Role of Local Biofertilizer in Enhancing the Oxidative Stress Defence Systems of Date Palm Seedling (Phoenix dactylifera) against Abiotic Stress

National Institute of Agronomic Research, Plant Protection Unit, Laboratory of Phyto-Bacteriology, Marrakech, Morocco Laboratory of Plant Biotechnology, Ecology and Ecosystem Exploitation, Department of Biology, Faculty of Sciences, El Jadida, Morocco Cadi Ayyad University, Laboratory of Microbial Biotechnologies, Agro-sciences and Environment, Marrakesh, Morocco Department of Biology, Polydisciplinary Faculty of Larache, Abdelmalek Essaâdi University, B.P. 745, Larache, Tétouan, Morocco National Institute of Agronomic Research, UR Agro-Biotechnology, Laboratory of Plant Biotechnology, Marrakech, Morocco National Institute of Agronomic Research, UR Environment, and Conservation of Natural Resources, Rabat, Morocco


Introduction
Agriculture production decreases globally mainly due to biotic and abiotic stresses. Abiotic stresses reduce the growth and development of plants at biochemical and molecular levels and cause immense crop loss in agricultural production [1,2].
is environmental stress poses a major challenge in our quest for sustainable food production as it reduces the potential yields as high as 70% in crop plants [3]. Overall, abiotic stress often results in several morphological, physiological, biochemical, and molecular changes that adversely affect plant growth, development, and productivity. Among these stresses, drought is the first environmental stress responsible for a decrease in agricultural production worldwide; it affects plants in various ways, including slowing down plant growth, disrupting the membrane integrity of vital cellular organelles such as chloroplasts, depriving photosynthesis, and creating an imbalance in osmoregulation yield. Salinity is the second most prevalent soil problem after drought [4,5]. It should also be noted that nearly, all of these abiotic stresses result in oxidative stress and involve reactive oxygen species (ROS) formation in plant cells [1]. Under normal conditions, antioxidant enzymes keep the production of ROS in cells at low levels. is balance can be disturbed by the loss of antioxidants or excessive concentration of ROS, resulting in oxidative stress and causing ultimate damage to cellular macromolecules and membranes and increased lipid peroxidation [6,7]. Nevertheless, in many cases, the production of activated oxygen in plants exceeds their ability to detoxify it [8].
erefore, sometimes, most plants possess an additional mechanism that helps them to tolerate stress, which consists of an association with the microbial population of their rhizosphere surrounding that can help them to survive and ameliorate their productivity [9]. e microorganisms can be present in the rhizosphere, root tissue, and/or a special root structure called a nodule, and they generally include bacteria, algae, fungi, protozoa, and actinomycetes [9]. Different types of bacteria have a significant effect on plant growth and are known as plant growth-promoting rhizobacteria (PGPR). ey play an important role in increasing plant growth and development through some direct and indirect mechanisms such as plant growth regulators and organic acids as well as protection through enzymes, under both nonstress and stress conditions [10][11][12]. Generally, PGPR bacteria can increase plant growth by increasing the nutrient's availability in the rhizosphere and also enhance the production of plant hormones, such as IAA [13]. ey can also stimulate plant growth and development throughout the production of substances such as exopolysaccharides and rhizobitoxin that allow the plants to withstand abiotic stress conditions [11,14].
In addition to the bacterial population present in the rhizosphere, fungi also represent a significant portion of soil rhizosphere microflora and play an important role in plant growth. e symbiotic association generated by fungi (mycorrhizae) with plant roots increases the root surface area and thus allows the plant to absorb water and nutrients more efficiently from large soil volume.
is obligated mycorrhizal association not only increases the nutrient and water availability but also protects the plant from a variety of abiotic stresses [15][16][17][18].
Some mechanisms used by arbuscular mycorrhizal fungi (AMF) under certain conditions can explain the growth promotion due to this association, which includes the production of metabolites such as amino acids, vitamins, phytohormones, and/or processes of solubilization and mineralization [19]. It is also well documented that AMF influence the expression of several antioxidant enzymes that protect plants from reactive oxygen species generated under stress conditions [20,21]. While supplying plants with nutritional and structural benefits, they also provide other benefits to them including production/accumulation of secondary metabolites for osmotic adjustment under osmotic stress, improved nitrogen fixation, enhanced photosynthesis rate, and increased resistance against biotic and abiotic stresses. Many researchers have reported that AMF can improve plant's tolerance to heavy metals, drought, and salinity and also protect plants from pathogens [22][23][24][25][26].
Date palm is one of the most important members of the Palmaceae family and one of the oldest fruit crops grown in the arid regions [27]. It has long been one of the major fruit crops for many arid and semiarid populations because of its high productivity, the high nutrient value of its fruits, and its adaptation to conditions of the Saharan regions. It has a very ancient history and it is still a key food supply for this population. During the past three centuries, dates were also introduced to new production areas in Australia, India, Pakistan, Mexico, southern Africa, South America, and the United States [27]. Dates are the main income source and staple food for local populations in many countries in which they are cultivated and have played significant roles in the economy, society, and the environment of those countries [28]. Moroccan date palm groves occupy a surface area of more than 48,000 ha with a population of 4.8 million trees; they are composed of about 55.6% seed-derived seedlings representing about 2.5 million trees, each of which is genetically different [29]. However, these groves are facing a tremendous risk of disappearing with the permanent stress due to the destructive "Bayoud" disease caused by the soil fungus (Fusarium oxysporum f. sp. albedinis), one of the known diseases in the world that is difficult to control, as well as the prolonged drought and traditional water management in the country. In order to combat "Bayoud" disease, the National Institute of Agronomic Research (INRA) has developed resistant cultivars for date palm trees: "Najda" cultivar, with good fruit quality and resistance to the disease [29]. Despite its good performances with the biotic stress, this cultivar is still very affected by drought stress and in need of more strategies against this abiotic stress.
In a previous study, we have demonstrated the effect of AMF and PGPR bacteria symbiosis on the growth parameters of date palm "Najda" cultivar under drought stress. e present study focuses on the biochemical activity and enzymatic responses of this cultivar under drought stress conditions. While featuring the role of the AMF and PGPR bacteria, symbiosis plays a role in the antioxidant response. To our knowledge, no study has been conducted for date palm "Najda" cultivar under water stress conditions. Plant cells produce different antioxidant enzymes such as catalase (CAT), peroxides (POX), superoxide dismutase (SOD), and glutathione S-transferase (GST) that scavenge the reactive free radicals [30]. In this paper, we studied the effect of inoculation of drought-tolerant plant growth-promoting bacteria Bacillus S48 isolated originally from arid rhizosphere and a complex of 28 different species of AMF isolated from the rhizosphere of a Zagora palm grove on the tolerance of date palm "Najda" cultivar to drought stress in terms of the biochemical status of the plants.

