Contribution of Rhizobium–Legume Symbiosis in Salt Stress Tolerance in Medicago truncatula Evaluated through Photosynthesis, Antioxidant Enzymes, and Compatible Solutes Accumulation

The effects of salt stress on the growth, nodulation, and nitrogen (N) fixation of legumes are well known, but the relationship between symbiotic nitrogen fixation (SNF) driven by rhizobium–legume symbiosis and salt tolerance in Medicago truncatula is not well studied. The effects of the active nodulation process on salt stress tolerance of Medicago truncatula were evaluated by quantifying the compatible solutes, soluble sugars, and antioxidants enzymes, as well as growth and survival rate of plants. Eight weeks old plants, divided in three groups: (i) no nodules (NN), (ii) inactive nodules (IN), and (iii) active nodules (AN), were exposed to 150 mM of NaCl salt stress for 0, 8, 16, 24, 32, 40, and 48 h in hydroponic system. AN plants showed a higher survival rate (30.83% and 38.35%), chlorophyll contents (37.18% and 44.51%), and photosynthesis compared to IN and NN plants, respectively. Improved salt tolerance in AN plants was linked with higher activities of enzymatic and nonenzymatic antioxidants and higher K+ (20.45% and 39.21%) and lower Na+ accumulations (17.54% and 24.51%) when compared with IN and NN plants, respectively. Additionally, higher generation of reactive oxygen species (ROS) was indicative of salt stress, causing membrane damage as revealed by higher electrolyte leakage and lipid peroxidation. All such effects were significantly ameliorated in AN plants, showing higher compatible solutes (proline, free amino acids, glycine betaine, soluble sugars, and proteins) and maintaining higher relative water contents (61.34%). This study advocates positive role of Rhizobium meliloti inoculation against salt stress through upregulation of antioxidant system and a higher concentration of compatible solutes.


Introduction
Global changes have increased abiotic stresses and mounted pressure on agriculture to produce more food from the existing land area to feed the ever-increasing human population. To overcome this challenge, there is a need to bring in large-area cultivation of problematic soils for crop production, such as salt-affected soils, which cover around 20% of the global irrigated area spreading over 60 million hectares [1].
(Jemalong A17) seeds, with a germination rate of more than 90%, were sacrificed by immersion in concentrated H 2 SO 4 for 5 min, and thoroughly washed with distilled water. Afterwards, seeds were surface-sterilized with 5% sodium hypochlorite for 20 min and lastly rinsed thoroughly four to five times with distilled water. After scarification, seeds were subjected to vernalization on wet filter paper in Petri dishes (placed for 48 h at 4 • C, in the dark). After that, Petri dishes were kept in dark in a growth chamber for 48 h at 23 • C with 60-70% relative humidity for seed germination. Five days old seedlings were transferred into pots containing 3 L of Hoagland's nutrient solution. There were total 63 pots, and each pot had 12 seedlings. The seedlings were kept in a growth chamber by maintaining a 16:8 h light:dark cycle, (23 ± 5 • C):(18 ± 5 • C) day:night temperature cycle, with a relative humidity of 60 ± 5%.
Out of the total pots, 42 pots containing 15-days-old seedlings were inoculated with Rhizobium meliloti (Dormal strain), and 21 pots of the seedlings were not inoculated. The noninoculated seedlings were irrigated with one-fourth strength Hoagland nutrient solution every day [19]. The inoculated seedlings were randomly distributed into two groups: (i) AN (active nodules): to allow for the formation of AN (visible as pink color), 21 pots of seedlings were watered with nitrogen-free one-fourth strength of Hoagland solution, and (ii) IN (inactive nodules): the remaining 21 pots of inoculated seedlings were watered with nitrogen-containing one-fourth strength Hoagland solution to develop inactive nodules (white color) [12].

Plant Growth and Nodule Characterization
Before salt stress induction, six pots were randomly selected from each group (NN, IN, and AN) for the examination of nodules, and their nitrogen content was analyzed using the Kjeldahl method. The dry weight of plant biomass was measured before and after salt stress treatments. Nodule volume was measured based on the diameter.

