An Evaluation of Aluminum Tolerant Pseudomonas aeruginosa A7 for In Vivo Suppression of Fusarium Wilt of Chickpea Caused by Fusarium oxysporum f. sp. ciceris and Growth Promotion of Chickpea

Chickpea wilt, caused by Fusarium oxysporum f. sp. ciceris, is a disease that decreases chickpea productivity and quality and can reduce its yield by as much as 15%. A newly isolated, moss rhizoid-associated Pseudomonas aeruginosa strain A7, demonstrated strong inhibition of Fusarium oxysporum f. sp. ciceris growth. An in vitro antimicrobial assay revealed A7 to suppress the growth of several fungal and bacterial plant pathogens by secreting secondary metabolites and by producing volatile compounds. In an in vivo pot experiment with Fusarium wilt infection in chickpea, the antagonist A7 exhibited a disease reduction by 77 ± 1.5%, and significantly reduced the disease incidence and severity indexes. Furthermore, A7 promoted chickpea growth in terms of root and shoot length and dry biomass during pot assay. The strain exhibited several traits associated with plant growth promotion, extracellular enzymatic production, and stress tolerance. Under aluminum stress conditions, in vitro growth of chickpea plants by A7 resulted in a significant increase in root length and plant biomass production. Additionally, hallmark genes for antibiotics production were identified in A7. The methanol extract of strain A7 demonstrated antimicrobial activity, leading to the identification of various antimicrobial compounds based on retention time and molecular weight. These findings strongly suggest that the strain’s significant biocontrol potential and plant growth enhancement could be a potential environmentally friendly process in agricultural crop production.


Introduction
Chickpeas (Cicer arietinum L.) are considered to be one of the oldest legumes known from ancient times. Most likely, it originated in southeastern Turkey and Syria's adjacent areas [1]. Globally, it is a valuable crop and about 2.3 million tons enter the world market annually [2]. The major chickpea legume grain-producing regions are in southern and South-Eastern Asia, Africa, and Australia, [2].
It is estimated that India produces 9.075 million tons of chickpeas annually, accounting for 65% of the total production of chickpeas. The remarkable growth of chickpea pulse has been documented in India, comprising the most significant production (47%; 10.90 MT) among all pulse crops in 2019-2020 [2]. Chickpeas are sustainable legumes with nutritional value for human and animal consumption as well as soil fertility. Chickpeas seeds and leaves are an excellent source of carbohydrates, vitamins, fibers, and proteins. Chickpeas play a leading role in food safety in the world by supplying the protein deficit of daily food rations [3]. Chickpeas-based diets are recommended to combat lifestyle disease since they contain several essential minerals such as calcium, phosphorus, iron, and zinc among other substances, including phenolics and oligosaccharides [3]. There are numerous living and bioavailability and nutrient as well as Al uptake in crop plants under acid soil conditions [43]. Pseudomonas plecoglossicida Pp20 strain ameliorates damages on maize roots induced by aluminum chloride (AlCl 3 ) at a concentration of 90 µM by producing the plant growth-promoting hormone indole-3-acetic acid (IAA) and ethylene degrading enzyme, 1-aminocyclopropane-1-carboxylic acid (ACC) deaminase [44]. Apart from the production of phytohormones, the PGPB may evolve diverse mechanisms such as mineral solubilization, the development of siderophores (metal-chelating compounds), inhibiting metal transport in the roots, reducing lipid peroxidation and hydrogen-peroxide production, and sustained enhancement of antioxidant enzymes in the plants [41][42][43][44][45]. Few reports are available for chickpea metal tolerance using PGPB under salinity and metal (Mn) toxicity conditions [46,47]. Combining endophytic bacteria (Stenotrophomonas maltophilia), mycorrhizal fungi, and ferrimagnetic magnetite (Fe 3 O 4 ) nanoparticles induced Rhizobium improved chickpea (Cicer arietinum L.) nodulation, leg hemoglobin content, nitrogenase activity, and growth by mitigating salt and metal stress and improving nutritional status of plants at salinity levels 75 and 150 mM [47]. However, no attempt has been made to employ PGPR inoculation to mitigate Al stress in chickpea plants growing in acid soil with high Al levels. The current study reports on the identification and characterization of a Pseudomonas aeruginosa strain A7 isolated from rhizoids of Polytrichum sp. from a waste disposal area. We report its biocontrol potential against phytopathogens and characterize its abilities to produce plant-growth promotion-related compounds such as indole-3-acetic (IAA), ammonia, siderophores, hydrogen cyanide (HCN), cellulase, chitinase, pectinase, proteases, the ability to solubilize tri-calcium phosphate, potassium, zinc oxide and can tolerate different abiotic stress conditions. The strain A7 enhanced the chickpea growth in aluminum stressed conditions and acts as a potential biocontrol agent to Fusarium wilt disease of chickpea caused by Fusarium oxysporum f. sp. ciceris (Foc). Adult moss plants identified as Polytrichum sp. were collected from a waste disposal area at Cachar Paper Mill Panchgram, Hailakandi, (Assam), India. Approximately 10 g of tiny rhizoids of the moss adhering with soil were cut out and mixed with 90 mL phosphatebuffered saline (PBS) (HiMedia, Mumbai, India) in a conical flask. The flask was kept in a rotary shaker incubator at 150 rpm at 30 ± 2 • C for 60 min. Following shaking, the suspension was serially diluted to a factor of 10 −6 with Phosphate-buffer-saline (PBS) buffer and plated on King's Base agar medium (KB) (HiMedia, Mumbai, India) plates supplemented with aluminum (AlCl 3 , SD Fine Chemicals, Mumbai, India) and incubated for 2 days at 30 ± 2 • C [48,49]. On the plates, bacteriologically distinct colonies were selected for further purification. Pure strains were preserved at −80 • C in 20% glycerol [50]. A strain designated A7 was studied for its morphological characteristics, such as color, shape, size, elevation, and surface. The fluorescent activity of the colonies that appeared under ultra-violet (UV) light on the plates was evaluated after 24 h by re-inoculating them on the KB plate. The strain was processed through different biochemical characterizations such as catalase, citrate utilization, indole synthesis, methyl red generation, nitrate reduction, starch hydrolysis, urease, Voges-Proskauer, and hydrogen sulfide (H 2 S) production was achieved using KB003 Hi25TM Enterobacteriaceae identification Kit (HiMedia, Mumbai, India) [51].

