Abstract
There is a lack of information on the rhizosphere of nut-bearing trees where microbial populations can benefit roots and tree growth. The current research aimed at discovering plant growth-promoting rhizobacteria (PGPR) in the rhizosphere of soil samples from around the root zone of six walnut trees, each of which was considered as a genotype, i.e. ‘TT1’, ‘TT2’, ‘SS2’, ‘ZM1’, ‘Chandler’ and ‘Haward’. The trees grew in different arid and semiarid regions of Iran and Turkey. The strains were isolated and identified based on different morphological and biochemical markers. Drought-stress tolerance was assessed in the case of each isolate through their transfer to culture medium, containing polyethylene glycol (PEG6000) at 0 and 373.80 g L−1. Resilient strains were analyzed for measuring their ability to produce siderophore, hydrogen cyanide (HCN), Indole-3-acetic acid (IAA) and Gibberellic acid (GA3). In sum, 211 isolates were identified, of which a large number belonged to the Bacillus genus and, specifically, 78% of the strains were able to grow under drought stress conditions. The genus Arthrobacter was only detected in the rhizosphere of ‘ZM1’, ‘Haward’ and ‘TT1’ genotypes. In 4% of the strains, IAA production exceeded 53 mg L−1, while a high level of phosphorus solubility was verified in 6% of the strains. No strain was found to have the capability of producing HCN. The strains were screened for drought-tolerance, which resulted in the discovery of two promising strains, i.e. ZM39 and Cha43. Based on molecular identification through amplification and sequencing of the 16S rDNA gene, these two strains seemed to belong to Bacillus velezensis and Bacillus amyloliquefaciens, respectively. The discovery of new PGPR strains could probably assist walnut trees in improving their mechanisms of adaptation to drought stress.
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Discover the latest articles, news and stories from top researchers in related subjects.Introduction
Drought stress is a pervasive impediment to horticultural endeavors in many regions of the world. Previous studies have shown that abiotic stress conditions, such as drought or flooding, can adversely affect the root microbiome, root exudates and morp1,2, thereby affecting plant growth and productivity. Among the many solutions that can assist in countering drought stress, the inoculation of rhizosphere with PGPR can have a wide range of benefits for plant roots and for the maintenance of plant growth in dry environments. In general, PGPRs can produce siderophores, antibiotics and cyanides that can further increase the availability of soil nutrients, stabilize atmospheric nitrogen, and generate antagonistic activity against plant pathogens and harmful microbes in the soil3,4.
The rhizosphere is a narrow zone of soil that encircles plant roots. It is a rich site of nutrients where a variety of organic compounds are released from the roots by exudation, secretion and deposition. This ecological feature of the rhizosphere provides carbon and energy sources to microorganisms, thereby facilitating a rapid rate of microbial growth and activity that can benefit the roots. While PGPR communities are able to colonize roots and stimulate plant growth5, it is possible to inoculate the rhizosphere artificially with more of the relevant PGPRs and increase their populations in the rhizosphere, thereby increasing the occurrence of benefits for plant roots.
PGPRs are diverse in genera and species, and specific set of PGPRs is usually found in the rhizosphere of each plant species. This means that not all PGPRs are suitable for artificial inoculation in the rhizosphere of a particular plant species. Thus, the correct species of PGPRs in the rhizosphere of a plant species need to be identified first. Then, they can be inoculated artificially in the rhizosphere so as to add to the existing population of PGPRs which naturally exist there. New PGPRs are increasingly being identified among bacterial genera such as Azospirillum, Pseudomonas, Klebsiella, Azotobacter, Alcaligenes, Enterobacter, Arthrobacter, Bacillus, Serratia, and Burkholderia6. With the exception of a few reports, the available literature on the rhizosphere of nut-bearing trees, such as walnut, is not substantive7,8.
Persian walnut (Juglans regia L.) is a deciduous tree species that has a high degree of adaptability to different growth conditions, although it grows more successfully in temperate regions and can survive at altitudes as high as 3550 m above sea level9,10. Walnut trees show allelopathy effects, meaning that unique species of microorganisms can survive and coexist under the canopy of the walnut trees. Therefore, it appears that microorganisms in the rhizosphere of this tree are entirely specific and different from those of other tree species. Yu et al.11 identified 11 strains with phosphate-solubilizing activity in the walnut rhizosphere using 16S rDNA. These 11 strains belonged to five genera namely, Pseudomonas, Staphylococcus, Planmicrobium, Microbacterium and Acinetobacter11.
