescine, and Spermine, were analyzed. Exogenous Spermidine treatment induced all Put genes, and Put2 was the most obvious, followed by Put5 ( Figure 2B). However, the expression of all Put genes was reduced by Putrescine, and the reduction magnitude differed among them. After the seedlings were treated with Spermine, all Put genes were upregulated, but reduced after 12 h treatment. Additionally, exogenous PQ treatment caused upregulation of all Put genes similar to that of Spermidine treatment ( Figure 2B).

Differential Expression of Put Genes during Abiotic Stress
Upon exposure to drought stress, the mRNA transcript of Put1-5 was rapidly induced, and Put2 was the most significant, but other members were reduced ( Figure 2C). Salinity stress resulted in the downregulation of Put3, Put4, Put6, Put7, and Put8, and upregulation of Put1, Put2, and Put5. Cold stress resulted in the most pronounced induction of Put4. Furthermore, when the seedlings were submitted to heat stress, sustained and stable upregulation of Put6 was observed, whereas two genes (Put7 and Put8) were reduced post-treatment ( Figure 2C).
for Put4 and Put6 (Figure 2A). In contrast, the transcripts of Put6, Put7, and Put8 reduced initially following GA3 and ETH treatments, and ETH also reduced the Put4 Put5 expression, a GA3 induced both. Put2 and Put3 were reduced after GA3 treatm and then induced after 6 h of treatment, Put1 was induced after GA3 and ETH treatm ( Figure 2A). To examine the possible roles of Put genes in the tomato, transcripts of Puts three treatments with polyamines, including Spermidine, Putrescine, and Spermine, analyzed. Exogenous Spermidine treatment induced all Put genes, and Put2 was the obvious, followed by Put5 ( Figure 2B). However, the expression of all Put genes wa duced by Putrescine, and the reduction magnitude differed among them. After the lings were treated with Spermine, all Put genes were upregulated, but reduced after treatment. Additionally, exogenous PQ treatment caused upregulation of all Put g similar to that of Spermidine treatment ( Figure 2B).

Differential Expression of Put Genes during Abiotic Stress
Upon exposure to drought stress, the mRNA transcript of Put1-5 was rapidl duced, and Put2 was the most significant, but other members were reduced (Figure Salinity stress resulted in the downregulation of Put3, Put4, Put6, Put7, and Put8, and regulation of Put1, Put2, and Put5. Cold stress resulted in the most pronounced indu (B) Heatmap representation of the responsiveness of Put genes after treatment with Spd, Put, Spm, and PQ. The scale (0 to 3) represents the expression level (from low to high). (C) Heatmap representation of the responsiveness of Put genes after drought, salt, cold, and heat treatment. The scale (0 to 3.5) represents the expression level (from low to high). qRT-PCR was conducted after treatment, according to the methods section. The expression of WT at 0 min in the different treatments was set to 1.

Expression Analysis of Put Genes in Different Tissues
To research the functions of the Put family of genes in the tomato, the expression patterns of Put in various tissues (e.g., root, stem, leaf, bud, flower, and fruit) were performed by qRT-PCR. As shown in Figure 3, the transcripts of Put2 and Put5 had high levels in the leaves and roots, Put3 exhibited high levels of expression in the leaves and flowers, while Put4 showed a high level of transcript expression in the roots and flowers. In addition, all Put, except Put6, Put7 and Put8, were highly expressed in flowers. Subsequently, the spatial expression pattern of Put2 and Put5 was analyzed by qRT-PCR in vegetative tissues of WT plants with salt stress. Put2 and Put5 showed increased expression in organs of plants under salt stress, with the highest level of Put2 transcripts in the leaves, and the highest level of Put5 transcripts in the roots. After 7 days of salt treatment, the Put2 gene is significantly more highly induced than Put5 in the leaves ( Figure 3B,C). flowers, while Put4 showed a high level of transcript expression in the roots and flowers. In addition, all Put, except Put6, Put7 and Put8, were highly expressed in flowers. Subsequently, the spatial expression pattern of Put2 and Put5 was analyzed by qRT-PCR in vegetative tissues of WT plants with salt stress. Put2 and Put5 showed increased expression in organs of plants under salt stress, with the highest level of Put2 transcripts in the leaves, and the highest level of Put5 transcripts in the roots. After 7 days of salt treatment, the Put2 gene is significantly more highly induced than Put5 in the leaves ( Figure 3B,C). were performed by qRT-PCR in different organs of WT plants without NaCl (Control) and salt stress (NaCl) (7 days salt treatment). The WT expression in the control condition was set to 1. The data in B and C are presented as mean values ± SD; n = 3. Different letters indicate significant differences were performed by qRT-PCR in different organs of WT plants without NaCl (Control) and salt stress (NaCl) (7 days salt treatment). The WT expression in the control condition was set to 1. The data in B and C are presented as mean values ± SD; n = 3. Different letters indicate significant differences between treatments (p < 0.05, Duncan's multiple range test). Three independent experiments were performed with similar results.