Molecular Identification of the Strain
The 16S rRNA-encoding gene sequencing-based molecular identification of the strain was performed using total genomic DNA [52]. For the amplification of the 16S rRNA gene fragment, the fD1 (5 -GAGTTTGATCCTGGCTCA-3 ) and rP2 (5 -ACGGCTACCTTGTTACGACTT-3 ) primer set was used [53]. Polymerase chain reaction (PCR) mixture (50 µL) contained 50 ng of genomic DNA template, 0.5 µM of each of the primers, 200 µM of dNTPs, 1X-High-Fidelity buffer, 1U of Phusion High-Fidelity DNA polymerase enzyme (Thermo Scientific, Waltham, MA, USA). The polymerase chain reaction amplification was performed using a C1000 Touch Thermal Cycler (Bio-Rad, Hercules, CA, USA) with cycle conditions of initial denaturation at 98 • C for 30 s, 35 cycles of initial denaturation at 98 • C for 10 s, 50 • C (annealing) for 30 s, 72 • C (extension) for 1 min 30 s, and a final extension of 72 • C for 7 min. Gel electrophoresis was performed on the amplified products using 1.5% agarose and Tris-Acetate-EDTA (TAE). The PCR product was purified using a QIAquick PCR purification kit (Qiagen, Hilden, Germany). The restriction enzyme EcoRV (NEB, Ipswitch, MA, USA) cut plasmid vector pLitmus28 (NEB, Ipswitch, MA, USA) and 16S rRNA DNA was blunt ligated with T4 DNA ligase (Thermo Scientific, Waltham, MA, USA) to clone the PCR product. Electrocompetent E. coli TOP10 cells (Thermo Scientific, Waltham, MA, USA) were prepared and transformed with a ligation mix using a Gene Pulser (Bio-Rad, Hercules, CA, USA), following the standard protocol [54]. Using the corresponding primer set, colonies on Luria Bertani (LB) agar fortified with Ampicillin 100 µg mL −1 were selected and confirmed by colony PCR and plasmid DNA was isolated. An EcoRI restriction digestion (Thermo Scientific, Waltham, MA, USA) was performed to obtain the product of the desired size of 4.3 kb. The recombinant DNA products were purified further using PEG 8000 (Sigma Aldrich, Bangalore, India) and sequenced commercially. Two reads of the amplicon sequencing were assembled and analyzed using Chromas Pro version 2 (http://technelysium.com.au/wp/chromaspro/, accessed on 25 July 2020). To identify the strain, a blastn analysis was performed by comparing the derived gene sequence to known bacterial 16S ribosomal RNA gene sequences obtained from the NCBI GenBank website (https://www.ncbi.nlm.nih.gov/, accessed on 25 July 2020). A phylogenetic analysis was performed with the Maximum Likelihood method with 1000 bootstrap replications using MEGA version 6.0 software (https://www.megasoftware.net/, accessed on 25 July 2020) [55]. This nucleotide sequence was submitted for inclusion in GenBank under accession number MN197639.

In Vitro Antagonistic Activity of the Strain A7
To assess the in vitro antimicrobial activity, plant pathogenic fungal strains Rosellinia arcuata Petch (Rap) ( The in vitro antifungal activity of strain A7 was performed using a concentric ring bioassay [56]. In the center of the Potato-dextrose Agar (PDA) plate, a 6 mm diameter mycelium disc was cut from the margin of a 4-day-old PDA grown fungal mycelium and placed. The bacterial strain was inoculated surrounding the fungal disc in a concentric ring manner with the help of a sterile funnel. As a control, a fungal disc without a concentric ring of bacteria was employed. The percentage of inhibition was calculated after 2 to 7 days of growth suppression at 30 • C, depending on the pace of growth. Using the formula below, the percentage of growth inhibition (PGI) of the fungal pathogen by the strain was calculated.
The dual-culture assay was used to produce antifungal volatile organic compounds (VOCs) [57]. A King's B agar plate was streaked with strain A7, and a fungal mycelium disc was placed onto the center of the PDA plate. Parafilm was used to seal both inoculation plates [58]. However, it should be emphasized that the Petri dishes create a gap in the growth media, preventing the nonvolatile exudates secreted by A7 from reaching the fungus. KB plates spread with sterile distilled water and the fungal disc on a PDA plate sealed with parafilm was considered a control. The growth inhibition was determined after 2 to 7 days at 30 ± 2 • C, depending on their growth rate and the percentage of growth inhibition was recorded. The percentage of growth inhibition (PGI) of the fungal pathogen by the strain was calculated as: where D c is the pathogen's growth rate in the absence of strain A7, and D t is the pathogen's growth rate in the presence of strain A7.
In vitro antifungal and antibacterial activities by the strain A7 with the cell-free supernatant (CFS) were completed by Agar-well diffusion and the Agar disk-diffusion method [59]. To establish the stationary phase cultures, A7 was cultured on KB broth for 2 days at 30 • C. The cell-free supernatant of the strain A7 was collected by centrifugation at 13,000 rpm for 10 min at 28 • C. To eliminate any debris, CFS was filtered using a 0.2 µM membrane filter (Millipore) and was ready to use [60]. Antifungal activity by using CFS was performed by inoculating a fungal disc at one edge of the PDA plate. A rectangular well was prepared at another edge using a sterile scalpel and a volume of 100 µL of CFS was introduced into it. The Petri dishes were incubated for 48 h at room temperature. The CFS was diffused into the medium and the growth of the fungal pathogen was inhibited and measured as above.
Antibacterial activity using the CFS of the strain A7 on KB agar plates was performed by inoculating freshly grown bacterial pathogens (0.1 optical density at 600 nm, OD 600 ) by streaking. Then, on both ends of the agar surface, filter paper discs (6 mm in diameter) were inserted and labeled accordingly (i) filter paper disc with 50 µL CFS, (ii) filter paper disc with 50 µL sterile double distilled water as control. The Petri dishes were incubated at 30 ± 2 • C for a day. CFS was diffused into the medium and the germination and growth suppression of the respective pathogen was calculated by measuring the diameters of the zone of inhibition [61]. All assays were performed in three biological replicates.

