Morphophysiological and Comparative Metabolic Profiling of Purslane Genotypes (Portulaca oleracea L.) under Salt Stress

Purslane, a fleshy herbaceous plant, plays a pivotal role in various preventive and therapeutic purposes. To date, no report has documented the consequence of salt stress on metabolite accumulation in purslane. Herein, we proposed an insight into the metabolic and physiological traits of purslane under saline stress environments. The gas chromatography-mass spectrometry analysis was used to scrutinize the metabolic profiling of leaves and roots of two purslane genotypes, Tall Green (TG) and Shandong Wild (SD), under the control and saline exposures. Results revealed that the morphological and physiological traits of leaves and roots of both the tested Portulaca oleracea cultivars in response to salt stress (100 mM and 200 mM) were dramatically changed. Similarly, significant differences were found in the metabolite profiles among samples under salinity stress treatments as compared with the control. Thorough metabolic pathway analysis, 132 different metabolites in response to 28 days of particular salt stress treatments were recognized and quantified in roots and leaves of purslane, including 35 organic acids, 26 amino acids, 20 sugars, 14 sugar alcohols, 20 amines, 13 lipids and sterols, and 4 other acids. In conclusion, this study can be useful for future molecular experiments as a reference to select gene expression levels for the functional characterization of purslane.


Introduction
The World Health Organization (WHO) documented purslane (Portulaca oleracea) as one of the most important C 4 medicinal plants, and it was named as "Global Panacea" [1], owing to the presence of immense omega-3 fatty acids and antioxidant vitamins [2]. Purslane can be consumed as a vegetable and play a pivotal role in various preventive and therapeutic purposes particularly in maintaining a healthy immune system and avoiding cardiovascular diseases [3]. Salinity is one of the most vital ecological tasks, which limits plant yield, mostly in the arid and semiarid climates [4]. Salinity in soils and irrigation water is one of the leading abiotic limitations facing agriculture worldwide. An estimated 800 million hectares of agriculture lands are affected globally by salinity [5]. A soil is considered to be saline when the electric conductivity (EC) of the soil solution reaches 4 dS m −1 (equivalent to 40 mM NaCl), generating an osmotic pressure of about 0.2 MPa that substantially reduces the crop yield. In addition, salt stress causes necrosis and chlorosis due to the accumulation of Na + that impedes many physiological developments in plants [6].
In plants, most of the salinity adaptation mechanisms involve certain physiological and morphological parameters; the genotypes that cannot grow in high salinity stress are known as glycophytes. On the contrary, halophytes are plants that are able to survive at a high level of NaCl (300-500 mM) due to the development of salt tolerance mechanisms [7]. It is also well recognized that the salt-tolerant genotypes demonstrate increased or unchanged chlorophyll under the salty environments, but chlorophyll contents are decreased in salt-sensitive genotypes [8,9]. At salt stress conditions, the carotenoid contents are converted from violaxanthin to zeaxanthin by the action of the violaxanthin deepoxidase enzyme [10]. The first most important organ in plants under salt stress conditions is the root system that impairs plant growth in the short term by inducing osmotic stress due to shortened water availability and in the long term by saltinduced ion poisoning due to nutrient disparity in the cytosol [11]. A decrease in the shoot to root ratio or increased root to shoot ratio is a common observation in salt stress regimes, which is connected with water stress rather than saltinduced effects. It is demonstrated that a higher root proportion in a saline environment retains toxic ions in that organ, governing their metabolic and translocation activities into the aerial parts. This response can establish a characteristic plant adaptation mechanism under the saline milieu [12,13]. In halophytes, salt-resistant plants exhibit the noteworthy capability to complete their life cycle in salt stress conditions. Throughout progression, they might constitute diverse morphological, physiological, and biochemical mechanisms to proliferate the metabolites in environments with high salt concentrations [14].