Estimation of Physiological Parameters and Measuring Survival Rate
From the remaining 45 pots, six pots from each group (NN, IN, and AN) containing eight-weeks-old seedlings were exposed to four NaCl stress treatments: 0 (control), 75, 150, and 300 mM NaCl for 3 days. For the measurement of electrolyte leakage, fresh leaves were punched and soaked in sterile water at 4 • C for 2 h. The first conductivity value was taken by a conductivity meter DDS-307 (Leici Corporation, China) and read as L1. The homogenate was boiled at 100 • C in a water bath for 20 min and cooled down to room temperature. Then, the second conductivity value was recorded and read as L2 [20]. Relative electrical conductivity was calculated by using the following formula: Electrolyte leakage (%) = (L1/L2) × 100 (1) Relative water content (RWC) was determined by following the method of Ahanger et al. [20] with minor modifications. Fresh leaves of Medicago truncatula were weighed (FW), then soaked into Petri dishes containing sterile water to gain turgidity for 24 h, and turgid weight (TW) was observed. After being oven-dried, the dry weight (DW) was measured. RWC was calculated by using the following formula: Carotenoids and total chlorophyll contents were measured by homogenizing fresh leaves in acetone (80%) using ice-cooled pestle and mortar. After completing the extraction, the homogenate was filtered, and the volume was adjusted with cold acetone up to 10 mL. Optical densities were observed with a UV-1800 spectrophotometer (Shimadzu, Kyoto, Japan) at 480, 645, and 663 nm [21]. The chlorophyll contents were calculated using the following equations: Chl a (mg g −1 FW) = (13.95 × D663 − 6.88 × D645) × 0.005/W where D645 and D663 are the absorbances of the chlorophyll contents at 645 and 663 nm, respectively, and W is the fresh weight of leaves (g). Photosynthetic efficiency, transpiration rate, and stomatal conductance were observed in the fully expanded leaf using photosynthesis-apparatus Li-6400 (LI-COR Inc., Lincoln, NE, USA), which maintained photosynthetic photon flux density (PPFD) at 1000 µmol m −2 s −1 and CO 2 concentration at 400 µmol CO 2 mol −1 [22,23]. RWC, electrolyte leakage, photosynthetic pigments, and gas exchange parameters were measured in all four salt-treated subgroups: 0 (control), 75, 150, and 300 mM NaCl after 3 days of stress.
The remaining 27 pots containing eight-weeks plants were given the abovementioned concentrations of NaCl for 10 days. After 10 days, plants were given the original nutrient solution without NaCl for another 12 days to allow plants to recover from stress. During this recovery period, plants that developed new green shoots or regained their green coloring of leaves were counted as survived plants. The regrowth capacity of plants was determined based on the fresh weight of regenerated shoots after salt stress.

Analysis of Enzymatic and Nonenzymatic Antioxidant Enzymes
Another experiment was conducted with all three groups of seedlings (NN, IN, and AN) mentioned above in Section 2.1, but this time Medicago truncatula plants were exposed to one level of NaCl (150 mM) salt stress, and biochemical changes were determined at various time intervals: 0 (control), 8,16,24,32,40, and 48 h. The harvested seedlings were immediately frozen in liquid nitrogen and stored at −80 • C for further analysis of osmotic and antioxidants contents, accumulation of secondary metabolites, and other attributes of oxidative stress analysis. All spectrophotometric analyses were conducted on a HITACHI spectrophotometer (UV-3900, Hitachi High-Technologies Corporation, Tokyo, Japan).
Plant leaves of 0.5 g were grinded in prechilled pestle and mortar, with 5 mL of 0.1 M potassium phosphate buffer (pH 7.8), and the mixture was poured into a centrifuge tube. The mixture was then centrifuged at 4 • C for 20 min at 12,000× g, and the supernatant was taken for the measurement of antioxidant enzymes activities. Superoxide dismutase (SOD, EC, 1.15.1.1) activity was calculated based on the ability to inhibit the reduction of nitroblue tetrazolium (NBT) by superoxide anion generated by the riboflavin system under 4000 W (light intensity) at 25 • C [24]. Peroxidase (POD, EC, 1.11.1.7) activity was measured following the method of Bianco and Defez [25], by using guaiacol (C 7 H 8 O 2 ) as an electron donor. Catalase activity (CAT, EC, 1.11.1.6) was determined by observing the conversion rate of H 2 O 2 into H 2 O and O 2 molecules [25]. The glutathione reductase activity (GR, EC, 1.6.4.2) was determined following the method by Palma et al. [18]. Glutathione-dependent oxidation of NADPH was observed at 340 nm for 2 min. Ascorbate peroxidase activity (APX, EC, 1.11.1.11) was measured by the method of Fan et al. [26], and H 2 O 2 -dependent ascorbate-oxidation was observed at 290 nm for 3 min.
Ascorbate (AsA) contents were measured by grinding fresh leaves in trichloroacetic acid (6%), and the supernatant was thoroughly mixed with di-nitrophenyl-hydrazine (2%) and thiourea (10%). Followed by the incubation in the water bath for 15 min, samples were cooled, 5 mL of H 2 SO 4 (80%) was added, and optical density was noted at 530 nm [20]. The standard curve of AsA was used for calculation. The concentration of reduced glutathione (GSH) was determined following the method of Ahanger et al. [27]. One hundred mg fresh leaf tissues were macerating in phosphate buffer (pH 8.0), and the 500 µL supernatant was extracted, which was mixed with 5, 5-di-thiobis-2-nitro-benzoic acid. Absorbance was recorded at 412 nm, and lastly, GSH concentration was calculated following the standard graph of GSH.