Trap
Culture. Trapping is highly necessary to obtain many healthy spores of colonizing fungi for identification and as inoculum. e trap cultures were prepared as follows: the plant's debris and shoots were removed from the soil samples collected, and the roots fragments were cut into small fragments and mixed with the associated soil. After that, the blend was mixed in 1:1 (v/v) ratio with autoclaved soil and then transferred into plastic pots (13 × 09 cm) with barley seeds (80-100 seeds/pot). Barley (Hordeum vulgare L.) was used as a host plant for the trapping cultures, and the pots were kept in a greenhouse for at least four months before being used.

PGPR Bacteria.
e bacterial strain was isolated from an arid soil in the Saada experimental domains of INRA, Marrakech. It was selected for its beneficial activities to plant growth and health, more precisely for its positive effect on two Moroccan wheat varieties (Triticum durum Desf.) in a previous study conducted in vitro by Chrouqi et al. [31] in the same laboratory.

Mycorrhizal Inoculum Multiplication.
e MF inoculum cannot be produced independently from the plant. Mycorrhizal fungi spores were isolated from different soils and have to be trapped and multiplicated on a host plant. ereby, the AMF inoculation was supplied in the form of barley root segments infected by the above AM fungi complex from the morphological identification. e parameters of barley root infection were calculated after 4 months of culture using the technique stated by Trouvelot et al. [32]. e frequency of infection was approximately maintained at 80% for the barley roots; then they were surface-disinfected for 10 min, rinsed with sterile distilled water thrice for 10 min, and cut into 1-2 mm long fragments to be used as an inoculum based on the method suggested by Strullu et al. [33].