Plant Growth-Promoting (PGP) Activities of the Strain A7
The strain's plant-growth-promoting activities were assessed qualitatively using a plate-based assay and quantitatively using a liquid assay. Luria-Bertani (LB) agar plates amended with 5 mM L-tryptophan (SRL, Mumbai, India), Sodium Dodecyl Sulfate (SDS, 0.06%), and glycerol (1%), was used to detect Indole-3-Acetic acid (IAA) production. To obtain a colony with a diameter of 0.2-5 mm, the plates were incubated for 24 h. After that, the Petri dishes were covered using Whatman no.1, filter paper, and incubated for another 24 h. The filter papers were removed after the incubation period, saturated with Salkowski reagent (4 mL prepared using 2% of 0.5 M Ferric III Chloride in 35% of Sodium hypochlorite), and studied at 30 • C for 1 to 2 h until appropriate color development. The development of the red halo zone around the colony on the filter paper was considered a positive IAA producer [62]. IAA production was also performed quantitatively by inoculating the strain on the LB broth using Salkowski reagent with a 48 h time interval of 196 h. The absorbance was measured at 530 nm after the development of the pink color. Using the IAA standard (LobaChemi, Mumbai, India), the concentration of the generated IAA was measured [62]. Phosphate was solubilized on Pikovskaya's (Pkv) agar (HiMedia, Mumbai, India), using the method outlined in [63]. Quantitative estimation was performed on the Pkv broth medium by the method described [64]. Briefly, 25 mL Pkv broth was inoculated with A7 and incubated at room temperature for 4 days. Additionally, 1 mL of the bacterial cell-free supernatant prepared by centrifuging at 30 min at 12,000 rpm, (Eppendorf Centrifuge 5804R, Eppendorf, Hamburg, Germany) was mixed with 10 mL chloromolybdic acid, and 35 mL of distilled water was added. The volume was then increased by adding chloro-stannous acid (0.25 mL). The total volume of 50 mL was maintained by adding distilled water. The absorbance was measured at 600 nm of the developing blue solution. The quantity of soluble phosphorus was determined us-ing the KH 2 PO 4 standard curve (Sigma Aldrich, St. Louis, MO, USA). A modified plate assay was used to determine the solubilization of the potassium [65] by inoculating the strain A7 on Aleksandrov agar medium mixed with Bromothymol Blue (an acid-base indicator dye) [66]. The Petri dishes were incubated at room temperature for 7 days. An improved visibility solubilization halo zone on the agar plates was positive for potassium solubilization. The formula for calculating the solubilization efficacy (SE) was as follows: SE = [the diameter of A7/the diameter of the halo zone] * 100 [67]. By inoculating the strain on zinc oxide agar medium plates and incubating them at 30 • C for seven days, zinc oxide solubilization was measured qualitatively [68]. The above formula was used to compute the solubilization efficiency. The strain A7 s ability to fix atmospheric N 2 was investigated using the nitrogen-free broth (Nfb) medium described [69]. At 30 • C, the plates were incubated for 24 h. After the incubation period, the medium's color changed from pale green to blue, indicating the isolate's ability to fix N 2 . Ammonia was produced by growing A7 on peptone water (10 mL) in each falcon tube and incubated for 2 to 3 days at 30 ± 2 • C. Following incubation, 500 µL of Nessler's reagent was added to each tube. Brown to yellow color development was taken as a positive test for the production of ammonia [70]. Chrome Azurol S (CAS) assays were used for siderophores production [71]. The freshly prepared CAS solution was added to the KB agar medium as a 1:15 ratio and sterilized by autoclaving. Plates inoculated with A7, showing an orange halo zone surrounding the colony at 30 ± 2 • C for 3 days of incubation, were considered positive for siderophores production, and the diameter of the colored zone was recorded. The A7 was inoculated on a 20 mL KB medium and incubated at the above-mentioned parameters to determine the production of siderophores. Centrifugation at 3000 rpm for 5 min was used to remove the cells. Furthermore, 3 mL of cell-free supernatant, 300 µL of 5N hydrochloric acid solution, 1.5 mL of Arnow's reagent, and 300 µL of 10N NaOH were mixed. The formation of a pink color was noticed after 10 min and recorded. The KB medium amended with 4.4 g of glycine/L was used to test the production of HCN using the strain A7. The socked filter paper (Whatman no. 1, Ankleshwar, India) on 2% Na 2 CO 3 in the picric acid solution (0.5%) was kept on top of the Petri dishes. The dishes were packed with black paper after sealing with parafilm and incubated at 30 ± 2 • C for 4 days. HCN production was detected by the hue changing from yellow to red brown [72]. The chitinolytic activity was assayed on the chitin agar plate, as described by [73] with some modification. In Petri dishes, the lukewarm medium was poured and was allowed to harden. The A7 was inoculated onto the medium and incubated at 30 • C, where it was monitored for the formation of a purple halo zone surrounding the colony, and the measurement of the purple halo was recorded. The polyamine production using A7 was tested by streaking on a Long Ashton Decarboxylase (LAD) agar [74] for 7 days, the Petri dishes were incubated in the dark at room temperature. The strain's arginine decarboxylation was represented by red halos on a yellow backdrop. The extracellular enzymatic activity of strain A7 was using different modified plate-based methods. Cellulase and xylanase activity was estimated by inoculating the strain on Congo-red gelatin agar medium supplemented with 0.5% Carboxymethylcellulose (Na-CMC, Sigma Aldrich, St. Louis, MO, USA) and xylan (Beechwood Xylan, Sigma Aldrich, St. Louis, MO, USA), respectively [75]. The Petri dishes were incubated for 3 to 7 days at room temperature. Bacterial colonies stained with congo-red were thought to be cellulose and xylan degraders [76]. The positive strain's degrading potential was also measured qualitatively by equating hydrolysis capacity (HC). HC = Ratio of the halo zone diameter to the colony diameter [77]. The ligninolytic activity was observed using a Minimal Salt Medium-Kraft Lignin (MSM-KL) medium containing 0.5% Alkali lignin (Sigma Aldrich, St. Louis, MO, USA) supplemented with Methylene blue as the lignin polymeric dye and incubated at 30 ± 2 • C for 3 to 7 days. The strain possesses ligninolytic enzymes that undergo the oxidation of indicator dye. The plates were checked daily for bacterial growth and Methylene blue dye decolorization [78]. Pectinase production was estimated by inoculating A7 on an MM Pectin agar medium supplemented with 0.5% Citrus Peel Pectin (Sigma Aldrich, St. Louis, MO, USA) [79]. The Petri dishes were incubated for 2 days at room temperature and flooded for 15 min with a 5.0% (w/v) iodine solution (LabChem, India) to detect the halo zone around the colony, which shows the strain's ability to produce pectinase. Proteases activity was performed by inoculating A7 on a Skim milk agar medium supplemented with 0.5% skim milk (Sigma Aldrich, St. Louis, MO, USA) and tested positive by the development of a distinct halo zone around the colony [80]. The above-mentioned formula was used to calculate the semi-quantitative enzyme production. The growth profile of strain A7 was checked to tolerate an increasing concentration of aluminum (AlCl 3 ) (0-4 mM) and other metal compounds using the Single Plate Serial Dilution Spotting (SP-SDS) method on modified M9 agar plates [80]. The liquid culture was in the M9 broth supplemented with 0.1% proteases peptone. Similarly, the effect of Fe (III) from 0-5 mM, Fe (II) from 0-3 mM, NaCl (0-8%) (Sigma Aldrich, St. Louis, MO, USA) [81], pH (1)(2)(3)(4)(5)(6)(7)(8)(9)(10)(11)(12)(13)(14) and temperature (4-50 • C) was checked in three biological replicates [82,83]. Freshly grown bacterial cells (0.1 OD 600 ) were serially diluted from 10 −1 to 10 −6 , and 3 µL from each dilution was inoculated into the demarcated areas of SP-SDP and in a 10 −1 dilution in a 50 mL broth. The Petri dishes were incubated for 18-48 h, and the flask was held in an orbital shaker at 160 rpm at 30 ± 2 • C for 48 h. The optical density of the cultures was taken at 600 nm (PerkinElmer UV/VIS spectrometer Lamda 25, USA). The relative growth (RG) was calculated using the formula [84]. Relative Growth (%) = A t /A c * 100, where A c = optical density of the average of three biological replicates of controls, and A t = optical density of average three biological replicates of the treatments. Bacterial 20% and 50% growth inhibitory concentration (IC) IC 20 and IC 50 values were calculated using the dose-response data.

