What is the Difference between the Response of Grass Pea ( Lathyrus sativus L.) to Salinity and Drought Stress?—A Physiological Study

: Understanding the mechanisms of plant tolerance to osmotic and chemical stress is fundamental to maintaining high crop productivity. Soil drought often occurs in combination with physiological drought, which causes chemical stress due to high concentrations of ions. Hence, it is often assumed that the acclimatization of plants to salinity and drought follows the same mechanisms. Grass pea ( Lathyrus sativus L.) is a legume plant with extraordinary tolerance to severe drought and moderate salinity. The aim of the presented study was to compare acclimatization strategies of grass pea seedlings to osmotic (PEG) and chemical (NaCl) stress on a physiological level. Concentrations of NaCl and PEG were adjusted to create an osmotic potential of a medium at the level of 0.0, − 0.45 and − 0.65 MPa. The seedlings on the media with PEG were much smaller than those growing in the presence of NaCl, but had a significantly higher content percentage of dry weight. Moreover, the stressors triggered different accumulation patterns of phenolic compounds, soluble and insoluble sugars, proline and β -N-oxalyl-L- α , β -diamino propionic acid, as well as peroxidase and catalase activity. Our results showed that drought stress induced a resistance mechanism consisting of growth rate limitation in favor of osmotic adjustment, while salinity stress induced primarily the mechanisms of efficient compartmentation of harmful ions in the roots and shoots. Furthermore, our results indicated that grass pea plants differed in their response to drought and salinity from the very beginning of stress occurrence.


Introduction
Adverse climatic and soil conditions force us to look for crop plants with innate resistance to abiotic stresses, in order to attain and maintain food security. The second most important food source, after cereals, is legume plants [1,2]. Legumes are appreciated not only for their nutritional (mainly high protein content) and health (bioactive compounds) values, but also economical (cheap meat replacement, especially in poorer regions) and ecological (nitrogen soil enrichment) ones [2]. This paper focuses on grass pea (Lathyrus sativus L.) [3], one of the oldest domesticated plants in Europe (i.e., since approximately 6000 BC) [4]. However, it is currently neglected by breeders and unused by farmers [3]. The nutritional composition of grass pea seeds surpasses those of chickpea, comparison of grass pea response to these two stressors was examined. To eliminate the influence of other adverse factors (extreme temperatures, pathogens, changing light intensities, etc.), experiments were conducted in vitro.
Our findings demonstrated that drought stress induced a whole-plant level response in the form of growth rate limitation and increased production of a secondary metabolite used in osmotic adjustment. In contrast, salinity stress induced acclimatization mechanisms involving mainly the compartmentation of harmful ions.

Plant Material, Growth Conditions and Stress Treatments
Plant material consisted of seeds of Polish grass pea (Lathyrus sativus L.) cultivar 'Krab'. The seeds were multiplied from those obtained from a collection of legume plants of the Institute of Plant Genetics, Polish Academy of Sciences in Poznań in 2007. The seeds were surface disinfected according to Piwowarczyk et al. [24] and seeded on a medium solidified with 5 g l −1 Phytagel (Merck KGaA, Darmstadt, Germany). Basal medium comprised macro-and microelements of MS medium [25] and 20 g l −1 sucrose. Drought stress and salinity stress were induced by adding polyethylene glycol (PEG) and sodium chloride (NaCl) to the basal medium. PEG and NaCl were added at concentrations generating the same osmotic potential of the medium (Table 1), as calculated according to Kawasaki et al. [26]. For each treatment, ten disinfected seeds were placed in each of five vessels, and the experiments were repeated twice. The vessels with the seeds were kept at 24 ± 1 °C, 16 h day/8 h night photoperiod and fluorescent light of 50 (μmol (quantum) m −2 s −1 ) intensity. Table 1. Osmotic potential of the media and corresponding PEG and NaCl concentrations.

Determination of Germination, Seedling Emergence Rates and Biometric Parameters
Seven days after sowing the seeds, the rates of seed germination and seedling emergence were assessed and presented as percentages of all sowed seeds. Seeds with a visible root were treated as germinating seeds. Seeds with visible roots and shoots were counted as emerging seedlings. After 14 days of culture, the shoot and root lengths of the seedlings were measured, and their fresh and dry weight were weighed. Separated shoots and roots were weighed, and then dried at 120 °C for 48 h and weighed again. Additionally, the percentage of organ dry weight content was calculated according to the formula: = × 100% ÷ , where x is the percentage dry matter content, a is dry weight (mg) and b is fresh weight (mg).

Determination of Na + and K + Content
Sodium and potassium content were determined using atomic absorption spectrometry (AAS). Freeze-dried root and shoot tissue samples (approx. 50 mg) treated with NaCl were placed in digestion vessels and predigested at room temperature in 5 ml of 65% HNO3. After one hour, 2 ml of 30% H2O2 was added to the suspension and digested for another 20 minutes. After preliminary digestion, the samples were mineralized for 40 minutes using a microwave digester (speedwave ENTRY, Berghof, Eningen unter Achalm, Germany), cooled to room temperature, transferred to flasks and adjusted to 25 ml with Milli-Q® water. The solutions were analyzed using atomic absorption spectrometer (Thermo iCE3000, Waltham, MA, US). The cation concentrations were measured against the calibration curves (Na + and K + standards of trace metal basis purity).