Mycorrhizal Inoculation and Growth Conditions.
e current experiment was conducted at the National Institute of Agronomic Research, Plant Protection Unit, Laboratory of Phyto-Bacteriology, Marrakech, during 8 months of growth in a greenhouse. Seedlings generated from "Najda" seeds were grown in plastic pots (15 × 14 cm) filled with 2 kg of a mixture of sterile sand and peat (2:1 v/v) under total conditions of 16 h light, 60-70% relative humidity, and 25-30°C temperature. e plants were divided into four major groups: control plants (C), plants inoculated with AMF (M), plants inoculated with AMF + PGPR bacteria (M + B), and plants inoculated with PGPR bacteria only (B), with 10 plants in each treatment. Two grams of fresh weight of barley root fragments was applied to the plant roots as an inoculum. After 2 months of growth, the bacterial suspension was added to the M + B and B treatments. e control plants were grown under the same conditions, without either the barley root fragments or the bacterial suspension.

Bacterial Inoculation.
e bacterium Bacillus genus was extracted from the wheat rhizosphere grown in INRA's Saâda experimental domain, Marrakech. is bacterium was found to be the most effective PGPR strain with different multiple plant growth-promoting activities as described by Chrouqi et al. [31]. Bacterial suspensions were prepared as specified by Mayak et al. [34]. In summary, one bacterial colony was grown on a solid DF [35] medium containing ACC (1-aminocyclopropane-1-carboxylic acid) as a pure source of nitrogen, then inoculated to the YT medium, and finally incubated for 24 h with extensive shaking, approximately 250 rpm, for proper aeration. e bacterial cells were pelleted by centrifugation at 5,000x g for 10 min and then resuspended in distilled water. is was repeated twice to adjust the bacterial concentration at 1.0 absorbance unit at 600 nm. e latter suspension was used to irrigate plants as indicated by Mayak et al. [34].

Water Stress Application.
e date palm plantation was conducted in plastic three liter pots, fitted with a drainage system to remove the excess water, which allows determination of the field capacity (FC) of the soil [36]. Tobar et al. [36] explained the technique for the water stress application. W1 is the first weight of the pot full of dry soil. e same pot was then irrigated to saturation and left to drain under gravity until it reaches a steady weight of W2. e difference between the two weights (W2 − W1) matches the volume needed to obtain 100% FC of the soil used (100% FC). Following this equation (1): (0.75 or 0.50 or 0.25) × (W2 − W1), the volume required for obtaining the weights of the buckets at 75%, 50%, and 25% FC ( W3, W4, and W5) was determined, respectively. All through the experiment, pots were brought back to the weight corresponding to the water treatments imposed (100%, 75%, 50%, or 25% FC) by successive weighing and irrigation. During the experiment, the pots were weighed twice a day in a balance of 70.041 M, 0.1-5 g accuracy, and 30 kg weighing capacity, and the lost water was replaced. For each experimental treatment, four water regimes were applied (100%, 75%, 50%, and 25% FC) with 10 plants in each treatment.

Determination of AMF Root Colonization.
A part of the roots from the lateral root system is properly rinsed from soil Applied and Environmental Soil Science remains, then cleaned using 10% KOH at 90°C for 30 min, acidified afterward with 1% HCl for 10 min, and finely stained with trypan blue at 90°C for 20 min as described by Phillips and Hayman [37]. e evaluation of the mycorrhization parameters was conducted for 30 root fragments of 1.0 cm in length using a Zeiss Axioskop 40 microscope at 40-100x magnification, according to Trouvelot et al. [32]. Two mycorrhizal parameters, the AMF infection frequency (Fa %) and the AMF infection intensity (Ma %), were calculated, as follows: where n5 is the root number with infection level of five (infection rate, 90-100%); n4 is the root number at level four (infection rate, 50-90%); n3 is the root number at level three (infection rate, 10-50%); n2 is the root number at infection level two (infection rate, 1-10%); and n1 is the root number at level one (infection rate, 0-1%).

Measurement of Plant Growth Parameter.
ese measurements were carried out in the laboratory in the same way and under the same conditions. e plants were harvested after 32 weeks of growth, before drying the leaves at 105°C for 24 h to measure dry shoot weight (DW), and the fresh shoot weight (FW) was measured to calculate the parameters related to the plant's water status.