In Vitro Protective Effect of Strain A7 on Aluminum Toxicity in Chickpea Growth
For the in vitro protective effect of strain A7 against aluminum toxicity in chickpea, growth was verified using the jar method [36]. An adequate quantity of chickpea seeds (Pusa-362) was surface-sterilized for 3-5 min in a 0.1% HgCl 2 solution followed by 6-7 washing with sterilized distilled water. The seeds were saturated in water for 12 h after which they were kept on moisten filter paper placed within a Petri dish for germination at 28 ± 2 • C for 72 h. The healthy germinated seeds of equal root and shoot length were transferred into a plastic jar filled with 400 mL of Hoagland nutritive solution (HiMedia, Mumbai, India). Over a 14 h photoperiod, plantlets were cultivated in a plant-growing room in white light with a photon flux intensity of 220 mol m −2 s 1 (PAR). The Hoagland nutritive solution changed every 48 h to maintain the seedlings proper growth. These plantlets were then pretreated with 500 µM CaCl 2 (pH 5) for a day. The growth of strain A7 was previously checked on different concentrations of CaCl 2 (100, 200, 500, and 1000 µM). After one day, the pretreated seedlings were transferred to an experimental setup (1) T 0 = Control (with no bacteria and no aluminum), (2) T 1 = AlCl 3 (only 100 µM of aluminum chloride), (3) T 2 = A7 (only 0.1 OD 600 cells of the bacterial strain) and (4) T 3 = A7 + AlCl 3 (0.1 OD 600 cells of the bacterial strain + 100 µM of aluminum chloride) for 12, 24, 36, 48 h. The root length and shoot length, root fresh weight and dry weight, and relative root length rate (RRL) were all assessed to determine total growth and biomass. Four plants from each treatment were randomly selected and root shoot length was measured. For plant biomass measurements, four plants were grouped to measure the fresh weight and were dried at 80 • C for 48 h, weighing the dry biomass. Seed vigor index (SVI) [85] and relative root length (RRL) rate [36] were calculated using the formulae: RRL = (Root length in aluminum stress conditions) / (Root length in control conditions) × 100

Control of Fusarium Wilt of Chickpea by Strain A7 in Pot Assay Experiment
The chickpea seeds of variety (Pusa-362) were collected from Krishi Vigyan Kendra, Hailakandi, Assam, India, and were used in the pot experiments. The variety Pusa-362 was tested for Fusarium wilt-disease control in pot and field experiments using bacterial biocontrol agents [86]. Fusarium oxysporum f. sp. ciceris (Foc) conidia were prepared by inoculating the pathogen onto the PDA medium incubated at room temperature for 8 days. For a healthier spore suspension, actively growing margins on the culture media plate was removed and 4 to 5 mL sterile dH 2 O was added. The mycelia were separated from the spore suspension, the conidial suspension was harvested, and the final concentration of the inoculum was prepared at 10 6 conidia/mL. Bacterial inoculum was prepared by growing the strain A7 in KB broth, 30 • C, 160 rpm, for a day. The cell culture was centrifuged for 10 min at 6000 rpm and a fresh pellet, the suspension was prepared in one-fourth strength of 1% sterile carboxymethylcellulose (Sigma Aldrich, St. Louis, MO, USA) to prepare a final concentration of 10 8 bacteria/mL [87].
Dry vermiculite soil collected from the vegetable field was crushed, sieved, and sterilized by autoclave. The seeds were surface-sterilized for 4-5 min with an HgCl 2 (0.1%) solution, then washed 6-7 times with sterile dH 2 O. The seeds were saturated in sterile water for 12 h, transferred, and placed properly in a seedling bed prepared with the soil in a plastic tray for germinated and grown at 28 ± 2 • C for 7 days. Seven numbers of 7 days old seedlings were then transferred to a pot containing 2 kg of soil.
The seedlings were treated by inoculating 5 mL of bacterial cell suspension and 5 mL fungal spore suspension in the following treatments: (1) T 0 = sterile distilled water as control (2) T 1 = only bacterial cell suspension (3) T 2 = only fungal spore suspension, (4) T 3 = bacterial cell suspension and fungal spore suspension, (5) T 4 = bacterial cell suspension two days before the fungal spore suspension, (6) T 5 = fungal spore suspension two days before the bacterial cell suspension. The pots were observed for diseases such as a yellowing of the leaves after 40 days with a 20-day interval, and root rot and darkening of vascular tissues were observed after 40 days after sowing [88]. Fusarium wilt disease severity was visually assessed on a 0-5 rating. The severity was calculated using the percentage of foliage with visible yellowing or necrosis along with acropetal progression compared with the control pots. The scale of 0 = healthier plants, 1 = 1 to 20% wilt disease on one fourth leaves, 2 = 21 to 49% wilt disease on two fourth leaves, 3 = 50 to 70% wilt disease on three fourth leaves, 4 = 71 to 100% wilt disease on the whole plant and 5 = all leaves dead [89]. The percentage of disease incidence (DI) [90], disease severity (DS), and disease reduction (DR) [89] was scored 40 days (with 20 days interval) after sowing according to the formulas below: where n = number of leaves infected by wilt, v = scale of disease severity (0 to 5), N = number of leaves observed, V = value the highest scale [89]. (6) Plant growth parameters, i.e., root and shoot length, fresh and dry weight of root and shoot, and the seed vigor index was measured for each plant after the completion of the experiments.

Characterization and Analysis of Bioactive Natural Compounds Extract Present in A7 by TLC, HPLC, and GC-MS
To determine the bioactive natural compounds responsible for the antifungal and antibacterial activities of A7, the strain was cultivated in 1 L KB broth and grown for 5 days at 30 ± 2 • C with shaking at 150 rpm [96]. Cells were centrifuged at 8000 rpm for 10 min, and the resulting cell-free supernatant (CFS) was acidified to pH-2 by adding concentrated hydrochloric acid. The acidified CFS was mixed with equal volume (1:1 v/v) of ethyl acetate and incubated until the separation of two layers. The organic layer was decanted and evaporated at room temperature. The dry residue obtained was dissolved in 250 µL of methanol. An amount of 10 µL was evaluated for antifungal activity along with the control (10 µL ddH 2 O) by the agar-disc diffusion method described earlier. Aliquots of extracts were filtered and analyzed by Thin-layer chromatography (TLC) [97] and High-Performance Liquid Chromatography (HPLC). TLC using silica-G plates activated at 110 • C for 30 min, were used to fractionate the extracted organic compound in chloroform/acetone (9:1 v/v). The chromatogram was visible under UV light (Bio Red) at 254 nm after the TLC plate had dried [98]. The R f value was calculated after the separation of the fractions, marked, recovered again in methanol, and evaluated again for antifungal activity. The maximum antifungal activity showed by the fraction was analyzed by an HPLC system (1260 Infinity, Agilent Technologies, Santa Clara, CA, USA, with a liquid autosampler, at Indian Institute of Technology Guwahati, IITG). The mobile phase was a 45% CH 3 CN solution containing 0.1% H 3 PO 4 , with a speed of 1.0 mL/min. The wavelength detection was fixed at 270 nm [99]. HPLC elutes of the purified extract were examined via Gas Chromatography-Mass Spectroscopy (GC-MS) (Clarus 680 GC and Clarus 600C MS, PerkinElmer, Waltham, MA, USA; Liquid Autosampler, Library Software: Turbomass NIST 2008, at IITG) equipped with Capillary column: Elite-5MS Capillary Column: Length: 60 m, I.D:0.25 mm (Max. Program Temperature 350 • C), Phase Reference: 5% di-phenyl 95% dimethylpolysiloxane (low bleed) and a mass detector activated in EMV mode. The flow rate of the carrier gas (helium) was set at 1.0 mL min −1 , the injection-port temperature was kept at 250 • C. The column oven was kept at 80 • C for 2 min, followed by 10 • C min −1 to 250 • C for 0 min, then at 50 • C min −1 to 280 • C for 9 min. Between m/z 40 and 450, electron impact spectra in a positive ionization mode was obtained [100].