Functional Analysis of Put Genes in Yeast
To examine the potential function of these proteins in polyamine transport, cDNA fragments containing the ORF were cloned and introduced into the yeast expression vector pYES2, driving expression under the GAL1 promoter. High concentrations of polyamines or paraquat are toxic to wild-type yeast strains, whereas mutant agp2∆ lacking the polyamine uptake transporter protein impairs the sensitivity to the high concentration of polyamines. The candidate positive polyamine transporter was introduced to the yeast mutant agp2∆. The expression of polyamine transporter proteins (Put1, Put3, Put6, and Put7) did not affect the phenotype of the agp2∆ mutant, however, among the eight Put proteins, Put2 and Put5 transformants were more sensitive than other Put transformants under 25 mM Spermidine conditions. The expression of Put2 or Put5 in the agp2∆ mutant conferred sensitivity to 25 mM Spermidine ( Figure 4A). In addition, transformants appeared sensitive to the polyamine's analog PQ, showing that these proteins are also involved in the uptake of PQ.
ines or paraquat are toxic to wild-type yeast strains, whereas mutant agp2Δ lacking the polyamine uptake transporter protein impairs the sensitivity to the high concentration of polyamines. The candidate positive polyamine transporter was introduced to the yeast mutant agp2Δ. The expression of polyamine transporter proteins (Put1, Put3, Put6, and Put7) did not affect the phenotype of the agp2Δ mutant, however, among the eight Put proteins, Put2 and Put5 transformants were more sensitive than other Put transformants under 25 mM Spermidine conditions. The expression of Put2 or Put5 in the agp2Δ mutant conferred sensitivity to 25 mM Spermidine ( Figure 4A). In addition, transformants appeared sensitive to the polyamine's analog PQ, showing that these proteins are also involved in the uptake of PQ.  Further analysis of these genes in light of their competence to transport polyamine was done by incubating with the liquid AP medium supplemented with either 15 µm Spermidine or Putrescine. Transformants of these Put genes improved the ability to trans-port Spermidine or Putrescine than in those of the agp2∆ mutant. These transformants possessed higher uptake of Spermidine or Putrescine relative to that mediated by the agp2∆ mutant. The Put2-and Put5-transformants were effective for Spermidine and Putrescine, respectively. The uptake ability was more pronounced for Put2 than for Put5 ( Figure 4B).
The yeast mutant G19 (∆ena1-4) (does not mediate Na + uptake) and CY162 (K + deficient strain) strain were used to further disclose whether Put could transport Na + or K + . The growth status had a significant difference between G19 transformed with Put2 or Put5 than the G19 empty, Put5 had a better growth status, whilst other Put trans-yeast strains were not significant different to the G19-empty vector under 100 mM NaCl treatment ( Figure 4C). Similarly, under 0.1 mM KCl, CY162 yeast transformed with Put2 or Put5 had a better-growing status compared to the CY162-empty vector, while other Put trans-yeast strains grew similarly to the CY162-empty vector, indicating that Put2 could transport K + , and Put5 could transport Na + and K + ( Figure 4C). Furthermore, the ion depletion assay exhibited that K + ions decreased significantly faster than Na + inoculated into the liquid AP medium with 200 µM NaCl + 200 µM KCl, confirming the role of Put2 in Na + and K + transport ( Figure 4D).