Determination of Photosynthetic Pigment Content
The content of photosynthetic pigments was determined using the spectrophotometric method described by Lichtenchtaler [28]. Freeze-dried shoot tissues were extracted twice in 1.0 and 0.5 ml of 80% acetone, and the extract was centrifuged (15,000 rpm, 15 minutes, 4 °C). The absorbance of the diluted extract was measured using a spectrophotometer (U-2900 Hitachi High Technologies Corporation, Tokyo, Japan) at 649 nm, 665 nm and 480 nm. The contents of chlorophyll a (Chl a), chlorophyll b (Chl b) and carotenoids (Car) were calculated according to Wellburn's [29] equations. In addition, total chlorophyll and the ratio of chlorophyll a to chlorophyll b (Chl a/b) were calculated.

Determination of Soluble and Insoluble Sugars
The sugar content was determined by a spectrophotometric method with anthrone reagent [30], with modifications. Freeze-dried tissues (shoots and roots, separately) were extracted overnight in 1 ml of Milli-Q-ultrapure water (Millipore Direct system Q3). After centrifugation (15,000 rpm, 10 minutes), the supernatant was collected, and the pellet was resuspended in 0.5 ml of 0.1 M H2SO4 and incubated for 60 minutes at 80 °C. Aqueous or acid extracts (0.2 ml) were mixed with 1 ml of anthrone reagent (1 g anthrone in 500 ml 72% H2SO4) and incubated for 15 minutes at 95 °C. The reaction was stopped on ice and the samples were left to cool to room temperature. The absorbance of the samples was measured at 630 nm. The content of sugars (mg g −1 dw) was calculated from the calibration curve of glucose.
2.2.6. Determination of β-N-oxalyl-L-α,β-diamino propionic acid (ODAP) Content ODAP content estimation was done according to the spectrophotometric method of Addis and Narayan [31]. Freeze-dried tissues (shoots and roots, separately) were extracted on a shaker overnight in 1 ml of 60% methanol. The extracts were treated with activated charcoal to remove pigments, mixed and centrifuged (15,000 rpm, 10 minutes). The supernatant was divided, and one part was hydrolyzed with 3N KOH for 30 minutes in 95 °C. Unhydrolyzed and hydrolyzed extracts were mixed with O-phtalaldehyde reagent (OPT) or borate buffer. The OPT reagent (pH 9.9) consisted of 50 mg OPT (Merck KGaA, Darmstadt, Germany), 100 μM β-mercaptoethanol, 0.5 ml of 95% ethanol and 49.5 ml of borate buffer. All the samples were incubated at 38 °C for 2 h. The absorbance of the samples was measured at 425 nm. The absorbance of the hydrolyzed sample with OPT reagent was reduced by the absorbance of the hydrolyzed sample with borate buffer, and by one third of the difference between the absorbance of the unhydrolyzed sample with OPT and the unhydrolyzed sample with the buffer. The content of ODAP (mg g −1 dw) was calculated from the calibration curve made for DL-2,3-diaminopropionic acid (DAP) (Merck KGaA, Darmstadt, Germany).

Determination of Proline Content
The proline content was determined by the spectrophotometric method of Bates et al. [32]. Freeze-dried shoots and roots were homogenized in 1 ml of 3% C7H6O6S×2H2O and centrifuged (15,000 rpm, 10 minutes, at 4 °C). The reaction mixture consisting of the extract (0.5 ml), acid-ninhydrin (0.5 ml) and glacial acetic acid (0.5 ml) was incubated for 1 hour at 100 °C. The reaction was terminated on ice. Then, the mixture was extracted with 1 ml of toluene, and the absorbance of the samples was measured at 520 nm. Proline concentration (mg g −1 dw) was determined from a calibration curve made for L-proline (Sigma-Aldrich Chemie, GmBH, Steinheim, Germany).

Determination of Antioxidant Enzymes Activity
Freeze-dried tissues (shoots and roots, separately) were homogenized in 1 ml of phosphate buffer (pH 6.2) and centrifuged (15,000 rpm, 10 minutes, at 4 °C). The reaction mixture, consisting of the diluted extract (1 ml), phosphate buffer (1 ml), p-phenyldiamine (0.1 ml) and 0.1 ml of H2O2 solution, was kept at 30 °C for 10 minutes. Absorbance was measured at 485 nm after 1 and 2 minutes [33]. An increase in absorbance of 0.1 equals one unit of peroxidase (POD) activity.
Freeze-dried tissues (shoots and roots, separately) were homogenized in 1 ml of phosphate buffer (pH 7.0) and centrifuged (15,000 rpm, 10 minutes, at 4 °C). The absorbance (240 nm) of the reaction mixture consisting of 0.2 ml of the extract, 1.8 ml of phosphate buffer and 1 ml of 0.3% H2O2 solution in phosphate buffer was measured for 4 min at 1-min intervals [34]. One unit of catalase (CAT) activity is the amount of enzyme that decomposed 1 μmol H2O2 in 1 min.