Statistical Analysis
The results are expressed as mean ± standard error mean (SEM) from data collected across experimental reports (n = 3 per data point, a biological triplicate, and repeated experiment). Data were analyzed using an analysis of variance (ANOVA), two-way ANOVA with Bonferroni posttests, and one-way ANOVA with Tukey's multiple comparisons means test to identify a significant difference with p-value < 0.05. All statistical analyses were carried out using GraphPad Prism 5 software version 5.01 GraphPad Software Inc., San Diego, CA, USA.

Isolation of the Strain and Its Morphological and Biochemical Characterization
A total of 24 distinct bacterial strains were obtained from the rhizoids of the gametophyte of Polytrichum sp. on King's Base agar medium supplemented with 100 µM of AlCl 3 . Among these isolates, A7 was selected based on its promising In vitro preliminary plant-growth-promoting, biocontrol activities against different plant pathogenic microbes, and other activities. Morphologically, A7 was rod shaped, smooth and green-pigmented. The green-pigmented, fluorescent activity of the strain was identified under UV light after 24 h of inoculation on KB agar medium. The strain reacted negatively but Gram-staining was found positive for the utilization of different carbohydrate sources, namely arabinose, xylose, glucose, trehalose, and melibiose but could not use adonitol, rhamnose, cellobiose, saccharose, raffinose, and lactose. Furthermore, A7 was also positive for the use of malonate, lysine decarboxylation, nitrate reduction, citrate and negative for ONPG, ornithine reduction, phenylalanine deamination, H 2 S production, Voges Proskauers, methyl red, and esculin hydrolysis ( Table 2).

A7 Was Identified as Pseudomonas Aeruginosa Using Molecular Tools
The 16S rRNA gene fragment was amplified through PCR amplification with the universal primer set corresponding to a single band (approx. 1.5 kb) ( Figure 1A) detected by gel electrophoresis. The transformation of E. coli TOP10 with a ligation mix by electroporation resulted in the appearance of small transparent colonies on Luria Bertani (LB) agar plates. The recombinant plasmid was verified by the colony PCR amplification of approx. 1.5 kb gene fragment. EcoRI digestion confirmed the recombinant plasmid of size 4.3 kb ( Figure 1B). Molecular characterization of the strain A7 was performed based on 16S rRNA gene sequencing identity using blast searches. NCBI blastn analysis of the fragment exhibited 99% similarity with the 16S rRNA gene sequences of Pseudomonas aeruginosa DSM 50071, Pseudomonas aeruginosa ATCC 10145, and Pseudomonas aeruginosa NBRC 12689. The phylogenetic tree of the strain was constructed with the closest Pseudomonas aeruginosa strains using the maximum likelihood method with 1000 bootstrap ( Figure 1D). The phylogenetic analysis showed that the A7 sequence clustered with several other Pseudomonas aeruginosa with high bootstrap support ( Figure 1D). Based on this observation, the strain was named Pseudomonas aeruginosa A7 and its 16S rRNA gene sequence that was determined deposited in NCBI GenBank with the accession number MN197639.

A7 Is Endowed with Multiple Plant Growth-Promoting Traits
The A7 plant growth-promoting activities were assessed on different plate-based and liquid-medium-based assays (Figure 3, Table 4). Indole-3-acetic acid production was considered positive after the development of a red halo zone on the Whatman no-1 filter paper membrane around the colony. IAA production was also checked quantitatively with the addition of L-tryptophan at 48 h intervals of incubation. The IAA production increased from 3.3 ± 0.30 to 6.5 ± 0.30 µg/mL during 48 to 96 h of incubation. With a further increase in the incubation time, the production decreased from 5.4 ± 0.03 to 3.1 ± 0.10 µg/mL during 144 to 196 h of incubation ( Table 4). The synthesis of IAA without the presence of L-tryptophan was also assessed ( Figure S1). The qualitative and quantitative phosphate solubilization activity of A7 was evaluated to be positive, and the solubilization of tri-calcium phosphate was 146 ± 0.50 µg/mL. The A7 was found to be able to solubilize potassium and zinc oxide, and the solubilization efficacy (SE) was recorded at 33% and 29%, respectively ( Table 4). The N 2 fixation was evaluated positively for A7 by the alteration of the color of the medium from pale green to blue (Figure 3e). The diameter of the pale green halo zone was recorded at 52 ± 0.05 mm. The increase in pH related to the creation of ammonia and nitrates from atmospheric N 2 fixation caused this color shift. Siderophores production was considered positive after the formation of an orange halo around the colony and was measured to be 45 ± 0.05 mm in diameter. Furthermore, the pink appearance in the supernatant indicated the production of siderophores (Figure 3f). The formation of a red-brown tint on filter paper indicated positive HCN synthesis by the strain. Positive ammonia production was also shown by the strain developing brown to yellow precipitate and the strain failed to produce polyamines (data not shown). Chitin degradation was considered positive after the development of the purple zone surrounding the strain from a yellow-colored chitin medium containing Bromocresol purple. In the region of chitin utilization, the pH of the medium shifts from acidic to alkaline due to the production of chitinase enzyme. The diameter of the degraded chitin chain was measured as a purple zone of 58 ± 0.05 mm in diameter. The other enzymatic activity of A7 was measured semi-quantitatively for hydrolytic capability (HC) of different nutrient substrates. The most common enzymatic activity in the bacterial strain A7 was for cellulase (2.4 HC), lignin (+), pectinase (2 HC), and proteases (1.3 HC), (Figure 3i-l and Table 4) and negative for xylanase activity (data not shown).