Profiling Soluble Sugars and Compatible Solutes
For evaluation of proline content, leaves were homogenized in pestle and mortar, with 3% sulphosalicylic acid and centrifugated at 3000× g for 10 min. After centrifugation, 2 mL of supernatant was taken and mixed with 2 mL each of ninhydrin reagent and glacial acetic acid, and then it was incubated at 100 • C for 1 h. Reaction was terminated on an ice bath, and toluene was used for separation of the proline, while absorbance was recorded at 520 nm [28].
Soluble sugars were determined by using the anthrone method. One hundred mg dry powdered sample was homogenized in 80% ethanol, and the mixture was centrifugated at 5000× g for 10 min. One mL of supernatant was mixed with 4 mL anthrone (0.2%), and optical density was observed at 620 nm [27]. The same protocol was followed for the evaluation of free amino acids [27]. One hundred µL supernatant was mixed with 1 mL ninhydrin reagent and incubated for 30 min, and optical density was measured at 570 nm [29].
For determination of soluble proteins, the Bradford method was used by using BSA as standard, and the absorbance at 595 nm was taken [30]. For determination of glycine betaine, 500 mg dry powdered sample was added in 20 mL distilled water, and samples were put on a shaker for overnight at room temperature. After filtration, 0.5 mL of mixture was mixed with 0.2 mL cold potassium iodide, and periodide crystals were dissolved in 1,2-dichloroethane and kept for 3 h. Optical density was observed at 365 nm, and the calculation was carried out from the standard curve [28]. Nitric oxide content was determined using the Griess-reagent prepared in an ice-cold sodium-acetate buffer (pH 3.6) by following Ahmad et al. [21].

Malondialdehyde (MDA) and Hydrogen Peroxide (H 2 O 2 ) Content
Fresh leaf tissues were homogenized in trichloroacetic acid (0.1%), centrifuged, and the supernatant was thoroughly mixed with thiobarbituric acid (0.5%) at 95 • C for 30 min. Absorbance was recorded at 532 and 600 nm, and an extinction coefficient (ε) of 155 mM −1 cm −1 was used for calculation [24]. H 2 O 2 was measured by employing the potassium iodide (KI) method. For the quantification of H 2 O 2 , 100 mg fresh leaf tissues were homogenized in 5 mL of trichloroacetic acid (0.1%) and centrifuged at 10,000× g for 10 min. Five hundred µL supernatant was mixed with a similar amount of potassium phosphate buffer (pH 7.0) and subsequent addition of 1 mL KI. After thoroughly mixing, the absorbance was read at 390 nm [31].
2.7. Determination of Na + and K + Na + and K + were estimated by a flame photometer that was connected with a continuous-flow system (microflow automated continuous-flow analyzer-III, Systea, Anagni (Fr), Italy) as described by Theerawitaya et al. [32].