Put2 Is a Positive Regulator Protein of Tomato Plant Salt Tolerance
We focused our present study on Put2, since Put2 was highly expressed in leaves after 7 days of salt stress. Furthermore, Put2 had the highest uptake ability of polyamines among the eight Puts and overexpression of Put2 increased salt tolerance in yeast (Figures 3 and 4). To further determine the role of Put2 in salt stress, as shown in Figure 5, we generated five overexpression lines (named OE#1 to OE#5) and selected two lines (OE#1 and OE#2) for further study after examining Put2 mRNA levels. Meanwhile, two lines of Put2 mutants (put2#1 and put2#2) were generated by CRISPR/Cas9 technology, which induced frameshift mutations. Next, we compared the salt tolerance of these tomato plants. In comparison to WT plants, the Put2-OE#1 and Put2-OE#2 plants exhibited decreased sensitivity to salt stress with less wilted leaves, higher Fv/Fm and dry weight, and lower REL after a salt treatment for 7 days. Whereas put2 mutants displayed salt hypersensitivity with lower Fv/Fm and higher REL than WT. These results suggest that Put2 positively regulates salinity tolerance.
To explore whether Put2 responds to salinity stress through mediating the Na + balance, we further analyzed the Na + and K + contents in WT, put2 mutants, and Put2-OE plants subjected to NaCl treatment. K + and Na + content did not differ significantly among the genotypes examined under normal conditions. However, after treatment with 200 mM NaCl for 7 days, in comparison to WT plants, the levels of Na + in shoots parts of the put2 mutants were much higher, the K + content was significantly lower in mutants, and so the ratios of Na + /K + were increased. Conversely, the contents of Na + and the Na + /K + ratio in the Put2-OE plants were lower, and the levels of K + were higher ( Figure 5H).
The transcription levels of encoding salt response genes such as SOS1-3 and NHX1-3 were examined in the WT, put2 mutants, and Put2-OE plants using qRT-PCR. The mRNA abundance of SOS1-3 and NHX1-3 in the mutants was lower than that in WT. On the contrary, the transcript levels of these genes were significantly increased in Put2-OE plants. These results demonstrated that Put2, as a positive regulator, is mediated by Na + /K + homeostasis ( Figure S2).

Put2 Improves Salt Tolerance by Facilitating Polyamines Synthesis
Previous studies reported that polyamines uptake proteins can facilitate polyamines synthesis, at least in rosette leaves of Arabidopsis thaliana plants (Ahmed et al., 2017), which enlightened us to next investigate the polyamine metabolites. In the polyamine synthesis pathway, key representative molecules (Put, Spd, Spm, and Dap) are derived from the amino acid Arg ( Figure 6A). Significantly, there was a considerable increase in the concentrations of Arg (the Put/Spd/Spm precursor), Spd, and Put in the leaves of Put2-OE plants, but the content in the put2 mutants were lower than those of WT plants in the absence of salt stress. When exposed to the salt treatment, the endogenous content of Arg, Spd, and Put increased significantly in Put2-OE plants than that of WT and put2 mutants, whereas the levels of these polyamines in Put2-OE plants were still considerably higher than those in the WT plants ( Figure 6B-D). Additionally, the Spm and Dap content showed no significant differences among the WT, put2 mutants, and Put2-OE lines ( Figure 6E,F). The transcription levels of encoding salt response genes such as SOS1-3 and NHX1-3 were examined in the WT, put2 mutants, and Put2-OE plants using qRT-PCR. The mRNA abundance of SOS1-3 and NHX1-3 in the mutants was lower than that in WT. On the contrary, the transcript levels of these genes were significantly increased in Put2-OE plants. These results demonstrated that Put2, as a positive regulator, is mediated by Na + /K + homeostasis ( Figure S2).

Put2 Decreases ROS Levels under Salinity Stress
The production of ROS is known to be increased under stress conditions, and H2O2 is the most stable ROS. To determine whether Put2 reduces ROS accumulation through antioxidant enzyme and non-enzymatic compound regulation under salinity stress, the following relevant indicators were detected. During salt stress, the level of H2O2 and In leaves, knockout or gain of function of Put2 did not influence the Put-dependent PAO and Spm-dependent PAO activity in the absence or presence of salt treatment ( Figure 6G,H). By contrast, Put2-OE plants showed an increase in Spd-dependent PAO activity, whereas put2 mutants exhibited a decrease in this activity, relative to WT plants under normal conditions. During salinity stress, there were no significant changes in the activity of Spd-dependent PAO between WT, put2 mutants, and Put2-OE lines ( Figure 6I). Since H 2 O 2 is one of the PAO reaction products, the levels of H 2 O 2 were measured. The leaves of Put2-OE plants showed an evident increase in H 2 O 2 content in the absence of salt stress, whereas the largest rise was shown in put2 mutants in the presence of 200 mM NaCl ( Figure 6J), proving that put2 mutants experience more severe oxidative damage from salt stress than WT and Put2-OE plants. Thus, it is possible that Put2-induced H 2 O 2 production is closely associated with PAOs under normal conditions. On the other hand, Put2 contributes to the decrease of H 2 O 2 content under salt conditions, which declined oxidative damage and enhanced salt tolerance. These results demonstrate that Put2 is required for some polyamines metabolism intermediates (including Arg, Spd, and Put), as well as the enzyme (PAO).