A7 Is Tolerant to Concentrations of Aluminum and Other Stress Conditions
To assess the metal tolerance potential of A7, the strain was tested for its growth on high aluminum and iron amended solid and liquid medium. The A7 could grow and tolerate 0-3.5 mM of aluminum on both the SP-SDS and MM broth medium. The minimum growth inhibitory concentration of A7 for the metal aluminum, i.e., IC 20 and IC 50 , was 0.76 ± 0.03 and 1.9 ± 0.05 mM. The strain could also tolerate and grow in the presence of FeCl 3 (up to 4.5 mM) and FeCl 2 (up to 2.5 mM). The IC 20 and IC 50 values were calculated for FeCl 3 (1.00 ± 0.04, 2.51 ± 0.02 mM) and FeCl 2 (0.47 ± 0.05, 1.18 ± 0.08 mM). Based on the different concentrations for the three metal compounds, the relative growth was equal, i.e., 73-96% at a concentration of 0.1-1.0 mM for AlCl 3 and FeCl 3 . Beyond this concentration, the relative growth decreased, and stopped at a concentration of 4, 4.5, and 3 mM for the three metal compounds, respectively. The strain was also checked for temperature, salinity, and pH tolerance potentials. The optimum temperature for A7 growth was 25-40 • C, with diminished growth and reduced fluorescent activity below 10 or above 40 • C (Figure 4a, panel V-VII). The A7 could tolerate salinity stress by up to 7% of NaCl. The optimum pH range for A7 was from pH 6 to 9 with maximum growth at pH-8, as the relative growth was recorded as 126.97 ± 2.0% as compared to control (pH-7). (Figure 4b and Table 5).

In Vitro Protective Effect of A7 against Aluminum Toxicity in Chickpea
Since strain A7 was isolated on an aluminum enriched medium, it was further tested for its ability to grow chickpea seedlings in aluminum conditions. The impact of the four treatments on the overall growth of chickpea, i.e., the root, shoot length, root, shoot fresh and dry weight, relative root length rate, was observed with 12 h time intervals for 48 h. The treatment of chickpea seedling by strain A7 in the presence of 100 µM FeCl 3 solution resulted in a significant (p < 0.001) increase in root length, shoot length, root-shoot fresh and dry biomass, seedling vigor index, and the relative root-length rate compared to only aluminum treated seedlings (Figure 5a,b). When the seedlings were treated only with aluminum, morphological changes on the root and root-growth inhibition were observed. When the seedlings were treated with A7 in presence of aluminum, the root length, as well as the fresh and dry weight of the root, exhibited a similar trend to the treatment of seedlings with A7 alone. The protective effect of A7 on aluminum treated chickpea was measured in terms of root length (max. 89 ± 1.4 mm and min. 42 ± 1.7 mm) and root fresh (max. 382 ± 3.8 mg and min. 123 ± 1.7 mg) root dry weight (max. 40 ± 0.8 mg and min. 13 ± 0.8 mg) relative root length rate (max. 97 ± 0.3% and min 82 ± 3.0%). The values of seed vigor index, i.e., plant overall growth was recorded as max. 1530 ± 3.0 and min. 1345 ± 1.5, respectively, during the incubation period ( Figure 5 and Table 6).

A7 Was a Potential Biocontrol Candidate against Fusarium Wilt of Chickpea
The in vivo control of Foc wilt disease of chickpea by strain A7 was evaluated in pot experiments using six treatments in which three treatments (T 3 -T 5 ) involved A7 and Foc. The disease symptoms on the leaves of chickpea such as yellowing or necrosis from top to bottom were observed and recorded after the 20th and 40th days after inoculation while root rot was observed after 40th days of inoculation (Figures 6 and S2A-C and Table 7). These symptoms led to the drying of leaves, drooping of petioles, and darkening of vascular tissues which are characteristic symptoms of Foc wilting. In comparison to the pathogen-inoculated positive control, all treatments, including A7, consistently suppressed the disease. When the chickpea seedlings were treated only with the spore suspension of Foc, severe wilt disease developed on the plants, and the percentage of disease incidence was 22.03 ± 0.4% to 65.43 ± 1.7%, and the disease severity was 22.43 ± 0.8% to 65.54 ± 1.7% (Table 7). The percentage of disease incidence was 12.12 ± 1.0 to 21.37 ± 1.3%, disease severity was 5.95 ± 0.5 to 10.29 ± 0.8%, and disease reduction was 44.70 ± 5.2 to 67.23 ± 2.3% when both A7 and Foc were inoculated in the soil simultaneously. Interestingly, when the soil was first treated with A7 before two days of the inoculation of Foc, the disease reduction was maximum 66.01 ± 2.9 to 77.00 ± 1.5% and minimum disease incidence 7.4 ± 0.6 to 14.99 ± 0.6 and disease severity 1.85 ± 0.1% to 3.92 ± 0.1% was observed from the plants compared to the soil treated only with Foc. Similarly, when the soil was treated with Foc prior two days to the inoculation of A7, the disease incidence was 13.20 ± 1.0 to 24.56 ± 1.0%, disease severity was 10.48 ± 0.5% to 19.38 ± 0.6%, and the disease reduction was 39.73 ± 1.6 to 62.26 ± 2.5%. From these different combinations of treatments, it was clear that strain A7 showed maximum disease protection when it was applied two days before inoculation of the pathogen and minimum when it was applied two days after the inoculation of the pathogen. From these experimental settings, the plant-growth-promoting activities of strain A7 on chickpea were also observed and recorded. The application of A7 on the plants resulted in the healthy growth of plants compared with the non-inoculated control at the end of 40th days of inoculation. The maximum root length, shoot length and plant biomass was recorded when treated with only A7 compared to control. The PGP parameters including root length, shoot length, root and shoot fresh and dry weight, and the seed vigor index were observed and recorded in different treatments (p < 0.05) ( Figure 6, Table 8).