Stress Response Models and Salinity-Tolerance Index
Yield response variables such as relative yield (Y r ) and maximum yield (Y m ) were calculated as described by Steppuhn et al. [33] and Abrar et al. [34]. Total plant dry biomass (roots and shoots) was represented as yield (Y), and it was converted to relative yield by using a dividing factor maximum yield that was dependent on the total dry biomass, which is independent of salt stress. The following equation was used to calculate Y r value at each salt stress level in all plant groups.
On the basis of the best-fitted results and maximum R 2 values, an exponential decay model was used to evaluate the yield response to salt stress after computing the data in Equation (6): where the electrical conductivity of Hoagland's nutrient solution is represented as ECi; a and b are the constants, the former depicting the curve shape and the latter determining the model intensity. The salinity-tolerance ondex (STI) shows the inherent ability of crops to tolerate root-zone salinity as suggested by Abrar et al. [34]. EC i50 can be concluded from Equation (7): it is the value of EC at which the yield was reduced to 50% of the maximum yield. The STI can be estimated as described by Abrar et al. [34].

Statistical Analyses
The data collected was arranged and analyzed using Microsoft Excel 2017. Significant differences among treatments were tested by one-way analyses of variance (ANOVA) using the general linear model (GLM), and finally, Tuckey's HSD test was used to compare means at p ≤ 0.05. Statistical analyses were completed using SPSS 20.0 (SPSS Inc., Chicago, IL, USA).

Effect of Rhizobium Symbiosis on Plant Growth and Nodule Characterization
Phenotypically plants showed a similar growth pattern among three nodulation groups (NN, IN, and AN), and no significant differences were observed in shoot and root dry biomass and nitrogen content before salt stress treatment (Table 1). Maximum nodule weight was observed in the AN group, which was 44.05% higher than IN plants (Table 1). The biomass yield of Medicago truncatula corresponding to salt stress levels is summarized in (

Effect of Rhizobium Symbiosis on Survival Rate, Relative Water Content, Electrolyte Leakage, Photosynthetic Pigments, and Gas Exchange Parameters
Rhizobium inoculation significantly ameliorated Medicago truncatula shoot regeneration capacity and survivorship under salt stress treatment (Figure 2A,B). All three groups had 100% survival at control (0 mM NaCl) and 75 mM of NaCl salt stress. However, at 150 mM of NaCl stress, the survival rate was decreased by 47.43%, 41.02%, and 14.   Results showed that rhizobium inoculation and salt stress significantly influenced RWC and electrolyte leakage ( Figure 2C,D). Compared with the control (0 mM), electrolyte leakage of NN, IN, and AN groups significantly increased with an increase in salt concentration ( Figure 2C). Maximum electrolyte leakage was observed at 300 mM level of salt stress. However, at 150 mM the electrolyte leakage was significantly increased by 9.6-fold in NN, 9.1-fold in IN, and 7.1-fold in AN plants, compared to control. RWC was around 85% in all three groups at control, but it showed a significant decline in NN, IN, and AN plants recording a decrease of 47.27%, 39.34%, and 28.64%, respectively, after 3 days of 150 mM stress ( Figure 2D).
Salt stress decreased the chlorophyll contents in all plant groups, more prominently in NN (75.79%) and IN (94.48%) plants at 300 mM of salt stress, compared with control ( Figure 3A). NaCl treatments reduced chlorophyll contents resulting in declined photosynthetic rate, transpiration rate, and stomatal conductance more severely at 300 mM of NaCl. Moreover, photosynthetic rate, transpiration rate, and stomatal conductance were higher with rhizobium inoculation in AN plants by 42 Figure 3B-D).

Rhizobium Symbiosis Up-Regulates the Activities of Antioxidant Enzymes
Before salt stress, no significant difference was observed in SOD activity in all groups. However, the SOD activity in NN and IN was almost similar but significantly higher than AN plants after 8 h of salt stress ( Figure 5A). The SOD activity in AN was higher after 24 h of stress, while it was low and almost similar in NN and IN. AN plants showed significantly higher SOD activity than NN plants after 32 h and 48 h of stress ( Figure 5A). The POD activity in AN plants was lower than NN and IN plants before salt treatment ( Figure 5B). The POD activity in AN plants displayed an increasing trend with salt stress till 24 h of salt stress and significantly higher than NN and IN plants by 35.98% and 15%, respectively. However, at 48 h of stress, the POD activity of NN plants was significantly higher than IN plants by 10.61% ( Figure 5B

Effects of Rhizobium Symbiosis on Osmolyte Contents and Nitric Oxide Quantification
Proline content in Medicago truncatula plants was affected by nodulation (