Put2 Decreases ROS Levels under Salinity Stress
The production of ROS is known to be increased under stress conditions, and H 2 O 2 is the most stable ROS. To determine whether Put2 reduces ROS accumulation through antioxidant enzyme and non-enzymatic compound regulation under salinity stress, the following relevant indicators were detected. During salt stress, the level of H 2 O 2 and MDA, two indicators of oxidative damage during salt stress, were significantly lower in Put2-OE plants than in WT; increases in H 2 O 2 and MDA content were detected in put2 mutants ( Figures 6J and 7A). Subsequently, antioxidant enzymes, including SOD, CAT, APX, and POD, are in the midst of the primary enzyme defense against ROS. The activities of SOD, CAT, APX, and POD were more pronounced in Put2-OE than in WT. In contrast, put2 mutants showed lower antioxidant enzyme activity than WT (Figure 7), which is consistent with lower levels of H 2 O 2 and MDA in Put2-OE than in WT and put2 mutants. These results indicate that Put2 improves salinity tolerance by reducing oxidative damage.
To confirm whether the Put2-mediated ROS decrease is regulated by non-enzyme compounds, we determined the effects of glutathione redox homeostasis, GABA, and flavonoid contents in put2 mutants and Put2-OE plants, which however, revealed no difference from the WT under normal conditions, except for GABA. The GABA content in put2 mutants was significantly lower than that of WT and Put2-OE plants before salt treatment. Overexpression of Put2 also considerably elevated the AsA/DHA and GSH/GSSG ratios, as well as the content of GABA and flavonoid, while knockout of put2 compromised the increase in these parameters compared to that in the WT under salinity conditions (Figure 8).

Put2 Triggers Upregulation of Polyamine Synthesis and Is Related to Detoxification Gene Expression
To investigate the transcriptional regulation of polyamine synthesis and detoxification by Put2, we examined the transcript levels of 27 genes involved in polyamine synthesis, ROS detoxification, and GABA synthesis by qRT-PCR in leaves under normal or salinity conditions. qRT-PCR analysis of polyamine synthesis genes in put2#1 mutant and Put2-OE#1 plants revealed that the set genes of encoding polyamine synthesis (including ADC1, ADC2, SPDS1, SPDS2, SPMS1, SPMS2, PAO1, PAO3, and PAO5) were upregulated in Put2-OE#1 plants; in contrast, they were downregulated in put2#1 mutants Furthermore, salinity treatment caused relative increases in the expression of polyamine synthesis genes only in WT and Put2-OE#1 plants (column 3 vs. column 1, and column 5 vs. column 3), while they decreased in put2#1 mutants (column 4 vs. column 3). Collectively, the analysis of differentially expressed genes also suggests that the modifications in gene expression in response to the stress conditions are more intense in the Put2-OE#1 plant. Additionally, we noticed an interesting finding with the greatest upregulation of the PAO5 gene in the five PAOs genes in the Put2-OE#1 plant under normal conditions, which may be a mechanism for the relatively higher PAO activity and levels of H 2 O 2 in Put2 OE plants (Figures 6J and 8).
Put2-OE plants than in WT; increases in H2O2 and MDA content were detected in put2 mutants (Figures 6J and 7A). Subsequently, antioxidant enzymes, including SOD, CAT, APX, and POD, are in the midst of the primary enzyme defense against ROS. The activities of SOD, CAT, APX, and POD were more pronounced in Put2-OE than in WT. In contrast, put2 mutants showed lower antioxidant enzyme activity than WT (Figure 7), which is consistent with lower levels of H2O2 and MDA in Put2-OE than in WT and put2 mutants. These results indicate that Put2 improves salinity tolerance by reducing oxidative damage.  ence from the WT under normal conditions, except for GABA. The GABA content in put2 mutants was significantly lower than that of WT and Put2-OE plants before salt treatment. Overexpression of Put2 also considerably elevated the AsA/DHA and GSH/GSSG ratios, as well as the content of GABA and flavonoid, while knockout of put2 compromised the increase in these parameters compared to that in the WT under salinity conditions ( Figure  8).  Similarly, the transcriptional levels of ROS detoxification-related genes, including Cu/Zn-SOD, MDAR, DHAR, APX, GR, CAT1, POD, and GPX, were further upregulated in the Put2-OE#1 plant compared with WT plants after the salinity treatment. By contrast, the induction of ROS detoxification-related genes in response to salt stress was compromised in put2 mutants; increased ROS-scavenging capacity failed in the put2#1 mutant (Figure 8). In addition, the expression of GAD1, GAD2, and GAD3, encoding glutamate decarboxylase, likely the key enzyme for GABA biosynthesis in the tomato, was induced in the Put2-OE#1 plant before salt treatment. Accordingly, the transcript levels of GADs were further enhanced after salt treatment in the Put2-OE#1 plant. Notably, increases in the expression of GADs in response to salt stress were suppressed in the put2#1 mutant. The enhanced GADs transcripts and GABA content was observed in the WT and Put2-OE plants but not in the put2 mutants after salt stress (Figures 7 and 8). Thus, the results indicate that Put2 participates in enhanced salt tolerance by mediating the ROS-scavenging capacity.