Discussion
In the current research, based on its 16S rRNA sequences and phylogenetic analyses, aluminum-tolerant A7 obtained from the rhizoids of Polytrichum sp. was identified as Pseudomonas aeruginosa. Morphologically, A7 was Gram-negative, coccus, round, smooth and green pigmented [105]. In this study, multiple phenotypes of A7 related to plant growth promotion (PGP) and biocontrol potentials are reported. The biological control of plant diseases using bacteria has evolved as a sustainable disease-management approach. Bacteria associated with the root or in the rhizosphere are capable of secreting a range of antibiotic compounds, making them a potential source of biocontrol agents [106]. Burkholderia sp., Pseudomonas sp., Flavobacterium sp., and Bacillus sp. are examples of antifungal and PGP root and rhizobacteria. They play an important role in plant-growth promotion by secreting phytohormones, most importantly Indole-3-acetic acid (IAA) [107,108]. The inability of P. putida GR12-2 deficient in IAA synthesis to increase root growth and lateral-root formation was indicative of the role of bacterial IAA in plant benefits [109]. Soil fertility and plant nutrition are critical for ensuring adequate levels of micronutrients such as potassium, phosphorus, zinc, and many others, necessary for plant growth and development [110]. A PGPR that solubilizes phosphate has great potential in agricultural applications. Richardson et al. [111] found that bacteria increased the amount of P available in the soil for plant uptake. Similarly, in this study, Pseudomonas aeruginosa A7 could solubilize tri-calcium phosphate in vitro. Pseudomonas sp. AF-54 showed the possibility of inorganic P-solubilization by reducing pH and releasing acetic, malic, and gluconic acid [112]. The rhizosphere typically contains P-solubilizing bacteria, which produce gluconic acids to liberate inorganic phosphate from the soil [113,114]. The action of PGPR is frequently linked to the regulation of phytohormones involved in root development and growth as well as phosphorus solubilization [115]. Potassium-solubilizing bacteria have been observed to produce potassium from decomposing organic matter, crop residues, aluminosilicates, kaolinites, and feldspars by acidosis, chelation, and complex formation and exchange reactions [65,[116][117][118]. Bacillus sp., Burkholderia sp., and Pseudomonas sp. have been reported to efficiently solubilize potassium from K-feldspar from tea-planted soil [119]. According to [67,120] Rahnella aquatilis, Pseudomonas orientalis, Pantoea agglomerans, and Enterobacter isolated from the rhizosphere of paddy soil and rubber plant-soil, respectively, may solubilize potassium. Arthrobacter sp., Mesorhizobium sp., Paenibacillus sp., Klebsiella variicola and Enterobacter cloacae rape rhizobacteria and Klebsiella variicola, and Enterobacter cloacae tobacco rhizobacteria are reported to be able to solubilize potassium [121,122]. To reduce the use of chemicals, nitrogen fertilizer application in plants and atmospheric nitrogen fixation in soil by bacterial strains boost nitrogen availability in soil vital for plant growth [110]. Rhizospheres such as Aster gymnocephalus, Gringelia sp., Haplopappus sp., Juniperus sp. and Lygodesmia sp., are the major source of the nitrogen-fixing genus Paenibacillus. However, Azospirillum lipoferum and Bradyrhizobium japonicum were the reported rhizobacteria of Haplopappus sp., and Viguiera linearis [123]. It has also been suggested that root-associated Pseudomonas stutzeri A1501 fixes atmospheric nitrogen [124]. Diazotrophs, isolated from pepper vines, possess an enzyme that can convert N 2 into NH 4 + that plants can take up through the biological nitrogen fixation process [125,126]. Azospiril-lum brasilense sp. 245 and Burkholderia kururiensis M130 improved lateral-root development and ethylene signaling responses during rice-seedling cultivation through the biological nitrogen fixation process [127]. Interestingly, in this study, A7 exhibited nitrogen fixation in the nitrogen-free medium, which can be explored for the mechanism and future use. Agrobacterium tumefaciens, Rhizobium sp. [67]. Pseudomonas and Gluconacetobacter are capable of oxidizing zinc in a solid environment [68]. PGPR, including Pseudomonas aeruginosa A7, produces iron-chelating agents that bind insoluble ferric ions, thereby inhibiting the growth of phytopathogens and thus helping to control plant diseases. Siderophores are metal-chelating agents of low molecular weight that produced by bacteria and secreted as a means of facilitating iron uptake into their cells under Fe-limiting conditions [71,128]. Moreover, siderophores can bind a variety of metals, in addition to iron and several chemical structures and properties. The bacterial siderophores act as biocontrol agents and help in plant growth, thus applicable in mineral weathering, biosensors, bioremediation, and chelation agents [129]. Various physiologic and biochemical activities in plant growth and metabolism involve either root-based chelate breakdown or ligand exchange to provide iron and other metals from bound siderophores [130,131].
Multiple rhizo-Pseudomonas from diverse environments are known to decrease plant diseases through the secretion of natural product metabolites [105,132]. Extracellular enzyme-like cellulase, chitinase, and proteases produced by these bacteria attack the cell wall of plant pathogenic fungi, causing cell lysis and subsequent death [133]. Chitinase hydrolyzes the polysaccharide chitin, a linear homopolymer of β-1,4-linked N-acetyl-Dglucosamine (GlcNAc) residue found in the cell wall of fungi [134,135]. Antifungal protein degrading enzymes, Proteases, are known to be produced by biocontrol and PGP bacteria [136]. Several species of Arthrobacter, Pseudomonas, Sphingobium, Streptomyces, and Rhodococcus possess ligninolytic activity in vitro [137]. Fungal pathogens and PGPR enzymes, the most effective agents of biological control of plant diseases caused by fungal pathogens hydrolyze the 1,4-glycosidic bonds between the N-acetyl glucosamine in fungal chitin [73]. Pseudomonas aeruginosa A7 was found to degrade chitin and demonstrated wide spectrum fungal growth inhibition suggesting one such biocontrol mechanism. Hydrogen cyanide (HCN), a major inhibitor of cytochrome c oxidase and several other metalloenzymes, is produced and secreted by a few bacterial species as a secondary metabolite [138]. HCN synthase is a membrane-bound flavoenzyme present in proteobacteria (especially Fluorescent pseudomonads) that oxidizes glycine to generate HCN and CO 2 . Sequence similarities exist between the hcnABC structural genes of Pseudomonas fluorescens and Pseudomonas aeruginosa and genes encoding different amino acid dehydrogenases/oxidases, particularly nopaline oxidase of Agrobacterium tumefaciens [138]. PGPB produces hydrogen cyanide that interferes with essential enzymes leading to the degradation of phytopathogens cell walls and their control in rhizosphere soil [139,140]. HCN has been associated with the control of M. javanica disease in tomatoes and O. obesity, an agricultural pest in India [141,142]. Both NIA-2 and NIA-5, as well as Pseudomonas fluorescence, impart a beneficial effect on wheat and banana growth in studies [143,144].
The use of bacteria that promotes plant growth in metal-rich environments has been touted as one of the newest trends since metal-tolerant bacteria can support the diverse growth of crops in metal-rich environments [28]. Al can have a beneficial or toxic effect on plants and other organisms, depending on factors such as metal concentration, chemical form, and growth conditions. Al has largely been studied for its physiological, biochemical, and molecular effects on plants (increased nutrient uptake, root growth stimulation, and enzyme activity stimulation, among other things) [145]. Plant growth is adversely affected by metal in acid soil, characterized by a deficiency of nutrients and toxicity by aluminum is the main limiting factor [146]. It has been shown that aluminum inhibits the rapid expansion of roots in plants and the rate of relative root length provides a standard indicator of the toxicity of aluminum [36]. It was shown that metal-tolerant bacteria can advance plant development and increase metal uptake by hyper-and non-hyperaccumulator plants [147]. Bacillus sp. KGMDI and Bacillus sp. K25 tolerate their growth up to 75 mg/L, equal to 0.56 mM of aluminum, iron, and copper [148]. A7 could tolerate AlCl 3 up to 3.5 mM, FeCl 3 up to 4.5 mM and FeCl 2 up to 2 mM. In this study, Pseudomonas aeruginosa A7 produced IAA in the presence of 100 µM AlCl 3 , which may be responsible for the growth of chickpea by increasing root and shoot elongation, leaf surface area, and dry biomass. Burkholderia ginsengiterrae N11-2, Chryseobacterium polytrichastri N10, Pseudomonas fluorescens, Pseudomonas fragi N8, and Pseudomonas simiae N3, have been reported to grow in aluminum stress conditions [28,29].
Several PGPR strains are reported to have been used in the integrated biological control of Fusarium wilt in chickpea [89,149,150]. Fusarium wilt, produced by the soilborne fungus Fusarium oxysporum ciceris is a major issue restricting chickpea output around the world [9,151]. The disease symptoms such as yellowing of leaves, abnormal branching, drooping petioles, necrosis of foliage, and drying of roots are early symptoms [9,152]. Currently, chemical-control approaches have no effect on the Fusarium wilt of chickpea control in the field, so biological control is the most promising and effective method [153].
In this study, we demonstrated that strain A7 showed antagonistic activities against Foc under in vitro and in vivo conditions. Remarkably, the strain was able to promote chickpea growth and no negative impact on its growth was observed. PGPR genus Bacillus (63.14%), Burkholderia, and Pseudomonas (53.52%) have been reported to be effectively exploited as control agents for the pathogen by producing HCN pyrrolnitrin, phloroglucinol, phenazine, siderophores, cell-wall-degradation enzymes that suppress the Fusarium oxysporum f. sp. ciceris by inhibiting mycelial growth. As a result, they play a critical role in a variety of microbial interactions, resulting in abnormal hyphal swelling, becoming exceptionally lengthy and vacuolization, which manipulates physiological processes in other fungi and bacteria [26,150,154,155]. In our in vivo experiment, we found that the PGPR strain A7 consistently suppressed yellowing disease caused by Foc when applied to the soil. The A7 strain significantly reduced the yellowing disease and root rot in chickpea plants compared to the pathogen-inoculated control. So, this strain could be an excellent choice for further biological control research and chickpea-farming success.
The presence of antifungal antibiotic genes in the bacterial strain A7 was confirmed by a polymerase chain reaction for marker genes for the synthesis of 2,4-DAPG, hydrogen cyanide synthase, and phenazine-1-carboxamide. These antibiotics are known to target plasma-membrane integrity or electron transport in many fungal and bacterial pathogens and indirectly help plant growth [156][157][158]. Additionally, A7 was shown to produce several interesting bioactive compounds with known and novel activities. According to earlier research, lipid derivatives such as 9-octadecanoic acid, hexadecanoic acid methyl ester, octadecenoic acid, 1,2-benzene dicarboxylic acid, mono (2-Ethylhexyl) ester, 1,2benzene dicarboxylic acid and diisooctyl ester [159] were found to be powerful antibacterial compounds [103]. They induced the autolysis of cell membranes, damaged cell walls, and inhibited transcription, and translation in S. aureus, E. coli, and Salmonella sp. [160]. Interestingly these compounds have been reported to have antimicrobial, anti-inflammatory, antioxidant, and anticancer properties [161]. The antimicrobial and antioxidant activity of 1-hexadecene and hexadecane extracted from Acanthophora spicifera was also reported [162]. It is reported that various indirect and direct mechanisms contribute to pseudomonas promoting plant development [163]. Similarly, in this study, we report multiple phenotypes and mechanisms of biocontrol and plant-growth promotion by the reported strain.
In our report, several isolates of Pseudomonas aeruginosa have been reported as plant growth-promoting rhizobacteria (PGPR). Pseudomonas aeruginosa RRALC3 isolated from degraded forest soil from the Indian state of Chennai, enhanced the growth, macromicronutrient contents, along with enhanced carbon content of the native legume Pongamia pinnata seedlings [164]. Pseudomonas aeruginosa isolated from Korean mine soil was reported to have several plant-protection traits including antagonism against bacterial phytopathogens and the stimulation of defense-related genes in tomato plants [165]. PGPR Pseudomonas aeruginosa was reported to be the dominant bacteria from the rhizosphere of sorghum, paddy, tobacco, tea, and maize crops in India [166]. Recently, the Pseudomonas aeruginosa strain RTE4, isolated from the tea plant rhizosphere [167]; tomato plant rhizosphere associated Pseudomonas aeruginosa strain CQ-40 [168] and Pseudomonas aeruginosa FG106 [169]; and saffron rhizosphere Pseudomonas aeruginosa strain YY322 [170], have been reported as PGPR with multiple beneficial phenotypes and biocontrol activities in the plants.
Using culture-dependent and independent methods, it is suggested that many human pathogenic bacteria from the genus Burkholderia, Enterobacter, Pseudomonas, Ralstonia, Serratia, Staphylococcus, and Stenotrophomonas are prominent members of several rhizospheres [171,172]. Several species from these genera possess growth-promoting properties for plants, as well as excellent antagonistic properties against plant pathogens; as a result, they are used to prevent disease and promote plant growth [171]. To use rhizosphere, isolate as a successful biocontrol agent, the strains should be tested for safety and risk assessments should be performed [20]. Human isolates of Pseudomonas aeruginosa are recognized as an opportunistic, nosocomial human pathogen and thus the environmental isolates must be extensively researched before being considered as a biological control agent. Thus, the comparative virulence attributes of the reported Pseudomonas aeruginosa A7 will allow it to be used as a BCA and a safe biofertilizer. Additionally, since the strain is already adapted to local environmental conditions, it may be transformed into a biofertilizer in future research involving different chickpea varieties, environmental conditions, and field trials. Further research is required to fully understand the multiple biocontrol and chickpea plant growth mechanisms of strain A7. This study thus provides another biocontrol arsenal against wilt disease which can be useful in the control of Fusarium wilt in aluminum and metal-rich soils.