Estimation of Relative Water Content.
e relative water content estimation stated by Boyer [38] is a reliable indicator of the water balance state of the plants and considers not only the differences in the amount of water present in the tissues but also the changes in their capacity to absorb water during the tissue saturation experimental stage. e fresh leaf tissues were weighed to get the fresh weight (FW) before being placed in Petri dishes with water and incubated at room temperature for 24 h. e tissues were later taken out, blotted dry, and weighed to get the turgid weight (TW). Subsequently, the samples were dried at 80°C for 24 h and weighed again to obtain the dry weight (DW). RWC (%) expresses the water content in the sample after harvest at a given time as related to the water content at full turgor (TW): 2.6. Determination of Membrane Permeability. Plant cell membranes play an important role in cell functioning, and they are made of a lipid bilayer with intrinsic or extrinsic proteins. In the event of stress, these membranes will undergo denaturation, which will alter their integrity. Leaf membrane permeability was measured by electric conductivity (EC) as described by Yan et al. [39]. Five discs from a leaf of each sample were removed with a cookie cutter and rinsed in a Petri dish containing distilled water. e discs were then placed in a beaker or tube containing 10 ml of distilled water. e leaf samples were immersed at 30°C for 3 hours, and then the conductivity of the solution was measured for the first time with a previously calibrated conductimeter (C1). en the conductivity was measured for a second time (C2) after placing the sample in a boiling water bath for 20 minutes and then cooled to room temperature. e percentage of electrolyte leakage was calculated as follows:

Estimation of Proline Content.
Proline is a part of the socalled osmoprotective molecules because they have a protective role at the level of proteins, protein complexes, and membranes. e accumulation of proline in leaves, stems, and roots is considered one of the most common induced responses to stress, making it an excellent stress detector. Leaf samples from date palm seedlings were collected for the experiment. Extraction procedure and colorimetric determination were carried out as follows [40]: samples of 1 g leaf fresh weight were ground in a mortar after the addition of a small amount of quartz sand and 10 mL of a 3% (w/v) aqueous sulfosalicylic acid solution.
e homogenate was filtered through two layers of Whatman filter paper. Two millilitres of filtrate was reacted with 2 ml acid ninhydrin and 2 ml of glacial acetic acid in a test tube for 1 hour at 100°C, and the reaction was terminated in an ice bath. Readings were taken immediately at a wavelength of 546 nm. e proline concentration was determined from a standard curve and calculated on a fresh weight basis (µmol proline (g FW) −1 ).

Preparation of Enzyme Extracts.
As previously mentioned, the enzyme extracts used were prepared at the same time as the protein extract and following the same method. erefore, after being immediately frozen in liquid nitrogen and stored at −25°C, the samples were ground, centrifuged, and then used for the assays of enzymatic activities and total protein determination.  [41]. e kinetic evolution of the absorbance at 470 nm was measured for 1 min. e speed of the reaction was recorded after adding a volume v (μl) of the sample at 470 nm, and the initial speed V i was measured in D O /min.

Estimation of Catalase.
e hydrogen peroxide absorbs at 240 nm (E240 � 39.4 L.mM −1 .cm −1 ), and therefore, its transformation in the presence of catalase will be followed by a reduction of the absorbance over time at this wavelength.
Catalase (CAT) activity was assayed spectrophotometrically by monitoring the decrease in absorbance of H 2 O 2 at 240 nm. CAT was measured according to the method of Brennan and Frenkel [42]. e reaction mixture consisted of 0.5 ml of protein extract (0.1 mg total protein/ml) in 1 ml of 50 mM potassium phosphate buffer (pH 7.0) containing 20 mM H 2 O 2 . e reaction speed is recorded after adding a sample volume at 240 nm, and the initial speed V i is measured in D O /min.