Discussion
Polyamines, which are small polycationic molecular regulators and signaling molecules, not only orchestrate fundamental growth and development in plants, but also induce a series of stress cascades [38]. Polyamines are involved in various pathways in plants and lessen the lethal effects of abiotic stresses by regulating transcription factors, hormonal responses, antioxidant enzymes, and the activation of signaling cascades [39,40]. Polyamine biosynthesis and degradation play important roles in various abiotic stress tolerance pathways and are closely associated with coping with ROS production [41]. The polyamine transporter belongs to the mammalian L-type amino acid transporter family, like polyamine synthesis and metabolism protein, which plays a critical role in plant growth, development, and the stress responses [42]. Though Put has been analyzed in Arabidopsis, rice, and the sweet orange, the effects of Put on abiotic stresses in the tomato have not been reported [43,44]. Here, we looked at the physiological and molecular function mechanisms of Put in the resistance to abiotic stress in the tomato. Eight Put proteins in the tomato were identified and characterized at the complete genome level through alignment with Arabidopsis Put proteins. Then, extensive analyses on the tomato Put proteins, including phylogenetic development, gene and protein structure, physiochemical characteristics, motifs, miRNAs, and cis elements, and their substrates were performed; and the effects of Puts on abiotic stress tolerance was evaluated in yeast and tomatoes. Furthermore, we demonstrated the importance of the Put2 mediation of polyamine metabolism and antioxidant capacity, and that overexpression of Put2 increased polyamines to influence the homeostasis of antioxidant capacity, showing that Put2 was a positive regulator for salinity stress in tomatoes. These findings enlarge the comprehension of Put family members, which may be employed in breeding for genetic modification and the development of abiotic stress tolerant crops.