Effects of Rhizobium Symbiosis on Ascorbate and Reduced Glutathione Content
Nodulation significantly affected ascorbate (AsA) content during salt stress ( Figure 6A). AN plants showed higher AsA content than IN and NN plants during first 8 h of stress, while, after 24 h of salt stress, almost the same level of AsA content was observed in AN and IN plants, but both were significantly higher than NN plants. During 32 h of stress, AN plants showed significantly higher AsA content than NN and IN plants ( Figure 6A).
Reduced glutathione (GSH) content was similar among NN, AN, and IN plants during 0-8 hrs of salt stress ( Figure 6B) Figure 6C).
There was no change in GR activity of NN plants which remained significantly lower than AN and IN plants ( Figure 6C).

Rhizobium Symbiosis Reduced Na + Accumulation and Improved K + Uptake
Na + accumulation was similar among NN, AN, and IN plants just before the onset of salt stress ( Figure 7A). A significant difference was observed at 24 h of salt stress, where NN plants showed higher Na + accumulation than IN and AN plants. However, at 40 h of salt stress, AN plants showed a significant decrease in Na + accumulation compared to NN and IN plants by 24.51% and 17.54%, respectively ( Figure 7A). K + uptake level was similar among NN, AN, and IN plants at 0 h ( Figure 7B). K + uptake reduced with time after inducing salt stress in all plant groups, even though IN and AN plants maintained higher activities during the first 16 h of salt stress. At 24 h of stress, NN plants showed a higher level of K + uptake than AN and NN plants, while, after 32 h of stress, K + uptake of NN plants was significantly lower than AN plants. After 48 h of stress, K + uptake of AN plants was 39.21% and 20.45% higher than NN and IN plants, respectively ( Figure 7B). K + /Na + ratio in all plant groups displayed the decreasing trend at all time intervals, except in AN plants which showed a significantly higher K + /Na + ratio ( Figure 7C).