Determination of Phenolic Compounds Content
The content of phenolic compounds was determined according to the Folin-Ciocalteu reagent method [35]. Freeze-dried shoot and root tissues were separately homogenized in 1 ml of 80% methanol. The extract was centrifuged (15,000 rpm, 10 minutes, 4 °C). The diluted supernatant (1 ml) was mixed with 0.2 ml of Folin-Ciocalteu reagent and 1.6 ml of 5% sodium carbonate (Na2CO3). The samples were incubated for 20 minutes at 40 °C. The absorbance of the mixture was measured at 740 nm. The content of phenolic compounds (mg g −1 dw) was calculated based on the standard curve made for chlorogenic acid.

Determination of Antioxidant Capacity
Total antioxidant capacity was determined using the FRAP (ferric reducing antioxidant power) assay [36]. The method is based on the reduction of ferric-tripyridyl-s-triazine (Fe 3+ -TPTZ) complex to its ferrous derivative (Fe 2+ ). Freeze-dried shoot and root tissues were separately homogenized in 0.5 ml of 80% methanol. The extract was centrifuged (13,000 rpm, 3 minutes, room temperature), and then 0.1 ml of the extract was mixed with 3 ml of FRAP solution and 0.3 ml of H2O. The FRAP solution (300 mM acetate buffer (pH 3.6), 20 mM FeCl3 and 10 mM TPTZ in ethanol (10:1:1, v:v:v) was prepared fresh and warmed to 37 °C before preparing the mixtures. After 30 minutes, the absorbance of the samples was measured at 595 nm (UV/Vis Spectrophotometer JASCO V-530). The antioxidant capacity was presented as Trolox equivalents calculated from standard curves using Trolox (6-hydroxy-2,5,7,8-tetramethylchroman-2-carboxylic acid) at 0.1 to 1.0 mM.

Statistical Analysis
All determinations were made in five replications. Statistical analyses were done using STATISTICA 12.0 (StatSoft Inc., Tulsa, OK, USA). The results, within the cultivar, organ and parameter, were subjected to a one-way analysis of variance (ANOVA), and the significance of differences between the arithmetical means was determined by Duncan post hoc test at p ≤ 0.05. The data were subjected to principal component analysis (PCA) performed for all analyzed traits in the shoots and roots in R v 3.

Germination Rate and Seedling Performance under Salinity and Drought Stress
Generally, seedling emergence rate was more negatively affected by the applied stresses than seed germination rate. Seed germination was reduced by both stress treatments at their higher concentration (150 mM NaCl and 22 mM PEG) ( Table 2), while the seedling emergence rate was reduced by both stress factors, regardless of the treatment type and concentration ( Table 2). Both parameters showed no differences in intensity for the corresponding concentrations of PEG and NaCl, generating the same osmotic potential of the medium ( Table 2). Seedling growth was also negatively influenced by the applied stresses. Shoot growth was more severely inhibited by drought-imitating conditions than by salinity (Figure 1a-c). Shoot length was reduced on the media with both PEG concentrations, and on the media with higher NaCl concentration (150 mM) ( Figure  1a). However, the fresh weight of the shoots was reduced also on the medium with a lower NaCl concentration (Figure 1b). The root length and fresh weight decreased both on the media with NaCl and PEG; however, no differences were observed between the corresponding NaCl and PEG concentrations (Figure 1a,b). Both stressors reduced the average dry weight of shoots and roots ( Figure 1d). However, an evaluation of dry matter content with reference to fresh weight of organs revealed the opposite direction of changes ( Figure 1e); the salinity generated by NaCl did not change the percentage of dry weight content in the shoots (Figure 1e), but it increased the percentage of root dry matter ( Figure 1e). In contrast, stress generated by PEG increased dry weight content [%] in both the shoots and roots (Figure 1e). In addition, a significantly higher content of dry weight was found in both the shoots and roots of the seedlings subjected to PEG-induced stress compared to NaCl-induced stress ( Figure 1e). Table 2. Percentage of grass pea seed germination and seedling emergence under NaCl and PEG-induced stress after 7 days of culture. Different letters in italic denote significant differences at p ≤ 0.05 within one parameter.

Na + and K + Content in NaCl Treated Seedlings
In 14-day old grass pea seedlings treated with NaCl, the content of K + ions did not change in the shoots, but decreased significantly in the roots (Figure 2a). In turn, sodium ion accumulation increased gradually with increasing NaCl concentration in the medium, both in the shoots and roots ( Figure 2b). The Na + /K + ratio changed in the same way ( Figure 2c). Figure 2. Content of K + (a) and Na + (b) ions and Na + / K + ratio (c) in the shoots and roots of 14-day old grass pea seedlings under NaCl and PEG-induced stress. Different letters in italic denote significant differences at p ≤ 0.05 within one organ.

Content of MDA and Leaf Pigments under Drought and Salinity Stress
In 14-day old grass pea seedlings, MDA accumulation increased in the shoots at lower PEG content, and decreased in the roots at lower NaCl content in comparison with the control and the corresponding concentration of the other stressor ( Figure 3). Stress generated by both NaCl and PEG reduced photosynthetic pigment (Chl a, Chl b and Car) content in grass pea shoots, with the exception of shoots at lower NaCl concentration ( Table 3). The decrease in pigment content was more pronounced in the seedlings cultivated under PEG-induced stress than NaCl-induced stress. There were no significant differences in the pigment content ratio (Chl a/b) between the control and the corresponding stress factors (Table 3). Table 3. Chlorophyll a (Chl a), chlorophyll b (Chl b) and carotenoid (Car) content (mg g −1 dw) and pigment ratio of 14 day-old grass pea shoots under NaCl and PEG-induced stress.