Several studies have reported on the accumulation of metabolites from plant parts under different salt stress conditions in many crops and found that saline stress exerts differential consequences on the evolution, ion equilibrium, compatible solutes, and metabolism in leaves [15,16]. Many compatible solutes are nitrogen-derived metabolites, such as amines, amino acids, and betaines; the reason behind this phenomenon is that the availability of nitrogen plays an important role during salinity conditions not only for growth but also for production of these osmoprotectant-related organic solutes [17]. The imbalance between the protein and nitrogen syntheses under salt stress is probably involved in the alterations or increased amino acid level in shoots and roots of plants [17]. In different studies, the salinity treatments exactly increased the levels of proline, sugars, and glycine betaine in wheat [6,18] like in other Poaceae [19,20]. It is well documented that most of the studies on wheat under salinity are conducted on leaves; scarce reports are available investigating the effects of salinity on root metabolic profile regarding changes of metabolites associated with cell physiology and root tissues [21,22].
Reports have shown that studying the effects of salinity in a heterogeneous split root system is more practical than by exposing whole roots to specific levels of NaCl stress [23,24]. This scenario reproduces the great results during salt stress, which adversely affect the growth, development, and biochemical and physiological mechanisms to acclimatize environmental stress, and various changes occur in the metabolic and physiological reactions in plants during the salinity stress [25]. Previously, we reported that the physiological changes of purslane along with fatty acid contents were increased under 200 mM salinity; however, the effect of the particular salinity stress on metabolite accumulation on purslane remains unknown. Herein, we proposed a new perception of the metabolic and physiological responses of purslane under salinity stress. In the existing research, GC-MS was used to analyze metabolic profiling of leaves and roots of two purslane genotypes, Tall Green (TG) and Shandong Wild (SD), under CK and saline exposure. The physiological and morphological traits were also instantaneously studied. Both types of genotypes were greatly affected under salt stress; mainly, salt stress alters the metabolic mechanism in "SD" roots compared to "TG" under salt stress. This study can be useful for future molecular experiments as a reference to select gene expression levels for the functional characterization of purslane.

Materials and Methods
2.1. Purslane Seeds, Cultivation, and Salt Treatment. To scrutinize the influence of saline treatment on the accumulation of metabolites, two different purslane genotypes were chosen from different geographical locations: "Tall Green" local ("TG"-American origin) and a wild variety "Shandong, China" local ("SD") ( Figure S1). Both genotypes were derived from seeds of a single plant and preserved in laboratory settings through self-fertilization for at least three generations. For the propagation of the seed, 72-cell plastic plug trays (50 cm 3 per cell) were used. The substrate used was composed of 30% perlite, 40% peat, and 30% vermiculite, and the substrate was supplemented with a sufficient amount of water during the seedling stage. After 14 days, the seedlings with an identical number of leaves and height for "TG" or "SD" were transferred into plastic hydroponic boxes (525 mm × 365 mm × 205 mm) in the greenhouse of School of Agriculture and Biology, Shanghai Jiao Tong University, China, on 23 rd March 2018. Plants of both genotypes were treated with three different salt concentrations, i.e., 0 mM, 100 mM, and 200 mM NaCl. For each salt treatment, 12 plants of "TG" and "SD" were set in the same box as one replicate, and experiments were run at least four times. A 15 L quarter strength of Hoagland's solution [26] with an electrical conductivity of 4.0 dS m −1 and a pH of 5.8 was put in each plastic box, and a quarter strength of Hoagland's solutions with the same salt concentration was replaced 2 times per week. The plantlets were allowed to grow in a greenhouse with a day and night temperature of 28 ± 2°C and 16 ± 2°C, along with relative moisture and photosynthetically active radiation of 70%-80% and 400 μmol·m -2 ·s -1 , respectively.