Discussion
The plants having active nodules produced in response to inoculation with Rhizobium meliloti strain maintained better growth and were better able to withstand salt stress compared to other plant groups (NN and IN). This increased salt tolerance is possibly due to the variation in the nitrogen nutrition levels, since all plant groups possessed nearly the same nitrogen content before salt treatment, and the differences among plant groups were nonsignificant. The viewpoint is additionally supported by improved regrowth capacity of shoots in AN plants at 75 and 150 mM NaCl treatments, respectively, when compared to NN plants. This suggests that the interaction between Medicago truncatula plants and Rhizobium meliloti fundamentally enhanced salt tolerance. Moreover, by following the ECi 50 and STI of AN plants (167.74 dS m −1 and 168.41 dS m −1 ), it was mathematically proven that AN plants seem to be more resistant to salt stress ( Figure 1C) than the NN and IN plants ( Figure 1A,B). By observing the ECi 50 and STI, Medicago truncatula looks more resistant to other crops, e.g., Jatropha curcas (ECi50 = 10.72 dS m −1 , STI = 11.41) and Prunus armeniaca (ECi 50 = 3.39 dS m −1 , STI = 4.63) as stated by Steppuhn et al. [33] and Abrar et al. [34]. However, we also observed that shoot regrowth was also better in AN plants compared to IN plants under the same level of induced salt stress. This could be explained by two points: (i) the physiological responses of AN plants were stronger compared to other plant groups, which suggest that the active nodulation process convert more nutrients for the host plants, which helps tolerate salt stress [24], and (ii) inactive nodules either act as parasites or compete for energy needed by host plants to withstand salt stress. According to Kiers et al. [35], the soybean plant can limit the oxygen supply as a sanction to the rhizobium if it is not fixing the nitrogen. Moreover, some studies have also shown that legumes involving active N fixation are more tolerant to environmental stress than nodules receiving N fertilization [36,37].
A plant's ability to tolerate salt stress depends to a large extent on the distribution and absorption of Na + within the plant [38,39]. Hence, plants respond to alleviate or minimize the harmful effects of extra Na + , by maintaining less Na + accumulation in photosynthetic organs and improving K + levels [30]. Less Na + and more K + in the cytoplasm helps in the maintenance and activity of numerous enzymatic processes [40]. It is well known that in many plants, higher Na + is refluxed by SOS1 proteins or through Na/H exchangers (NHX) into vacuole at the root levels [41]. Better activities of transport proteins that facilitate sequestration and active compartmentation of Na + ions significantly contribute to better salt stress tolerance in plants [42]. K + is one of the most important macronutrients and is directly involved in many plant processes such as enzyme activation, protein biosynthesis, osmoregulation, and photosynthesis [43]. Horie et al. [44] reported that higher salt concentrations cause increased transport and uptake of Na + and lower K + content in shoots. The substitution of K + by Na + may lead to nutritional imbalance, which can reduce plants' ability to withstand stress.
Our data indicated that better growth in plants with rhizobium inoculation (AN plants) restricted Na + uptake by 24.51% and 17.54% followed by an increase in K + uptake by 39.21% and 20.45% than NN and IN plants, respectively ( Figure 7A,B). Moreover, improving K + uptake increased K + /Na + ratio in AN plants at all time intervals ( Figure 7C). Our results were coherent with Ahanger et al. [30], that nitrogen availability minimized the harmful effects of extra Na + by maintaining less Na + accumulation in photosynthetic organs and improving K + levels which maintained a higher K + /Na + ratio [30]. Recently, Abdelaal et al. [45] have also demonstrated that foliar application of silicon significantly mitigated salt stress by reducing Na + and increasing K + contents in sweet pepper.
Salinity leads to oxidative stress by increasing the release of ROS species such as H 2 O 2 , which causes lipid peroxidation (MDA) and maintains membrane integrity in plants. Rhizobium inoculation significantly mitigated the adverse effects of salinity-induced ROS. This could be associated with higher nutrient uptake and lower accumulation of ROS in AN plants, which showed a better antioxidative system to face toxic effects of salt stress. In our study, under 150 mM of salt stress, the AN group significantly produced lower lipid peroxidation recorded in terms of MDA content and a lesser production of H 2 O 2 and EL in comparison to both IN and NN groups ( Figures 2D and 4A,B). Similar results were found in two genotypes of faba bean (Vicia faba), where salt stress significantly enhanced H 2 O 2 , MDA, and EL in both genotypes [46]. Rhizobium-legume symbiosis may protect lipid membrane by lowering H 2 O 2 production and alleviating MDA by increasing activities of antioxidant enzymes such as CAT, SOD, and GR, as well as the contents of AsA and GSH.
ROS can influence enzymatic activities, plant photosynthetic apparatus, and integrity of cellular membranes [47,48]. Nodules contain a set of antioxidant enzymes and metabolites which help avoid the accumulation of ROS and subsequent adverse effects associated with it, including nodule functioning [49]. Higher activity of antioxidant enzymes and their accumulation facilitate the inhibition of lipid peroxidation and in this way, help scavenge ROS. Our results showed that among NN, AN, and IN groups, SOD, CAT, POD, and APX activity were significantly upregulated in the AN plants compared to IN and NN plants ( Figure 5A-D). This result is consistent with Bianco and Defez [25] who reported that activities of SOD, POD, and GR were increased, whereas CAT and APX activities were severely deactivated in the leaves of Medicago truncatula plants under salt stress. Studies have documented that an increase in antioxidant enzymes activity after salt stress is a universal phenomenon observed in almost all kinds of crops, such as in cucumber [26], alfalfa [18], soybean [50], and wheat [30].