Osmolyte Accumulation under Salinity and Drought Stress
The soluble sugar content increased in the shoots grown on the media with PEG and with higher NaCl concentration, compared with the control. In the shoots at a lower level of NaCl, it did not change in comparison to the control, and was lower than in the shoots from the corresponding PEG treatment (Figure 4a). In the roots, the accumulation of soluble sugars increased only at a higher PEG concentration and decreased at lower NaCl concentration ( Figure 4a). In turn, the accumulation of insoluble sugar in the shoots intensified under both stresses, and was greater in PEG-stressed than NaCl-stressed shoots ( Figure 4b). Increased accumulation of insoluble sugars in the roots occurred only for higher NaCl concentration ( Figure 4b). The ratio of soluble to insoluble sugars decreased in the shoots under both stress conditions (Table 4), while in the roots, it increased at higher PEG concentration and decreased at lower NaCl concentration. Furthermore, the ratio was higher under drought-imitating conditions than in the presence of NaCl (Table 4).
Different letters in italic denote significant differences at p ≤ 0.05 within one cultivar and organ.

Neurotoxin Accumulation under Salinity and Drought Stress
ODAP accumulation increased both in the shoots and roots under PEG stress (Figure 5a). Moreover, its significantly higher content was noted in the shoots grown in the media with PEG than that with NaCl. In the roots, accumulation of ODAP was also noted with a higher concentration of NaCl, and it was greater than for the corresponding PEG concentration (Figure 5a).

Proline Content under Salinity and Drought Stress
Generally, both stress treatments increased proline accumulation in the shoots and roots of 'Krab' grass pea seedlings (Figure 5b). However, the increase was significantly higher in the shoots exposed to PEG-induced stress than to salinity (Figure 5b). Similarly, proline accumulation in the roots was higher in the seedlings treated with PEG than with corresponding NaCl concentrations (Figure 5b).

Antioxidant System under Salinity and Drought Stress
POD activity was higher, compared with the control, in the shoots subjected to both PEG and higher NaCl concentration, and in the roots growing on the media containing NaCl (Figure 6a). Moreover, higher POD activity was noted in the roots cultivated on NaCl media than in those cultivated on PEG media (Figure 6a). CAT activity, as compared with the control, increased in the shoots of the seedlings cultivated at a higher PEG concentration, and decreased at lower salinity and drought stress (Figure 6b). In the roots, CAT activity increased following exposure to higher PEG and NaCl concentrations, and did not change at the lower ones (Figure 6b). The accumulation of phenolic compounds, in relation to the control seedlings, enhanced in the shoots cultivated on the media with PEG and lower NaCl concentration (Figure 6c). No differences between the stressors and concentrations were noted. In the roots, phenol content increased in the seedlings cultivated on the media with NaCl and higher PEG concentration (Figure 6c). Greater accumulation of phenols was observed in the roots of the seedlings growing on the media with lower NaCl concentration vs. roots from the media with PEG generating the same osmotic potential (Figure 6c). The total antioxidant capacity dropped in the shoots of seedlings growing at higher concentration of NaCl and PEG (Figure 6d). No significant differences were noted between the corresponding treatments. In contrast to this, the antioxidant capacity was significantly higher in the roots under NaCl-induced stress than under the corresponding PEG-induced stress (Figure 6d).

Principal Component Biplot Analysis
PCA biplots were generated for shoots and roots separately. They indicated that both principal components explained almost 84% of the total variance in the shoots, with the first principal component (PC1) explaining 71.4%, and the second (PC2) only 12.22% (Figure 7a). The analysis revealed clear differences in grass pea shoot responses depending on the medium used, as distinguished by PC1. Under drought stress induced by PEG, shoot response was rather similar, regardless of the stressor concentration. Under salt stress, a lower NaCl concentration resulted in a similar plant response as the control, while a higher sodium chloride concentration triggered a different reaction, as distinguished by PC1 and PC2 (Figure 7a). The PCA biplots explained also almost 75% (PC1: 43.65%, PC2: 31.03%) of the total variance in the roots (Figure 7b). Plant roots reacted similarly, regardless of the stressor concentration, with a clear difference in reaction between PEG and NaCl, as explained by the second principal component (PC2) (Figure 7b). Furthermore, the analysis revealed that the mechanism of response to drought stress in shoot cells was associated with an increase in the content of proline, ODAP, soluble and insoluble sugars and POD activity. Additionally, these parameters correlated negatively with the content of photosynthetic pigments and fresh weight (Figure 7a). The response to the higher NaCl level involved CAT activity. The analysis also revealed positive correlations between ODAP, proline and sugars, and negative correlations between CAT activity and total antioxidant capacity (Figure 7a). In the roots, the response to salinity stress manifested in increased POD activity, phenol accumulation and total antioxidant capacity, which were also positively correlated (Figure 7b). In turn, root response to drought stress manifested in increased soluble sugar accumulation and MDA content (Figure 7b). Furthermore, in the case of more intense stress (both drought and salinity), the roots responded similarly by increasing accumulation of proline, ODAP, insoluble sugar, dry weight and activity of CAT (Figure 7b).