Estimation of SOD.
Superoxide dismutase (SOD) includes a transition metal (Fe, Mn, or Cu) at their active site. In the dismutation reaction, the metal ion picks up an electron from the superoxide anion and transfers it to the imidazole nucleus from one of the histidines at the active site. e SOD activity was determined according to the method of Beyer and Fridovich [43], which was measured using spectrophotometry at 560 nm and by monitoring the inhibition of the photochemical reduction of the nitro blue tetrazolium (NBT) by the superoxide anion produced following the photoreaction of oxygen and riboflavin in the presence of an electron donor such as methionine. One unit of SOD activity was defined as the amount of enzyme required for 50% inhibition of the reduction rate of NBT. e reaction mixture consisted of 2. e reaction was then stopped by placing the patch in the dark and at 4°C for about 10 min, and then the absorbance was read with a spectrophotometer. A control was made and placed directly in the dark.
e maximum photochemical reduction of NBT, Amax, is determined from the tubes exposed to light and containing the reaction mixture without enzymatic extract. e percentage inhibition of the photochemical reaction of NBT by SODs was calculated as follows: where Cprot is the protein concentration obtained by the Bradford method (mg/ml), Ve is the volume of the extract, % inh is the percentage inhibition of the formazan formation reaction, Ae is the absorbance of the extract (Abs light -Abs dark), and Ac is the absorbance of control.
2.11. Estimation of Glutathione S-Transferase. Glutathione S-transferase activity is determined based on a continuous spectrophotometric rate determination as previously reported by Habig et al. [44]. Enzyme activity with aromatic substrates was usually determined by monitoring changes in absorbance with a spectrophotometer. A complete assay mixture without enzyme was used as a control. Assays were conducted by mixing CDNB 1 mM and GSH 5 mM prepared solutions with the enzymatic extract. e absorbance reading was conducted every 1 min for 5 min at a wavelength of 340 nm.

Experimental Design and Statistical Analysis.
e experimental design was conducted in a greenhouse experiment design as a complete-block design with four field capacity levels consisting of four treatments (C: control plants; M: plants inoculated with mycorrhizal fungi; M + B: plants inoculated with mycorrhizal fungi and PGPR bacteria; and B: plants inoculated with PGPR bacteria only) with 10 plants in each treatment. All measurements were done in triplicate. Data analysis was carried out by a two-way analysis of variance (ANOVA) followed by Tukey's post hoc tests to evaluate significant differences among the samples at a 95% confidence interval using the SPSS computer program, version 20. 0. e level of significance was p < 0.05.

e Plant Water Status.
Severe water stress conditions (25% and 50% FC) negatively influenced the RWC (Figure 1(a)) and EC in the plants (Figure 1(b)). RWC significantly (p < 0.05) decreased under 25% FC compared with the 100% FC (by 55% for the control treatment). e same decrease (by 32% for the control treatment) was obtained regarding membrane permeability of the plants. AMF and PGPR inoculation resulted in an increase of the RWC and EC parameters of date palm plants compared with the noninoculated plants ( Figure 1) under normal conditions (100% and 75% FC). Under severe water stress conditions (25% and 50% FC), RWC and EC increased in all inoculated AMF and PGPR treatments in comparison with noninoculated plants. Mycorrhizae plants have reached the highest RWC value in severe water stress (25% FC) compared with all the other treatments.

Mycorrhizal Inoculation.
e arbuscular mycorrhizal fungi successfully colonized all the mycorrhizal plants and developed typical intraradical structures such as arbuscules, vesicles, and hyphae. e frequency of colonization (Fa%) reached a value of 96.67% ± 5.774 for the mycorrhizae (M) and a value of 86.67 ± 5.774 for the mycorrhizae + bacteria Applied and Environmental Soil Science (M + B) treatment in a normal water regime (100% FC) ( Figure 2). e results were more satisfying in the severe water stress regime of 25% FC. Fa% reached a value of 76.67% ± 5.774 and 90.00% ± 10.00 for M and M + B treatments, respectively ( Figure 2). As for the intensity (Ia%) of both M and M + B treatments, it increased significantly (p < 0.005) when the soil water deficiency increased, with a value of 81.67% ± 1.528 and 95.00% ± 0.000 in 25% FC for both treatments, respectively (Figure 3). e mycorrhizae + bacteria showed very high values for both Fa% and Ia% of colonization compared with M treatment regardless of the water stress regime.

Proline.
e proline content significantly increased under severe water stress conditions (25% and 50% FC) compared with well-watered conditions (100% and 75% FC) regardless of the treatments applied ( Figure 4). However, the results also indicated that single inoculation either with the AMF species or with PGPR significantly increased the proline content of date palm seedlings compared with the control plants in severe water stress conditions. e maximum proline content was obtained in plants inoculated with the AMF species and PGPR (combined) under severe water stress conditions (25% and 50% FC) reaching a value of 2.588 ± 0.034 in 25% FC compared with 0.978 ± 0.024 for the control. In normal irrigation conditions (100% and 75% FC), there is no significant effect on the proline accumulation with the application of the mycorrhizal and bacterial treatment compared with the control.