Oxidative damage (MDA, H 2 O 2 , and EL) is closely linked with antioxidative defense machinery. In the first step against ROS generation, SOD comes into the act and converts O 2 to H 2 O 2 . This H 2 O 2 is neutralized by activities of CAT in cytosol, POD activities at the membranes, or by activities of GR and APX in chloroplast and mitochondria through AsA-GSH cycle, as suggested by Ahanger and Agarwal [27]. These results might demonstrate why plants with active nodulation process survived adverse conditions better as when O 2 −• levels increased, CAT activity also increased in AN plants leading to a strong response for H 2 O 2 detoxification [12]. In addition, AN plants also showed higher levels of ASA and GSH accumulation for countering oxidative damage ( Figure 6A,B). Similar results were also observed in wheat plants, where AsA and GSH contents were significantly increased resulting in the protection of the photosynthetic electron transport chain by maintaining higher NADP levels and limiting the production of toxic radicals under salt stress [31]. GSH is a low molecule thiol compound in cell regulating scavenging of active oxygen [51] and is also considered to be vital for better development of root nodules. Legumes show a significant positive correlation between nodule GSH and nitrogenase activity with homo-glutathione (h-GSH) contents [52]. Thus, h-GSH concentration controls the efficiency of biological fixation of nitrogen in nodules. Consequently, a deficiency of h-GSH can adversely affect the growth of nodule [53]. In addition to their obvious role in improving nitrogen fixation efficiency, AsA and GSH both regulated the development and growth of plants by upregulating key cellular processes such as cell elongation, senescence, mitosis, etc. [54].
Plants release high contents of osmolytes in the cytosol to avoid the negative effects of osmotic stress induced by salt stress [55]. Amelioration of salinity by improved antioxidant systems in AN plants was further facilitated by the consistent accumulation of compatible osmolytes, including amino acids, proline, glycine betaine, soluble sugars, and soluble proteins ( Table 2). Plant species that showed higher osmolytes accumulation had better growth performance and tolerance under stress by maintaining protein functioning and structure and tissue water contents [20]. Consistent with our results, Ahmad et al. [21] reported a higher accumulation of soluble sugars, glycine betaine, proline, and soluble proteins in chickpea under salt stress. Improvement of the osmolytes accumulation is regulated by modulating their assimilatory pathways that are associated with up-and down-regulation of their synthesis and catabolism [30,38,56]. Verdoy et al. [57] have shown that N 2 fixation in Medicago truncatula proline accumulation enhanced the plants under salt stress. Compatible solutes like proline and glycine betaine protect plants from damages induced by salt stress because of their role in antioxidant defense and osmoprotectant [29]. Soluble proteins also contribute to osmotic adjustment and source of nitrogen storage [58]. Higher soluble protein accumulation under stress could be due to higher biosynthesis of stress-related specific proteins [28]. Therefore, it is suggested that AN plants through improved synthesis and by downregulating the catabolism of osmolytes maintained their higher accumulation under salt stress. Osmolytes accumulation is a ubiquitous response for improving the RWC under salt stress, and rhizobium inoculation-mediated improvement in their accumulation observed in our study explains the beneficial role of active nodules in enhancing the growth performance of Medicago truncatula under salt stress conditions. Higher accumulation of glycine betaine is considered to protect photosynthesis by increasing Rubisco activity under salt stress [59]. Photosynthesis maintains plant growth and subsequently improves plants' ability to tolerate a variety of environmental stresses [60]. Salt stress reduced chlorophyll synthesis, photosynthesis, stomatal conductance, and transpiration rates significantly. However, we found that rhizobium inoculation mitigated that decrease significantly with the impact being much clear due to active nodulation. Our results demonstrated the reduction in chlorophyll content was observed among all groups of Medicago truncatula plants under NaCl stress ( Figure 3A). This reduction in chlorophyll content could partially induce a reduction in biomass yield and growth in all plant groups (NN, AN, and IN). These results are coherent with López et al. [61] that foliage yellowing is generally one of the stress hallmarks, and it is linked with an associated decrease in the contents of photosynthetic pigments [62]. This was also an obvious sign in our study that coincided with an increase in Na + and with the decrease in chlorophyll contents in Medicago truncatula plants. Salt stress causes degradation of pigments by upregulating the activity of chlorophyllase enzyme and downregulating the activities of enzymes linked to chlorophyll biosynthesis in sunflower leaves, which consequently influence the chlorophyll fluorescence and net photosynthesis [63]. Another study showed similar results that salt stress decreases photosynthetic efficiency due to its deleterious impacts on the biosynthesis of chlorophyll's pigment and Rubisco protein [56].

Conclusions
Our study demonstrates that active nodulation is beneficial for increasing the salttolerance capacity of Medicago truncatula plants mainly through upregulating different antioxidative stress mechanisms and maintaining consistent production of compatible solutes. Plants involving active rhizobium symbiosis had higher survival rates and recovered quickly, which was linked with the active metabolism of antioxidants, osmolytes, and metabolites. There is a need to explore more about the active nitrogen fixation process and whether there are opportunities to further enhance salt tolerance. This can help efficiently utilize problematic salt-affected soils for food production. Therefore, inoculation of Rhizobium meliloti could be a promising strategy for improving salt stress management in the fore coming era of climate change.