Discussion
Germination is considered the most critical stage in a plant life cycle; the process is highly sensitive to stresses, mainly abiotic ones. It starts with the uptake of water (imbibition), and completes with the appearance of a radicle [39]. Germination is a very complex process during which seeds need to quickly switch from dormancy to accelerated metabolic activity to enable the appearance of the radicle, followed by a plumule [40]. Imbibition consists of rapid water uptake until the complete hydration of all cell components and the reactivation of metabolism have occurred, allowing for further stages of germination. Thus, environmental conditions limiting water availability, such as drought, salinity or freezing, negatively affect this key process [41]. Many authors, who compared germination efficiency under stress induced by NaCl and PEG, observed a stronger reduction of germination rates in the presence of PEG, compared to NaCl [42][43][44][45][46]. In our study, no significant differences were observed in grass pea seed germination on media with the same osmotic potential generated by various stressors (NaCl and PEG). Our results do not confirm the observation of Zhang et al. [43], i.e., that sodium ions can act as an osmotic regulator that increases water uptake by germinating seeds. Moreover, Na + ions may have a toxic effect on seed germination. Desiccation of seeds upon entering dormancy, and subsequent changes related to seed rehydration during imbibition, generate free radicals and damage cellular components. After the seed rehydration phase, the seed cells synthesize enzymes associated with the repair and reduction of cellular damage that can be adversely affected by sodium ions [40]. The different outcomes of previous studies may also have resulted from different experimental techniques. The use of in vitro cultures requires seed sterilization by soaking in aqueous solutions for several to a few dozen minutes. Grass pea seeds have to be sterilized for over 30 minutes [47][48][49][50]; in this way, preliminary imbibition already occurs during sterilization. Under stressful conditions, this may facilitate the transition to further germination stages, but may also delay them. The delay would be due to the increased water potential of the seeds impeding the further uptake of water from an environment with lower water potential. This was observed in our study at higher concentrations of NaCl and PEG. Moreover, the mobilization of storage material from the cells and the reactivation of cell energy metabolism control the seed transition to the next (final) stage of germination. This germination stage is often inhibited by harsh environmental factors. The final stage of germination (sensu stricto) is the elongation of a radicle and its breaking through the seed coat; this depends on the growth of the embryo cells (radicle and surrounding tissues), which is executed by water absorption [40,51]. That is why seed germination decline is so often observed in the conditions preventing water uptake from the environment [24].
Some authors report that the germination capacity of seeds under stress may better reflect seedling growth, followed by better plant yield [44]. In our research, however, the percentage of seedling emergence was lower (between 10 to 50%), relative to the percentage of germinating seeds. Other authors also noted that both salinity and drought had a more negative impact on the growth of a hypocotyl than of a radicle [45,46,52]. The postgermination stage of shoot growth commences with intensive cell divisions that are very sensitive to water deficit [40]. Interestingly, also for this parameter, no significant differences were spotted between NaCl and PEG-induced stress, which may suggest that the observed plant response is a reaction to osmotic, rather than chemical, stress. Still, dividing cells should be more sensitive to adverse ion ratios, due to a lack of a well-developed vacuole into which harmful ions could be discharged [51].
The physiological process most sensitive to water deficit is cell growth. Water stress is a highly limiting factor in the initial phase of growth, because low turgor pressure inhibits cell growth and development [53]. The stressors applied in our study significantly affected shoot and root length and weight after two weeks of culture. In this case, our observations were consistent with those of other authors, who reported a stronger inhibition of organ growth under stress imitating drought than salinity [42,44,46,54,55]. According to Munns [17], the harmful effects of salinity stress involve primarily water (osmotic) stress, and chemical stress only after a few days, resulting from the accumulation of harmful ions. One of the most important adaptations of plants to water shortage is osmotic adjustment [56][57][58][59]. Osmotic adjustment, consisting of the accumulation of organic and inorganic water-soluble compounds, has two main roles to fulfil: osmoregulation and osmoprotection [56,58]. Osmoregulation involves the accumulation of osmotically active compounds to reduce the osmotic potential and to maintain the cell turgor necessary for the proper course of many physiological processes [58]. In addition, under salinity stress, this process may be associated with either complete exclusion of toxic sodium and chlorine ions, or their accumulation, but only to a level that is nontoxic to cells [59]. Our results indicate that salinity stress is less harmful to grass pea seedling growth than drought stress. One possible explanation is the reduction of root osmotic potential, due to the accumulation of Na + ions, which allows plants to absorb water more efficiently and continue uninhibited growth [51]. High content of Na + ions, both in the roots and shoots of the examined grass pea seedlings, indicated that this parameter controlled the effective seedling growth under salinity. Such an effect was not observed in the case of PEG 6000, because its high molecular weight does not allow its transport via cell wall pores and into the protoplast [41]. As a result, water is withdrawn not only from the protoplast, but also from the cell wall causing cytorrhysis, not plasmolysis, which is observed in the case of drought in natural conditions [41]. On the other hand, the accumulation of Na + ions, and to a lesser extent, also Cl -, has a disastrous effect on cell growth and function over time [16,23,59]. Consequently, an effective mechanism of ion exclusion and the compartmentation of harmful ions in the vacuole, increasing with growing cells, and/or preclusion of ion transport to seedling shoots, has to occur [16,17]. A high content of Na + ions in the shoots of cv. 'Krab' grass pea seedlings, together with milder growth inhibition effects, suggest the occurrence of an effective mechanism of ion compartmentation. Our results also revealed no limitations in ion transport to the shoots, despite reduced transpiration in the tissue cultures [41].