Identification of Tomato Put Family
The tomato Put proteins were divided into four groups, which have a high similarity to those in rice and Arabidopsis (Figure 1). Differences among these proteins are probably due to environmental impacts, and analysis of the structure and motif in these genes indicated that Put genes disclosed a close exon-intron and motif structure, showing that a closer evolutionary pattern in these genes and diverse functional relationships also exist among the other group members ( Figure 1). Interestingly, protein analysis indicated that the PotE (Putrescine-ornithine antiporter) motif is highly conserved, suggesting that it may be involved in amino acid and polyamine transport ( Figure 1C) [45,46]. A series of cis elements is a specific sequence at the promoter region of a given gene, which is involved in the expression of protein-coding transcripts and is mediated by transcriptional regulation and small RNAs. Repression and activation of gene expression by binding with these cis elements are a general means of modulating various life processes [47]. Plant miRNAs have a function in regulating related genes that are involved in response to abiotic stresses [48]. miR390 was strongly induced after exposure to salinity during lateral root formation in poplar and positively regulated auxin signaling subjected to salt stress [49]. miR6024 negatively mediates the resistance genes and defense system, facilitates disease by the necrotrophic pathogen A. solani, and perturbs immunity in the tomato [50]. The module of miR164a-NAM3 affords cold resistance by increasing ethylene production in the tomato [51]. Tomato Put was targeted by miRNAs including miR390, miR6024, and miR164a, which might be associated with various stress responses ( Table 2). We also discovered several types of conserved cis-regulatory elements in the promoter regions of Put; these cis elements are associated with transcriptional regulation of the core gene network, and of plant growth and development [52]. The Put genes of the tomato contain various cis elements including stress, hormone, light, auxin, GA, ABA, and methyl jasmonate (MeJA) responsive elements ( Figure 1E). The presence of numerous abiotic stress-specific cis-regulatory motifs and hormonal cis elements implicate these genes stimulating the hormone signaling pathways and providing stress tolerance in the tomato [47]. Of note, the cis elements activate their downstream genes after binding to specific transcription factors, playing an important amplifier role during various abiotic/biotic stresses. Meanwhile, we also speculate that Put is involved in salinity stress since these cis-regulatory elements are also closely implicated in salinity tolerance [53].

Expression Profiles of the Put Gene Family after Treatment with Various Hormones, Polyamines, and Abiotic Stresses, in Different Tissues
A gene expression profile can provide critical symbols for its biological functions. Here, we examined the expression pattern of the Put genes via qRT-PCR under treatment with exogenous hormones and polyamines, as well as abiotic stress conditions. We observed the Put genes appeared to be upregulated in ABA treatment. On the other hand, all Put genes, except for Put7, were induced by SA. Put6, Put7, and Put8 were inhibited initially after GA 3 treatment. The expression of five Put (Put4, Put5, Put6, Put7, and Put8) genes were downregulated, and the other Put (Put1, Put2 and Put3) genes were induced in leaves at 3 and 6 h of ET treatment. Similarly, the critical role of growth factors and hormones in increasing polyamine transport rates in mammalian cells has been demonstrated [54]. Together with the presence of hormone-responsive cis elements and altered transcripts levels after hormone treatment, this implies that Put may have a crucial role in the hormone regulatory pathway. Furthermore, the differential expression profiling of Put in response to polyamine treatment was evaluated. All Put genes are involved in exogenous polyamines treatment; the Puts exhibited varied patterns in response to the same polyamine. For instance, Put2 and Put5 were dramatically upregulated, while the other genes were slightly induced after spermidine treatment. However, putrescine resulted in suppression of these Put genes. Additionally, spermine led to the upregulation of Puts, especially Put2 and Put5. On the other hand, the qRT-PCR analysis revealed pronounced effects of the spermidine and spermine-induced Put gene expression ( Figure 2B). Since polyamines are used as substrates required for the polyamine uptake proteins [43], the different polyamine responses may involve the substrate specificity of polyamine transport and homeostasis. In fact, rice Put1 is a specific and high-affinity spermidine uptake transporter involved in polyamines uptake, leading to the accumulation of polyamines in yeast [55]. The lower affinity of Put may be the reason for its higher proportion in the free state. Therefore, spermidine, spermine, and putrescine, may severe as Put substrates. Interestingly, after salt and drought stress, Put2 and Put5 were significantly induced compared with the others. However, their expression was significantly inhibited under cold and heat temperature stress ( Figure 2C). Altogether, these results indicate that Put genes are potentially involved in hormone and polyamine induction, as well as in response to salinity stress.
The Put genes exhibited a divergent expression pattern in different tissues. Put2 and Put5 displayed the highest expression in leaves and roots, and all genes had high expression in flowers and fruit ( Figure 3A). Similarly, the Put family appears to have a distinct tissue expression profile in Arabidopsis and Citrus sinensis [43,44], and a divergent pattern of intracellular localization [13], which implied specialization in a spatial manner. Furthermore, Put2 was more significantly induced by salt stress than Put5 in leaves and roots, indicating that the functional role of Put2 related to salt stress may be important. In the tomato, the functional role of Put2 in abiotic stress tolerance remains largely unknown.