Antioxidant Enzyme Activities.
e SOD activity in plants leaves significantly (p < 0.01) increased under severe water stress conditions (25% and 50% FC) compared with well-watered conditions (100% and 75% FC) (by 208%) (Figure 5(a)). Furthermore, bacteria inoculated plants demonstrated a higher SOD activity with a maximum value of 203,985 ± 14,042 in severe water stress conditions (25%) compared with the control. However, the results showed a decrease in the SOD activity with the application of mycorrhizae alone or combined with PGPR in severe water stress conditions compared with the control plants.
An elevated leaf CAT activity was observed in date palm plants under severe water stress conditions (25% and 50% FC) compared with well-watered conditions (100% and 75% FC) (by 208%) (Figure 5(b)). e mycorrhizae and mycorrhizae + bacteria treatments showed a decrease in leaf CAT activity during water stress conditions, and the mycorrhizae plants had lower leaf CAT activity than that of all the other treatments applied during the same conditions. e same pattern was observed for the leaf POX activity ( Figure 5(c)), while it increased with the application of severe water stress conditions in all of the treatments, it decreased with the application of mycorrhizae, Vertical bars represent the standard deviation (n � 3). Bars with different lowercase letters indicate significant differences between treatments at the same FC (p < 0.05). Bars with different uppercase letters indicate significant differences in the same treatment at different FC percentages (p < 0.05). mycorrhizae + bacteria, and bacteria treatment compared with the control and despite the application of the severe water stress conditions. e results showed an increase in the GST activity with the application of severe water stress regime in all of the treatments (Figure 5(d)). In the normal irrigation conditions, the GST activity increased with the application of mycorrhizae, mycorrhizae + bacteria, and bacteria treatments, while in stressful conditions, the GST activity decreased with the application of mycorrhizae, mycorrhizae + bacteria, and bacteria compared with the control.