Morphological and Physiological
Analysis. At the end of 28 days of salt treatments, the number of leaves, diameter of the stem, main stem length, and root length were recorded with a minimum number of six plantlets. Appropriately, 0.2 g samples of dried roots and leaves were taken, immediately placed in liquid nitrogen, and preserved at -80°C freezer for the physiological and metabolite identification. For Fv/Fm analysis, leaf photochemical efficiency was estimated by measuring chlorophyll fluorescence in the form of the Fv/Fm ratio, with a fluorescence induction monitor (OS 1FL, Opti-Sciences, Hudson, NH). Leaves were covered in a leaf clip to darkness for 30 min before Fv/Fm measurement. For leaf chlorophyll and carotenoid analysis, we cut 0.1 g leaves into pieces, which were placed into small centrifuge tubes with 10 mL dimethyl sulfoxide (DMSO) and saved in the dark environment for 2 to 3 days. After the designated time, the chlorophyll and carotenoid were measured at 663 nm and 645 nm, respectively, by a spectrophotometer (Rochester, NY, USA). Electrolyte leakage was recorded as the percentage of C initial /C max [27]. Leaves and roots of each genotype were harvested separately after the salt treatment and kept at -80°C until further investigation. The polar metabolites were extracted by adopting the protocols as reported earlier with some modifications [27,28]. Frozen samples were ground into a fine powder with mortars and pestles in liquid nitrogen. Approximately, 25 mg powder of each sample was mixed with 1.4 mL (80% v/v) aqueous methanol in a 10 mL centrifuge tube. The resultant mixture was centrifuged for 2 h followed by incubation at 70°C in a water bath for 15 min. Afterward, the extracts were centrifuged (at 12000 rpm) for half an hour and the supernatants were decanted into new culture tubes. Following the addition of 0.75 mL of chloroform and 1.4 mL of water, the mixture was vortexed and centrifuged (at 5000 rpm for 5 min), and 300 μL of the polar phase (methanol/water) was dried in a vacuum concentrator. The dried residue was subjected to derivatization in methoxyamine hydrochloride, and N-methyl-N-(trimethylsilyl)trifluoroacetamide, and analyzed by GC-MS [29]. The derived extracts were analyzed with a PerkinElmer gas chromatograph coupled with a TurboMass-AutoSystem XL mass spectrometer (Perkin Elmer Inc., Waltham, MA). Adequately, the 1 μL extract was injected into a DB-5MS capillary column (30 m × 0:25 mm × 0:25 μm) with an inlet temperature of 260°C. After a 5 min solvent delay, the initial temperature of the GC oven was maintained at 80°C, which was raised to 280°C with 5°C min −1 after 2 min of injection and finally retained at 280°C for 13 min. Helium was employed as the carrier gas with a continuous flow rate of 1 mL min −1 . The analytical measurements were ensured by using electron impact ionization (70 eV) in the full scan mode (m/z 30-550).  [30]. The Kyoto Encyclopedia of Genes and Genomes database was used for pathway analysis.

Morphological and Physiological
Traits. After 28 days of the growth period, ANOVA was used to confirm the differences between morphological parameters. There are significant variations observed under particular salt stress in both cultivars. Table 1 shows that both varieties produced a different number of leaves, length of the stem, diameter of the stem, and length of roots. Salt stress treatment decreased the number of leaves in "TG" at 200 mM and increased in "SD" at the control. The length of the stem was reduced in "SD" at 200 mM and increased in "TG" at the control. The diameter of the stem in "TG" was high at 0 mM and reduced in "SD" at high salinity stress of 200 mM. However, "TG" showed long roots at 100 mM and "SD" showed a short root length at 200 mM compared to the control. Chlorophyll fluorescence measurement is an important index to determine changes in photosynthetic pigments in leaves. The photochemical efficiency (Fv/Fm) values were improved under 0 mM in "TG" and "SD" at 100 mM. Nevertheless, a slight reduction was observed in "SD" at 200 mM ( Figure 1(a)). The chlorophyll content was significantly increased under control conditions in "TG" while 200 mM salinity stress decreased the chlorophyll in both cultivars. However, "SD" showed minor changes at 100 mM salt stress compared to "TG." In addition, the carotenoids were decreased in "TG" and "SD" at 200 mM. Even so, the reduction was observed in "TG" at 200 mM compared to the control. The slight increments of chlorophyll were noticed at 100 mM in "SD." Moreover, under control condition, both cultivars showed an improvement in carotenoid content (Figure 1(b)). The electrolyte leakage was enhanced with increasing salinity levels in purslane leaves in "SD" at 200 mM and decreased at 100 mM. "TG" showed a significant increment in electrolyte leakage at 100 mM and decreased at 200 mM. Moreover, a substantial decrease was observed at the control in both cultivars. Nevertheless, in roots, the higher increments were observed in both cultivars at 200 mM. However, the salinity stress decreased the electrolyte leakage in "SD" at 100 mM, while an increase was noted in "TG" at 100 mM compared to the control (Figure 1(c)).