Crops respond to salinity or drought stress by changes in dry matter content [24,46,50,60,61], which is considered one of the key indicators in assessments of plant tolerance to abiotic stress [60]. Dry matter production in plants is a result of a complex physiological process whose main substrates are carbohydrates. Their synthesis occurs primarily during photosynthesis, but also in alternative cycles such as gluconeogenesis [62,63]. Disorders affecting photosynthesis and resulting from water (osmotic) and chemical stress significantly impair the production of assimilates and their distribution in the plant. Often, the main organs using sugars from primary and secondary production are the roots, in which osmotically active compounds are produced to change the water potential of cells in order to maintain water uptake from the environment [61,63]. Thus, an increase in dry matter content is often treated as a feature typical of plants tolerant to water and chemical stress [24,50]. Disturbances in carbohydrate metabolism under stress conditions may lead to a negative carbon balance, unless at the same time there is a reduction of growth [63]. In the presented research, dry matter content increase was observed in the shoots and roots of grass pea in conditions imitating drought (PEG-induced stress), as compared with control conditions. Moreover, the dry matter content in these seedlings was significantly higher than in the seedlings growing at corresponding NaCl concentrations. Such a significant increase in dry matter content, in both the above-and underground parts of the seedlings growing in drought-imitating conditions, most likely resulted from the production of osmoregulatory compounds (e.g. sugars, proline, glycine betaine), as well as osmoprotective and antioxidant compounds (e.g. phenolic compounds) [64]. At the same time, as mentioned earlier, these seedlings showed a stronger inhibition of shoot and root growth in relation to the control, and shoot growth in relation to the corresponding NaCl concentrations. To synthesize 1 mole of an osmolyte, a plant requires much more ATP molecules than to accumulate 1 mole of NaCl, and ATP synthesis this takes place at the expense of plant growth [16,59]. Moreover, a lower increase of dry matter content in the seedlings growing under salinity additionally confirmed the role of Na + ions as osmoregulators.
To determine plant sensitivity to stress conditions, cell membrane integrity is often assessed by evaluating lipid peroxidation [65,66]. The unsaturated membrane lipids of plant cells are attacked by ROS overproduced during stress and leading to lipid oxidation (peroxidation) [67]. Peroxidation breaks down the unsaturated lipids resulting in, among others, the formation of malonyldialdehyde (MDA) [65,67]. The increased accumulation of MDA indicates intense lipid peroxidation, and is often interpreted as a symptom of impaired antioxidant system activity [65,68,69]. In the presented research, the content of MDA remained fairly stable in both organs (shoots and roots) and under both stresses (salinity and drought). This indicates either effective scavenging of free radicals by the antioxidant system, or the prevention of free radical production. However, it seems that the mechanisms that protect membranes from excessive lipid peroxidation are different, depending on the type of stress and organ, and can be associated with increased phenol accumulation or peroxidase activity.
The sensitivity of plants to stress conditions is very often evaluated by photosynthetic pigment content analysis, which allows for an initial assessment of the photosynthetic apparatus condition [16,70]. A decrease in the photosynthetic pigment content under conditions of water scarcity, both due to drought and salinity, results primarily from disorders in their synthesis [71][72][73]. A number of enzymes are involved in the synthesis of plant pigments [74]. Studies indicate that both drought and salinity reduce the content of 5-aminolevulinic acid (ALA), a precursor of porphyrins and, consequently, chlorophylls, by interfering with ALA dehydrogenase [71][72][73]. Dalal and Tripathy [72] reported that under stress, plants reduce the expression of genes associated with porphyrin biosynthesis, preventing the production of intermediates that could generate free radicals. Pigment synthesis disturbances may also result from impaired enzyme activity as a result of disturbances in the ionic homeostasis of cells, affecting the availability of enzyme cofactors [75,76]. In the shoots of grass pea, the content of photosynthetic pigments decreased under both NaCl-and PEG-induced stress. A significantly greater decrease was observed under drought-imitating conditions than under salinity. Under NaCl-induced stress, cells are most likely capable of uptaking water for longer periods, due to the better osmotic adjustment resulting from (Na + ) ion accumulation [59]. This way, they can protect the enzymes involved in pigment biosynthesis from dehydration and/or ensure ion homeostasis. The drop in pigment content as a result of chlorophyll synthesis disorders, not degradation, was also confirmed by no changes in Chl a/b ratio. During the process of chlorophyll degradation, Chl b is transformed into Chl a, and this changes the ratio of these pigments [71].