Put2 Contributes to Polyamins Biosynthesis and Catabolism Associated with Salt Tolerance
Although our results above have shown that Put is involved in abiotic stress, its function is yet to be understood, especially regarding polyamine transport and salt stress. Previous studies have shown that yeast is an excellent heterologous expression system to study the function of genes in polyamine transport and salt stress [43]. Here, we used the yeast model to preliminarily investigate their function in polyamine uptake and salt stress tolerance (Figure 4). The results showed that transformants of agp2∆ mutants expressing Put2 and Put5 had higher sensitivity to spermidine and paraquat, indicating that both function as an importer. Here, we also showed that the yeast agp2∆ cells' capacity to transport paraquat may be compensated by Put2 and Put5 ( Figure 4A), since paraquat is transported by the polyamine transport system [12]. A time course absorption experiment directly provided evidence that Put2 and Put5 encoded a transporter that can regulate polyamines import, with high activity of polyamine uptake for Put2 ( Figure 4B). Furthermore, overexpression of Put2 increased salt tolerance in yeast, hampered the influx of Na + , and enhanced K + uptake ( Figure 4C,D). Indeed, polyamine transporters have recently been linked to the regulation of salt stress through promoting Na + efflux and K + channels [56]. Thus, combining the previous results in this article (Figures 2-4), we speculate that the induction of Put2 expression by salt may be regulating the polyamines and Na + /K + homeostasis to alleviate salt damage.
To further validate the function of Put2, the put2 mutants and overexpression lines were generated ( Figure 5A,B). Our results showed that put2 mutants were more shriveled than WT plants under salinity stress, whereas overexpression elevated salt tolerance ( Figure 5C). Likewise, Put2-OE plants displayed increased levels of Fv/Fm and dry weight, and reduced levels of relative electrolyte, which agrees with an increase in salt tolerance and a decrease in Na + content and the Na + /K + ratio ( Figure 5D-H). Similarly, Put3 is critical for Na + and K + homeostasis by physically interacting with SOS1 and SOS2, forming a complex with SOS2 under stress conditions [56]. As such, the induction of SOS1-3 and NHX1-3 in Put2-OE plants could also synergistically activate the SOS1 and SOS2 ( Figure S2). Thus, subsequent increases in the Put2 activity would enhance salt tolerance by activating the Na + /H + exchange activity.
Polyamines, an important regulator in the plant kingdom, are necessary for plant growth, development, and the stress response. The dynamic balance of polyamines in the plant is stringently regulated by polyamine synthesis, degradation, and transport [57,58]. The latter was previously involved in subcellular polyamine transport through the complementation experiment in yeast [55], and the transport of paraquat in Arabidopsis [12]. While the implication of Put2 in polyamine biosynthesis and catabolism was not noted. Here, under control conditions, overexpression of Put2 increases the endogenous Arg, Spd, and Put content, which failed to increase in put2 mutants. Upon salt stress, meanwhile, the polyamine content in WT plants performed much better than put2 mutants, and Put2-OE plants were better than the WT ( Figure 6A-D). NaCl supply treatment also increased the activation of polyamine synthesisrelated genes more clearly in Put2-OE plants (Figure 8), demonstrating the important function of Put2 in the polyamine biosynthesis process. On the other hand, considering polyamine catabolism, the higher activity of PAO spd confirmed the acceleration of polyamine catabolic reactions in Put2-OE plants ( Figure 6I), and evidenced that Put2 positively regulates PAO activity. In addition, two main sources of ROS were indicated to exist in plants, including NADPH oxidases and polyamines catabolism by PAO activity [8,59]. In put2 leaves, H 2 O 2 was lowered with respect to WT plants under normal conditions; however, an upregulation was observed in Put2-OE plants, and likewise PAO activity and PAO gene expression were altered ( Figures 6J and 8), further demonstrating that Put2 attributes to PAO activity. Accordingly, enhancement of PAO activity has been shown to alleviate salinity damage and increase the polyamines and H 2 O 2 content [60,61]. Therefore, Put2 may contribute to governing polyamine biosynthesis and catabolism. However, we cannot completely rule out other possibilities, for example, Put2 may be capable of regulating the long-distance and appropriate tissue distribution of polyamines [62].