Discussion
In general, date palm plants are expected to be droughttolerant, with a high yield potential under drought stress since they grow in arid and semiarid regions; however, actually, drought is a major limiting factor in date cultivation, making irrigation necessary, especially at an early stage of the plantation. Although these crops are known for their resistance to drought, their development is strongly impacted by variations in water availability and soil water content [29]. ere are many agrophysiological parameters to evaluate drought stress in a plant (leaf area index, stomatal conductance, water potential, etc.) [45]. In this study, the leaf's relative water content (RWC) and the membrane permeability (EC) were used to evaluate the water status of the plants. e leaf's RWC is a significant predictor of water status in the plants since the balance between water supply to the leaf and transpiration rate can be more accurately expressed by the RWC's direct relation to cell volume [46]. e membrane permeability has long been considered a measure of the action of various stresses; it has often been used for screening against drought stress tolerance in different crops such as wheat [47], maize [48], and rice [49]. e parameters related to the plant's water status are represented in Figure 1. Leaf's RWC and membrane permeability (EC) were significantly (p < 0.05) higher in the plants treated with mycorrhizae and mycorrhizae + bacteria regardless of the water regime applied compared with their respective controls. In the same context, the application of severe water stress decreased the value of both leaf's RWC and EC regardless of the treatment of the plants, with the reduction being stronger in control plants than in the treated ones. Similar results were found by Faghire et al. [50] who reported that, with decreasing irrigation, RWC significantly decreased in nonmycorrhizal than in mycorrhizal seedlings. In fact, RWC was 4% higher in mycorrhizal seedlings than in nonmycorrhizal seedlings. Bacteria treatment only slightly improved the RWC in normal conditions (100% and 75% FC) compared with the control; however, under stressful conditions, the bacterial inoculation did not enhance the RWC of the plants compared with the control. is could be due to the fact that bacteria did not interact directly with the plants but with another indirect mechanism, such as increasing root cell permeability by the bacteria for AMF colonization, thereby positively influencing the physiology of plants.
e positive effect of the mycorrhizal inoculation on the plant's water status that was shown in our results (Figure 1) could be explained by the creation of a mycorrhizal hyphal network that provides access to more nutrients and water to pass to the plants, thereby increasing their water absorption [51]. Furthermore, Jones [51] also mentioned that the absorptive region of mycorrhizal hyphae is about 100 times more efficient than root hair, which might justify the accessibility of more water for the plants and the high RWC value of the leaf.  Several researchers have noticed that AMF can improve plant resistance to water deficiency [52][53][54], primarily due to the capacity of mycorrhizal roots to increase water conductivity [55]. ere are opposed findings about the dual impact of AMF and PGPR inoculation on the plants [56][57][58]. However, some reports support the beneficial results obtained in the current study. For instance, Aalipour et al. [59] suggested that PGPR and AMF were successful in enhancing the activities of both communities in the rhizosphere. ese synergistic relationships between PGPR and AMF can increase the plant water absorption and nutrient assimilation under water stress conditions and reduce the negative stress impacts on plant growth and development, which is demonstrated in this study using the mycorrhizal inoculation parameters (Figures 2 and 3). e complex of mycorrhizal fungi showed a good capacity to infect the roots of date palm plants in nonstressful conditions; infection parameters such as the frequency and intensity of these mycorrhizal fungi were hardly affected by the application of severe water stress (25% FC).
Under stress conditions, especially drought and soil salinity, plant's proline is considered a fundamental osmoregulation solute. In fact, the accumulation of this amino acid may be a form of an adaptation to harsh environmental conditions, as reported by several researchers [14,[60][61][62]. In this study, leaf proline concentration was affected by both the severe water stress conditions and the treatment applied to the plants (mycorrhizae, mycorrhizae + bacteria, and bacteria) (Figure 4). When faced with oxidative stress, the best biochemical response of plant cells is the accumulation of osmolytes, like proline, in order to enhance osmosis and prevent dehydration. is explained the sudden increase of this molecule in our results ( Figure 4). Comparable with our findings, an increase of proline accumulation in response to abiotic stress was reported in different studies [59,[63][64][65][66]. From these results, it can be concluded that the accumulation of proline under severe water stress conditions (Figure 4) was likely a general response of date palm to water stress conditions as an osmotic regulator. e proline content was higher in the dual inoculated plants than in separate inoculated plants.
e mycorrhizal and bacterial inoculation may be the reason behind the proline accumulation in the leaves of the host plant. As a way of enhancing the defence mechanism of the plants, this inoculation increases the proline metabolism, thus a better osmotic adjustment [67]. Ortiz et al. [68] conducted a study on Trifoliumrepens plants inoculated with both PGPR bacteria and mycorrhizae under drought stress conditions. ey showed that the greatest proline accumulation in shoots was found in plants dually inoculated with PGPR bacteria and mycorrhizae. Proline accumulation is a mechanism of resistance to abiotic stress by adjusting intracellular osmotic pressure. ese results are in agreement with the works of Cherif [69] who reported that inoculation with Bacillus sp. and Pantoea agglomerans strain helped improve salt stress tolerance of wheat. is result does confer with ours under water stress conditions. Overall, the enhanced proline accumulation found in most dually inoculated plants resulted in a decrease in the osmotic cell potential, thereby increasing water absorption to preserve osmotic balance. It is a sign of the elevated osmoprotective potential and the ability to sustain the plant water status in inoculated plants under severe water stress conditions. It has been previously reported that proline can act as a chemical protein chaperone and prevent protein aggregation under water stress [70]. e enhancement of proline in plants treated with both AMF and PGPR helped to protect against oxidative stress compared with single inoculation since it is involved in the stabilization of redox enzymes. Also, this synergic relationship may be due to the bacterial effect on AM fungal germination, which leads to better mineral nutrition, facilitating the plant's growth promotion through the AM association. Anjum et al. [71] reported that the exogenous application of proline to cell cultures was positively correlated with the increased activity of different antioxidant enzymes (SOD, CAT, and POD enzymes) under water stress conditions. Some new insights into the regulation of plant immunity by amino acid metabolic pathways have been reported by Zeier. Hence, co-colonization by PGPR and AMF may lead to synergistic levels of immune priming in AMF-responsive plants. Moreover, when plants are under water stress conditions, inoculation with AMF and PGPR helps trigger proline gene expression and enzyme accumulation preventing cell death.