Determination of Metabolites from P. oleracea Leaves and
Roots under Different Salinity Stress Conditions. The metabolic variations in roots and leaves of purslane cultivars under the particular condition of salt stress were analyzed by GC-MS to understand the physiological responses and Table 1: Morphological comparison of 2 purslane genotypes "Tall Green" and "Shandong Wild" at 28 d of 0 mM, 100 mM, and 200 mM NaCl stress.  (Table 2). First, the mean rank of detected metabolites from leaves and roots of both purslane cultivars at  Figure 1: Effects of salt stress on (a) photochemical efficiency (Fv/Fm) in leaves of "TG" and "SD" and (b) chlorophyll and carotenoid content in (A) leaves of "TG" and "SD" (B) roots of "TG" and "SD." Meanwhile, (c) electrolyte leakage (%) in (A) leaves of "TG" and "SD" and (B) roots of "TG" and "SD" purslane genotypes at 0, 100, and 200 mM salt stress. Vertical bars indicate the SE of each mean (n = 4). Columns marked with small letters indicate significant differences between salt treatments for "TG" or "SD" based on the LSD test (P = 0:05). Columns marked with a star represent statistical significance for comparison between species at a given NaCl treatment (P = 0:05).   Note: relative retention times (RT, min), molecular formula (MF), and mass ratio (m/z) of 132 detected metabolites in purslane genotypes "TG" and "SD" at 21 d of 0, 100, and 200 mM NaCl stress. 7 BioMed Research International 3.3. Metabolic Profile in Roots and Leaves of Two P. oleracea Cultivars in response to Salt Stress. After the determination of metabolites in response to salt stress, the levels of each metabolite were compared with the control. Based on the result of fold change and significant differences, the levels of metabolite responses were different in roots and leaves in "TG." In leaves, 12 major metabolites were significantly increased including 2 organic acids, 2 amino acids, 3 sugar alcohols, 3 amines, and 2 lipids and sterols. The other 12 metabolites exhibited no change, and one metabolite named tyramine was decreased at 100 mM. Under salt stress of 200 mM, 20 metabolites increased including 7 organic acids, 6 amino acids, 4 sugar alcohols, and 3 amines. α-Linolenic acid and guanosine were meaningfully decreased. In roots, a total of 33 metabolites were selected generally: 11 metabolites increased along with 2 organic acids, 4 amino acid, 2 sugars, 1 sugar alcohol, and 2 lipids and sterols; 16 had no significant change; and 6 were decreased under a salt treatment of 100 mM. Besides, 27 metabolites increased along with 10 organic acids, 7 amino acids, 6 sugar, 2 sugar alcohols, and 2 lipids and sterols at 200 mM salt concentration; three had no difference, and 3 decreased at 200 mM as compared to CK. In "Shandong Wild," the metabolic responses are dramatically changed in both leaves and roots. In leaves, 12 metabolites including 1 organic acid, 3 amino acids, 1 sugar, 5 sugar alcohols, and 2 amines were increased signif-icantly. In 200 mM salt stress concentration, the 12 metabolites increased including 3 organic acids, 3 amino acids, 1 sugar, and 5 sugar alcohols. Furthermore, 80 metabolites were calculated with a significant fold change in "SD" roots. In 80 filtered metabolites, 50 increased including 20 organic acids, 19 amino acids, 10 sugars, 8 sugar alcohols, 10 amines, and 3 lipids and sterols; 24 had no difference; and 6 decreased significantly at 200 mM. On the other hand, 70 metabolites showed a significant improvement together with 12 organic acids, 14 amino acids, 7 sugars, 7 sugar alcohols, 7 amines, and 3 lipids and sterols. In addition, six metabolites exhibited no changes and 4 were decreased at 100 mM salt concentration compared with the control (Figures 2(a)-2(d)). In TG leaves, L-alanine and L-serine were

Total Metabolic Contents in Leaves and Roots of Two P. oleracea Cultivars under Different Salt Stress Conditions.