Put2-Mediated Antioxidant Capacity Establishes Suitable ROS Levels under Salt Stress
PAO activity has been reported to contribute to an increase in salt tolerance through the production of H 2 O 2 [63]. However, Put2-OE plants treated with NaCl showed that the increase in H 2 O 2 content was lower than in WT plants. Furthermore, the H 2 O 2 content increased considerably in put2 mutants accompanied by serious salt stress injury, which correlated inversely with the activities of PAO ( Figure 6J). Thus, PAO-induced H 2 O 2 production was stunted under salt conditions in Put2-OE plants; therefore, another mechanism to eliminate H 2 O 2 must exist. Indeed, plants exposed to salt stress generate a super-excess of ROS, which is highly toxic and can overwhelm the PAO-induced H 2 O 2 , ultimately damaging cellular activity and leading to plant death [8]. In the current study, Put2-OE plants exhibited obviously increased activities of antioxidant enzymes after salt treatment. Additionally, the ASA-GSH cycle was also activated by overexpression of Put2, which could be another exploration for Put2 enhanced salt tolerance, as the enzymatic system and scavenging procedure could be activated in Put2-OE plants (Figures 7 and 8). These findings indicate that Put2 functions as an important regulator linking polyamines and ROS, and affects both the production and elimination of ROS. The results coincided with a previous study showing that Put2 promoted phyA-mediated germination by sensing seed oxidation and protecting the decaying seed from oxidative damage [64]. Therefore, there is strong evidence that Put2 increased salt tolerance probably by promoting antioxidants in plants. A similar report has been conducted showing that CsPUT4 can protect against cold stress by modulating polyamine homeostasis and turning on the antioxidant enzyme defense system in the sweet orange [44]. Meanwhile, GABA and flavonoids, as free radical scavengers, have been exhibited to alleviate salinity damage and heat damage by inducing polyamine enhancement [65,66], which are increased in Put2-OE plants under salinity stress; this further demonstrates positive feedback regulation by Put2.

Conclusions
In this work, eight Put family proteins were found in the tomato, and their chromosomal location, structure, phylogenetic tree, and physiochemical properties were investigated. Furthermore, molecular characterization was performed in yeast to understand their involvement in polyamine uptake and salt stress tolerance. Additionally, the cis elements in the promoter, miRNAs targeting Put, and the expression profiles of Put genes in different tissues and their responses to exogenous hormones and polyamines, as well as abiotic stress, were analyzed, proving they may play a vital function in abiotic stress, growth, and development. Furthermore, we show the role of Put2, which, to our knowledge, is the first polyamine uptake protein characterized in the tomato shown to play a role in salinity tolerance. Firstly, in yeast, Put2 was highly tolerant to salt stress, as indicated by less Na + invasion and K + efflux, which also could be attributable to an enhancement in the absorption of polyamines. Importantly, overexpression of Put2 in the tomato decreased salinity sensitivity, evidenced by enhanced polyamine biosynthesis and catabolism and maintained Na + /K + homeostasis, in addition to activated ROS-scavenging enzyme activities and nonenzymatic antioxidant process. These findings shed light on Put2-regulated salinity tolerance in the tomato. Here, we provide comprehensive deciphering of the mechanisms of Put2 for enhancing salt tolerance and some valuable evidence for interpreting the potential functions of tomato Put genes in abiotic stress tolerance.
Clearly, further studies are required to understand the precise function of Put and the upstream and downstream targets of the individual Puts. Generating loss-and gainof-function mutations and characterizing their roles will provide useful tools, generating new evidence and new findings.
Supplementary Materials: The following supporting information can be downloaded at: https: //www.mdpi.com/article/10.3390/antiox12020228/s1, Figure S1. Cartoon of the predicted topology of tomato Put proteins. Transmembrane domains are indicated as blue rectangle. Figure S2. Relative transcript levels of SOS1, SOS2 and SOS3 (A), NHX1, NHX2 and NHX3 (B) gene expression in WT, put2 mutants, or Put2 OE lines after exposure with or without salt stress for 7 days. Data are presented as mean values ± SD; n = 3. Different letters indicate significant differences between treatments (p < 0.05, Duncan's multiple range test). At least three independent experiments were performed. Figure S3. The MDA content in WT, put2 mutants, or Put2 OE lines after exposure with or without salt stress for 7 days. Data are presented as mean values ± SD; n = 3. Different letters indicate significant differences between treatments (p < 0.05, Duncan's multiple range test). At least three independent experiments were performed. Supplemental data S1. The protein sequences of Put in Arabidopsis, rice and tomato, respectively. Supplemental data S2. The Put genes Cis-element distribution. Supplemental data S3. Primers used in this study.