is study mainly focused on the oxidative responses of date palm seedlings inoculated with mycorrhizae and PGPR bacteria during water stress conditions. e results of the present study clearly showed the beneficial effects of AMF and PGPR bacteria inoculation in protecting plant cells.
However, plants tried to cope with the challenge through several mechanisms, such as the production or activation of antioxidant enzymes. e enzymes SOD, CAT, POX, and GST are among the main natural "detoxifiers" produced by the plants. ey counteract the generation of the reactive oxygen species (ROS) and scavenge them in order to avoid the destruction of the cell membranes and oxidative damage inside the cells. ese enzymes have been documented in many research works as a defence mechanism against biotic and abiotic stresses [1,[72][73][74][75]. During normal conditions, the amount of ROS in the plant cells is kept under control by the antioxidant enzyme scavenging activity. However, this balance is disturbed in stressful conditions, causing the intracellular ROS levels to increase [76]. is leads to the application of new methods to help the plants cope with these imbalances. Numerous research works have highlighted the effect of mycorrhizae and PGPR bacteria on improving plant resistance, productivity, and metabolism under normal and stressful environments [77][78][79][80][81][82][83]. erefore, to evaluate the effect of mycorrhizal and bacterial inoculation accurately during the application of different irrigation conditions (100%, 75%, 50%, and 25% FC), the enzymatic activity of SOD, CAT, POX, and GST was measured and is represented in Figures 5(a)-5(d). Contrary to Alguacil et al. [84] who found that, during water stress conditions, the Juniperusoxycedrus L. plants inoculated with AMF mixture expressed a higher SOD activity than noninoculated plants, Chang et al. [85] have reported that mycorrhizal Elaeagnus angustifolia L. seedlings had a higher leaf SOD activity than that of the nonmycorrhizal seedlings during salt stress conditions. e higher SOD activity expressed in the control and bacteria plants leads to the hypothesis that the noninoculated plants and plants with only bacterial inoculation were more sensitive to water stress than mycorrhizae or mycorrhizae + bacteria treatments. erefore, they enhanced SOD activity earlier than the other treatments.
Drought stress caused a significant increase in the leaf CAT activity of the control and bacteria treatments ( Figure 5(b)). From these findings, it can be concluded that the mycorrhizae and mycorrhizae + bacteria treatments decreased the leaf CAT activity in the date palm seedlings during severe water stress conditions. e same pattern was observed for the leaf POX activity (Figure 5(c)). Glutathione is the main category of antioxidants enzymes with a wide variety [86]. GST in plants plays an important role in the regulation of hormonal balance, herbicide detoxification, and plant senescence control in response to various abiotic stresses.
Considering the fact that H 2 O 2 accumulation inside the plant cells triggers CAT and POX activity and that H 2 O 2 is a product of SOD activity, a correlation between the activities of these enzymes can exist [87,88]. Low CAT and POX activity along with reduced SOD activity in both mycorrhizae and mycorrhizae + bacteria treatments than in control plants under severe water stress conditions can confirm that both mycorrhizal symbiosis and its combination with PGPR bacteria can alleviate plant oxidative stress. is agrees with previous results, in which Kohler et al. [89] found that Applied and Environmental Soil Science Glomus intraradices, alone or in combination with Pseudomonas mendocina, caused a significant decrease in SOD activity in plants grown under drought conditions. is reduction in antioxidant enzymes can be interpreted in part by the fact that these plants could have been less sensitive to oxidative stress under water stress conditions. Otherwise, this is the first research to show the influence of both mycorrhizae and PGPR on POX, SOD, CAT, and GST activities of date palm plants grown under extreme drought conditions for "Najda" cultivar.

Conclusion
is study demonstrated the role played by the mycorrhizal and PGPR bacterial inoculations in reducing the damages of the oxidative stress in date palm plants at an enzymatic level.
e results above supported that abiotic stress can negatively affect plant growth and development. However, this effect of stress on plant growth may be mitigated and/or reduced by the rhizosphere living microorganisms including bacteria and mycorrhizal fungi, applied individually or in combination. e enhanced resistance of the mycorrhizal fungi/ bacteria symbiosis in the date palm seedlings (Najda cultivar) during water stress conditions, in comparison with control plants, was affiliated with several biochemical characteristics such as better water absorption in normal and drought conditions, and improved the enzymatic response of the plants which improves the total health of the date palm plants. is can serve as a biological strategy for better crop production of plants exposed to severe water stress conditions, especially in arid and semiarid regions. erefore, introducing the mycorrhizal and bacterial inoculations to these plantations can enhance the yield and production with less water consumption. However, since the experience was conducted under greenhouse conditions, it remains limited to a specific environment and leads towards a field experiment to better understand the effect of the biofertilization on date palm and its effect on the growth and the development of the plants.

Data Availability
e data used to support the findings of this study are included within the article.

Conflicts of Interest
e authors reported no potential conflicts of interest.