Major metabolites with fold increase and decrease data were pretreated with formula log 2 (treatment/control), and the R package software was used to construct a heat map, displaying the changes in levels of metabolites between P. oleracea cultivars in roots and leaves under different salinity stress conditions (Figures 3(a)-3(d)). Further, the total contents of metabolites were prominently changed under different salt concentrations as compared to the control. The total amount of sugar was higher in "TG" under all concentrations, but no meaningful differences were observed. In leaves, the amino acid, organic acid, sugar alcohol, and amine contents were significantly increased at salt stress of 200 mM compared to "CK." At 100 mM salt stress, high contents of amino acids, sugar alcohols, and amines were accumulated, excluding organic acids and sugars in contrast to the control. In "TG" roots, 200 mM salt stress mainly results in a significant improvement in amino acid and sugar than the control. In addition, no significant changes were observed in organic acid and sugar alcohol (Figures 4(a) and 4(b)).
In leaves of "SD," the organic acid at 100 mM and the amino acid at 200 mM were decreased significantly relative to the control. No substantial changes were noticed in sugar contents under all tested salt concentrations. However, sugar alcohol was increased significantly at 200 and 100 mM compared with the control. In addition, the total organic acid contents were increased in the roots of "SD" and sugar alcohol was significantly increased at 200 mM. The content of amine enhanced at 100 mM compared to the control. Moreover, the organic acid, amino acid, and sugar contents were also improved significantly at 100 mM and amines at 200 mM. There is no significant change in sugar alcohol compared to the control in the roots of "SD" (Figures 4(c) and 4(d)).   Columns marked with small letters indicate significant differences between salt treatments for "TG" or "SD" based on the LSD test (P = 0:05). Columns marked with a star represent statistical significance for comparison between species at a given NaCl treatment (P = 0:05).

11
BioMed Research International and 80 and 41 in roots of "Shandong Wild." Some metabolites responded differently to different salt stress conditions in a genotype-dependent manner, such as myoinositol which was increased 1.59-and 2.79-fold at 100 mM and 200 mM salt concentrations compared to the control, respectively, in "TG" leaves. L-Serine, alanine, L-glutamine, cadaverine, αketoglutaric acid, and malic acid decreased significantly under 100 mM and increased at 200 mM salt stress compared to the control. Tryptophan was increased 1.54-fold at 100 and 1.26-fold at 200 mM. Linolenic acid was increased 1.50-fold at 100 mM and decreased 0.49-fold at 200 mM in comparison to the control. In roots, sugar contents such as sucrose, glucose, fructose, maltose, and mannose were   (1.45). Under 100 mM, sucrose and Ltyrosine resulted in a downregulation in the fold increment and were affected under both salinity stress conditions. Furthermore, DL-ornithine acid showed upregulation but did not demonstrate any significant effect under both salinity concentrations as compared to the control ( Figure 6).