Conclusions
A Fusarium oxysporum f. sp. ciceris (Foc) antagonist bacterium was identified from the rhizoids of adult moss, identified as Pseudomonas aeruginosa A7 on a morphological and molecular basis. The strain produced antimicrobial metabolites with strong antagonistic activities against multiple plant pathogenic fungi and bacteria. It was shown to have significant inhibitory effects on the Fusarium wilt of chickpea and enhanced chickpea growth in a pot experiment. Chickpea seedlings under aluminum stress grew significantly better when treated with A7. Based on the PCR results, the strain carried several biocontrol markers related to the biosynthesis of antibiotics HCN, 2, 4-DAPG, and PCN. Furthermore, A7 s poly-extremophilic and extensive adaptations to metal stress can be useful in the bioremediation of metal-rich soils. The strain showed promising phenotypes with the potential of improving seedling growth and development while reducing losses caused by fungal plant diseases. Thus, the strain can be used in agriculture as a natural alternative to conventional PGPR and fungicides after the comprehensive biological safety assessment using the tools of whole-genome sequencing, transcriptomics, and metabolomics studies. Additional research is required to establish strain A7's mechanism of plant-growth promotion in chickpea or other plants. Interestingly, the strains' lignin degradation and production of bioactive compounds can be harnessed using other biotechnological interventions.
Supplementary Materials: The following supporting information can be downloaded at: https:// www.mdpi.com/article/10.3390/microorganisms10030568/s1, Figure S1: Bar diagram showing the production of Indole-3-acetic acid in the presence (5 mM) and absence of L-tryptophan by the bacterial strain A7 with 48 h time interval for 196 h, Figure S2A: In vivo establishment and control of Fusarium wilt disease of chickpea caused by Fusarium oxysporum f. sp. ciceris by the bacterial strain A7 at the first day (Day-1) of inoculation, Figure S2B: In vivo establishment and control of Fusarium wilt disease of chickpea caused by Fusarium oxysporum f. sp. ciceris by the bacterial strain A7 at 20th days  of inoculation (a,b), Figure S2C: In vivo establishment and control of Fusarium wilt disease of chickpea caused by Fusarium oxysporum f. sp. ciceris by the bacterial strain A7 at 40th days (Day 40) of inoculation (a,b).