One of the most important functions of the photosynthetic apparatus is the production of carbohydrates that are indispensable for plant primary and secondary metabolism [77]. Under stress conditions, carbohydrates are accumulated and used, e.g., for the osmotic adjustment [56,57]. In addition to the aforementioned osmoregulation, osmotic adjustment also plays a protective (osmoprotective) role by accumulating compounds that stabilize proteins, especially enzymes, or participating in scavenging of newly formed free radicals, thus protecting the plasma membrane integrity [78,79]. In the present study, a significant increase in soluble sugar content was observed in the shoots of grass pea growing under conditions of PEG-induced stress. In the case of lower salinity, other compounds or ions participated in the osmotic adjustment of shoot cells, as evidenced by the shoot growth rate and lower content of soluble sugars. Generally, the production of osmotically active compounds depends on the efficiency of photosynthesis and/or gluconeogenesis activity under stress conditions, and their accumulation in the roots from the partitioning of assimilates [80]. The increase in soluble sugar content in the roots was slightly higher on the medium with PEG than NaCl. No changes in the content of insoluble sugars, with one exception, were noted. A significant increase in insoluble sugar content and no change in the ratio of soluble to insoluble sugars was observed in the roots on the medium with higher NaCl concentration, which may suggest effective osmotic adjustment mediated by Na + . In addition, the increment in insoluble sugar content indicated an increase of other polysaccharides content, e.g., the ones building the cell wall, which may act as free radical scavengers [81] or regulate cell growth [82]. In addition to their osmoregulatory function, carbohydrates can also serve as osmoprotectants [58]. Simple sugars, together with plant hormones, create a signal network in plants participating not only in the cell cycle and cell division, but also enabling plant response to emerging stress. Moreover, sugars are believed to play an important role in scavenging hydroxyl radicals (OH • ) through the Fenton reaction in the presence of Fe 2+ ions [83]. Regardless of the strategy chosen, effective protection against the negative effects of both ionic and osmotic stress was observed in the roots.
The neurotoxin ODAP is a characteristic compound for grass pea [84]. Grass pea breeding has sought to produce cultivars and lines with the lowest content of ODAP [7,10,85]. Meanwhile, some research studies have suggested changes in the content of this compound under the influence of environmental stresses, indicating that it can play a significant role in plant response to abiotic stress [86][87][88][89][90][91][92][93]. Drought stress, most often induced by PEG, increased the ODAP content in various organs and tissues [86,[88][89][90][91]. Under salinity stress, greater variability was observed in ODAP accumulation patterns. The content of ODAP decreased at lower concentrations of NaCl (below 0.4%), but it increased at higher ones (above 0.4%) [86]. In our study, a higher accumulation of ODAP was also observed in both the shoots and roots of grass pea seedlings under PEG-induced stress. Furthermore, salinity stress did not reduce ODAP content either in shoots or roots, and did not change or increased it in the roots under higher NaCl concentration. It is believed that ODAP, as a soluble nonprotein amino acid, can act as an osmoregulator [88,81], or even as free hydroxyl radical (OH • ) scavenger [94].
Under abiotic stress, plant cells struggle to maintain a balance between energy production and consumption. Imbalances, occurring mainly in chloroplasts and mitochondria, result in excessive production of ROS and free radicals [95,96]. Plant cells cope with the excess by activating and synthesizing de novo antioxidants, both enzymatic and nonenzymatic [97].
Under stress conditions, the efficiency of the dark reactions (Calvin cycle) of photosynthesis is reduced, leading to the photo-oxidative generation of huge amounts of ROS. To protect cells against the uncontrolled generation of oxygen free radicals, plants increase the rate of photorespiration, preventing limitation on the PSII acceptor side. However, as a result of intensive photorespiration in peroxisomes, H2O2 is intensively produced. CAT is an enzyme that very effectively and efficiently scavenges hydrogen peroxide molecules, and its high activity was observed in the leaves of many plant species as a response to osmotic stress [96,98]. At the same time, catalase activity may also be associated with lignification [99,100]. Grass pea shoots showed intense catalase activity only at higher PEG concentrations, indicating massive production of H2O2 during drought stress, which was not observed in the case of severe salinity stress. At the same time, higher concentrations of NaCl and PEG induced high CAT activity in the roots. In the case of seedlings growing under NaCl-induced stress, increased CAT activity, together with increased accumulation of phenolic compounds and POD activity, may indicate a progressive process of root lignification.
Peroxidases (ascorbate, glutathione, guaiacol) belong to the most common enzymatic antioxidants [101]. The method used in this study to determine the enzyme activity using p-phenylenediamine as a substrate is useful in the determination of guaiacol peroxidase (POD) activity [24,102]. Guaiacol peroxidase, also called phenolic peroxidase, is involved in H2O2 scavenging, as well as in lignin biosynthesis, and therefore, in cell growth and development [101]. Different POD isoforms occur in the cytosol, vacuoles, and primarily in the cell wall. It is believed that the latter take part in plant defence responses to various stresses [102]. In our research, POD activity increased in both shoots and roots under stress conditions. The increase was greater in shoots exposed to PEG-induced stress, and in the roots under NaCl-induced stress. Enhanced POD activity in the shoots most likely results from stronger stress, as evidenced by stronger growth reduction. Increased POD activity in the roots may result from the intensification of lignin biosynthesis in the cell walls that can permanently bind Na + ions [81]. This was also confirmed by the observation of increased accumulation of phenolic compounds in these roots.