Discussion
In this study, the morphological, physiological, and metabolic changes of the purslane plant were compared under different saline conditions. Results showed that the morphological attributes were affected by 200 mM salt stress compared to 100 mM in "TG." The number of leaves and roots was decreased at 200 mM than the control, whereas the diameter of the stem and length of roots was reduced at 200 mM in the "SD" wild genotype. During the salinity stress, different abiotic factors such as variations in temperature and nonexistence of O 2 can reduce the root length and disrupt the natural architecture of the root system because the cell wall of roots under salinity becomes often irregularly thickened and complex. There is a general decrease in plant growth especially in the number of leaves, reduction in root growth through osmosis, and toxic effect in plants subjected to salinity stress [31]. The photochemical efficiency and chlorophyll contents were significantly improved at 0 mM compared to 100 mM salt stress. At a salt level of 200 mM, the chlorophyll content and carotenoid resulted in a decrease in "TG" and "SD." It is a well-known fact that salt-resistant genotypes showed augmented or unchanged chlorophyll content under the salt stress conditions, whereas the chlorophyll and carotenoid levels declined in saltsensitive genotypes because of the severity of the salt stress [32,33]. The leakage of electrolyte was improved with rising salinity levels in purslane leaves in "SD" at 200 mM. Moreover, a substantial reduction was observed at the control in both cultivars. Nevertheless, in roots, the higher increments of electrolyte leakage were observed in both cultivars at 200 mM compared to leaves.
Purslane is among the C 4 plants with prominent palisade layers on both sides of leaves. C 4 plants exhibit high water use efficiency and CO 2 adaptive strategies to make C 4 photosynthesis, which directly affect chlorophyll pigments during the photosynthesis process in different abiotic stress conditions [34,35]. Under different salt stress conditions, the cell membrane of the purslane plant plays a key role in sustaining the cell turgor pressure and different physiological attributes. In saline environments, plants elicit diverse biochemical and physiological mechanisms to deal with the resultant stress. These mechanisms comprise alterations in morphology, leaf cell membrane stability, photosynthesis, and biochemical variations [1,7]. Further, the metabolomics profiles in the roots and leaves of two purslane genotypes were compared under different salt stress conditions. The alteration of plant cells in a salty environment is firmly associated with different metabolic processes [36,37]. It has been reported that most of the metabolites are involved in different biochemical pathways such as proline synthesis and amino acid pathway metabolism [38]. In these metabolic pathways, carbohydrates, amino acids, and organic acids are key metabolites, which play an important role in plant tolerance and abiotic stress conditions [39]. We found that the contents of organic acid in "TG" leaves significantly increased with increasing salinity and did not show any improvement at 100 mM in contrast to the control (Figure 4(a), leaves). These results indicate that organic acids might engage in regulating intracellular pH by gathering in vacuoles to counteract additional cations [37,40]. Most of the metabolites involved in organic acids were significant in the roots of "SD" under 200 mM salinity stress (Figure 4(d), roots). The metabolites associated with the TCA cycle may indicate that their metabolic activity is related to the plant's capability to improve its growth under the salt stress environment. An earlier report revealed that many organic acids might function as osmoprotectants and thus possibly improved the barley performance under salt stress [41]. In this experiment, increasing organic acids in roots may act to compensate for charge difference [42]. The salt-induced increase in amino acids in leaves and roots in both genotypes suggests a role for these detected solutes in osmotic adjustment during the physiological and biochemical processes under salt stress mechanisms or might be a common phenomenon of particular genotypes' growth and development during salinity exposure. In addition, the content of amino acids significantly increased in "TG" leaves but significantly decreased in "SD" leaves at 200 mM ( Figure 4(a), "TG" leaves; Figure 4(c), "SD" leaves). In roots, the amino acid increment was observed in both of the tested genotypes under 200 mM compared to the control (Figure 4(b), "TG" roots; Figure 4(d), "SD" roots). An increase in tryptophan and phenylalanine content under salinity stress in purslane is linked with shikimic acid and secondary metabolites, which play an essential role in tolerating stress [43]. In amino acid, tryptophan is an inducer of tyrosine and phenylalanine biosynthesis enzymes, which are upregulated in response to abiotic stress [44]. Amino acids such as alanine, valine, threonine, ornithine, glutamine, tyrosine, methionine, and lysine increased significantly under 200 mM salt stress in both genotypes "TG" and "SD," respectively. Another study confirmed that amino acid metabolism is linked to abiotic stress tolerance [45]. Our results displayed that the sugar contents of purslane seedlings were improved in roots at 200 mM in both genotypes. However, a remarkable decline in sugar content was found in the control and 100 mM (Figure 4(b), "TG" roots; Figure 4(d), "SD" roots). Increasing sugar content in roots of both genotypes under salinity stress acts as an osmolyte to stabilize the integrity of the membrane and maintain cell turgor [46]. High levels of fructose, glucose, sucrose, and maltose have been associated with many plant species under various stress conditions [47,48]. The increase in proline, threonine, and proline under particular salt stress in "SD" and "TG" roots may be a characteristic phenomenon of genotypes related to salt tolerance. Proline plays an imperative role in plants under salinity by defending plant cell membranes and protein 14 BioMed Research International degradation by acting as a ROS capture [49]. In addition, glutamic acid is correlated to chlorophyll biosynthesis and glycine as a precursor of glutathione biosynthesis plays an impotent role in antioxidant defense [50,51]. Sugar alcohols were increased in "TG" leaves and "SD" roots and leaves at high salt stress (200 mM) relative to the control (Figure 4(a), "TG" leaves; Figures 4(c) and 4(d), "SD" roots). The content of GABA was enhanced in the roots of "SD" under salt stress conditions due to membrane stability and osmotic adjustment [37] in plants under different abiotic factors. Limited studies also confirmed the presence of GABA as noteworthy nonprotein amino acid, and the levels of GABA increased under different environmental stress conditions [52,53]. Li et al. demonstrated that GABA supports the excess of metabolites in GABA shunt, such as sugar and amino acid metabolism [39], to maintain the metabolic homeostasis under long-term salt stress. In the present case, malate and α-ketoglutarate are increased in roots compared to leaves along with citrate at 200 mM in both genotypes. Besides this, the oxalic acid increased significantly in "SD" roots under 200 mM salt stress. Oxalic acid plays a vital role during low temperature and salt stress due to elevated antioxidant capacity in mango and pomegranate. The content of amines was not much higher compared to other metabolites. Even though 200 mM salt stress showed an increase in metabolites in leaves of genotype "TG" (Figure 4(a), leaves), the contradictory increments were observed in "SD" leaves at 200 mM ( Figure 4(c), leaves). Fatty acids are the important compatible solutes in the purslane plant, which are located downstream of acetyl-CoA in the metabolism pathway. In our results, the palmitic acid was slightly increased in "SD" at 200 mM, while linolenic acid was increased remarkably in "TG" roots at 100 mM with reference to the control. Our results corroborated that augmentation in linolenic acid plays a crucial role in the tolerance of soybean to salinity stress [47].

Conclusions
In this study, the metabolic profiling of leaves and roots of two purslane genotypes, Tall Green "TG" and Shandong Wild "SD," was investigated under the saline stress environments by GC-MS. The morphophysiological attributes of leaves and roots of both the tested P. oleracea cultivars were dramatically altered following salt stress exposure at 100 and 200 mM. Likewise, significant differences subsist on the metabolite profiles among samples under the salinity stress treatments as compared with the control. Metabolic pathway analysis quantified 132 different metabolites in roots and leaves of purslane in response to particular salt stress treatments including 35 organic acids, 26 amino acids, 20 sugars, 14 sugar alcohols, 20 amines, 13 lipids and sterols, and 4 other acids. Most of the metabolites detected are involved in biochemical pathways, such as the TCA cycle, GS/GOGAT cycle, GABA, glycolysis, proline synthesis pathway, shikimic acid, and amino acid metabolic pathway. In conclusion, this study can be useful for future proteomic and molecular research as a reference to select the gene expression level for functional characterization of purslane, which in turn can be advantageous for sustainable agriculture to meet ever-increasing demands for fresh vegetables.

Data Availability
All the data used to support the findings of this study are included within the article or in the supplementary materials.

Conflicts of Interest
The authors declare no conflict of interest.