Nonenzymatic components of the antioxidant system comprise glutathione, ascorbate, tocopherol, carotenoids, and phenolic compounds [103]. Phenolic compounds belong to a very wide family of secondary metabolites synthesized in the shikimic acid pathway [104]. It is estimated that about 20% of carbon assimilated in photosynthesis is directed to the phenylpropanoid pathway [103]. Studies indicate the importance of phenolic compounds in alleviating the negative effects of abiotic stresses [105][106][107]. An increase in drought and salinity tolerance was observed, along with an increase in phenolic compound content in both wild and crop plants [108][109][110]. The antioxidant properties of phenolic compounds result from their structure, which makes them excellent reducing agents, as well as from the possibility of chelating metal ions, which prevents uncontrolled redox reactions [106]. Phenolic compounds can also react with free radicals, becoming phenoxyl radicals, which, thanks to their stable structure, stop radical propagation and terminate the radical chain reaction [106]. Phenolic compounds also participate in the synthesis of components building the secondary cell wall, increasing its thickness and, at the same time, resistance to stress [105]. The increase in the content of phenolic compounds that we witnessed in plant roots exposed to NaCl, especially at lower concentration, and in comparison with PEG-induced stress, indicated that these compounds play important roles in the mechanism of root resistance to salinity stress. Most likely, they participated in the chelation of Na + ions mainly in the cell wall. A similar increase in phenols in plants treated with both stressors, as compared with the control, indicated that shoot phenolic compounds acted as osmoprotectants during salinity and drought stress.
Apart from phenols, other low molecular compounds may also play an important role in scavenging free radicals or repairing their harmful effects. Therefore, a FRAP assay was used to estimate the total antioxidant capacity. This method allows for quick assessments of the total antioxidant activity of low molecular weight antioxidants including phenols, but also ascorbic acid and simple sugars [111,112]. Generally, our results indicated that the activity of low molecular weight antioxidants was of greater importance in the roots than in the shoots of stressed seedlings. Furthermore, the observed alterations point to a greater contribution of low molecular weight antioxidants to the acclimatization of grass pea roots to salinity than to drought stress. However, strong correlation between FRAP and phenol accumulation, as revealed by PCA analyses, indicated a crucial antioxidant role of phenols.
Different stresses imply disturbances of anabolic process efficiency, leading to a reduction in carbon skeleton synthesis during photosynthesis. Moreover, stress imposes the allocation of these carbon skeletons from primary metabolism to secondary metabolite production, and leads to the synthesis of secondary metabolites involved in plant resistance and/or tolerance mechanisms [113]; one such secondary metabolite is proline [114]. The role of proline and the mechanism of its action are not clear. Over the years, proline has been treated as an osmotically active substance, responsible for the rapid and effective reduction of the cell water potential [114]. Many studies pointed to its marginal role in the cell osmotic adjustment [115][116][117]. It seems that under stress conditions, the mechanism of proline action is associated with the protection of enzymes and cellular membranes. Due to its kosmotropic properties, proline protects key enzymes against conformational changes induced by dehydration under osmotic and/or salt stress. Additionally, it indirectly reduces the effects of oxidative stress by protecting antioxidant enzymes against denaturation [118]. The higher accumulation of proline in the shoots and roots of grass pea seedlings under PEG-induced stress indicated its greater importance in the acclimatization of grass pea to osmotic than to chemical stress. Proline, in addition to its role in stabilizing tertiary and quaternary structures of enzymatic and structural proteins, is also an important element of osmotin and late embryogenesis abundant (LEA) proteins. These proteins are part of a large protein system involved in plant response to abiotic stresses, including drought and salinity [119,120]. Under stress conditions, the action of these proteins consists of the regulation of the osmotic adjustment by intracellular compartmentation and the redistribution of osmolytes, changes in the metabolic rate, as well as increasing cell wall elasticity and membrane permeability [121]. Moreover, under salinity stress, these proteins are responsible for the redistribution and complementation of Na + in vacuoles and/or in the cytosol, as well as the distribution of sodium ions to the apoplast and its sequestration in the cell wall [122][123][124]. Increasing knowledge of the importance of these proteins in the mechanisms of plant acclimatization to abiotic stress underlines the importance of analyses of osmotin and LEA proteins in the future research of the response mechanisms of grass pea to stresses.

Conclusions
Our experiment on NaCl and PEG stressors at concentrations generating the same osmotic potential of the medium revealed differences in the mechanisms of grass pea response to salinity and drought stress. Grass pea cv. 'Krab' was characterized by greater tolerance to salinity (NaCl induced) than to drought. The mechanism of grass pea response to salinity stress seems to be primarily associated with an effective distribution of Na + ions, which can be used as osmotically active compounds, ensuring adequate hydration of cells, and reducing the need for excessive production of osmoprotectants (lower proline accumulation), thus not limiting the growth and development of the seedlings. Moreover, increasing phenol and insoluble sugar accumulation, as well as the lack of severe stress symptoms (low MDA accumulation), may indicate the sequestration of excessive Na + ions in cell walls. In contrast, grass pea acclimatization to drought depends mainly on the mechanism of osmotic adjustment, using soluble sugars as osmoregulators, and proline as well as probably ODAP as osmoprotectants, at the expense of plant growth and development. It is believed that in the initial stages, salinity stress is also water (osmotic) stress, and that plant responses follow the same mechanisms in both cases. However, our findings indicate that grass pea exhibits a clearly differentiated response to salinity and drought stress from the very beginning of its vegetation.