Although few PGPRs have been inoculated in the rhizosphere of walnut roots so far, the benefits of inoculation are considered valuable in the available literature7,12, including research on the mitigation of drought stress and maintenance of biological features which can be achieved by inoculating the correct species of PGPRs in the rhizosphere. Accordingly, a complete and detailed identification of PGPR communities in arid and semiarid habitats of walnut can assist with tolerance to drought stress conditions. In this regard, the available literature can benefit from new research on reliable comparisons between the specific abilities of each identified strain, especially in terms of their ability to withstand unfavorable conditions of stress13. Such cases of research can contribute to their preservation and mass production by high-tech facilities in approaching future exploitation as biofertilizers.
Since walnut trees have the tolerance to grow in adverse conditions, it was hypothesized that it coexists with PGPRs that contribute to its resilient growth behavior. The present study was conducted to explore and identify bacterial diversity in the rhizosphere of several promising walnut genotypes grown in arid and semiarid regions of Iran. A thorough comparison was carried out among the identified and isolated strains under drought stress. Definitely, resilient strains would be considered as resources for improving walnut production in regions where drought stress is prevalent.
Materials and methods
Plant materials for rhizosphere sampling
The population of each strain was collected from the rhizosphere surrounding the root zone in each of six walnut genotypes, i.e. ‘TT1’, ‘TT2’, ‘SS2’, ‘ZM1’, ‘Chandler’ and ‘Haward’, grown in arid and semiarid regions of Iran and Turkey. These genotypes were coded nominally by the authors and are free to access upon request. All experiments were performed in accordance with relevant guidelines and regulations. The phenological and agronomic traits of the walnut genotypes were provided as supplementary data (Table S1).
Sample collection and isolation of PGPR
In the case of each genotype, soil samples were collected from 5 to 50 cm depths of the rhizosphere around the walnut roots. The samples were coded as ‘RS-SS2’, ‘RS-TT2’, ‘RS-TT1’, ‘RS-ZM1’, ‘RS-Haward’ and ‘RS-Chandler’, and were placed in sterilized plastic bags before being transferred to the laboratory after 24 h. The samples were stored at 4 °C until further analysis followed procedures that were outlined in a soil test-kit model (KA-054). Bacterial isolation involved adding 1 g of the rhizosphere soil to 9 ml of phosphate buffer with a specificity of 20 mM, pH 7.0, which was incubated inside a rotary shaker at 150 rpm for 30 min at 30 °C. The strains were grown in nutrient agar culture media (NA) and stored in a nutrient broth (NB) containing 15% glycerol at 80 °C, which is a long-term storage method for these bacteria.
Morphological and biochemical characterization
The strains were identified in relation to biochemical and morphological traits. Morphological characteristics were identified by observing each bacterial colony. A composite microscope (Gaynor) at 100X was used for observing the color, shape, size and margin of colonies of the bacterium. Also, the cell shape, size, endospore presence and the gram’s reaction were considered. Several biochemical traits were evaluated according to the Manual of Bergey’s Determinative Bacteriology14.
Drought stress tolerance assessment for the isolates
Single colonies were cultured and transplanted into 500 ml containers containing NB. They were aerobically grown on a rotary vibrator at 150 rpm for 48 h at 27 °C. This was followed by adding distilled water along with a suspension of bacteria, reaching a final concentration of 109 ml mL−1. Various strains were transferred to a culture medium containing PEG6000 at 0 and 373.80 g L−1 which was equivalent to osmotic stress at 0 and − 1.5 MPa. The growth rate of isolates in a pilot study was previously recorded at different PEG6000 concentrations. Screening tests on these strains were calculated based on the growth rate of bacteria by measuring the optical density of their growth medium at 600 nm, using spectrophotometric analysis. Cultures that were able to grow in the presence of PEG6000 were analyzed further for biochemical traits through a factorial (PEG6000 at 0 and 373.80 g L−1 as factors) based on completely random design.
Phosphate-solubilization and amylase activity assay
The culture medium in this test was a modified type of the Sperber (Sp) medium15, and was supplemented with inositol hexaphosphate. Instead of tricalcium phosphate; however, inositol hexaphosphate was used. The test was performed on both solid and liquid media. The Sp medium, contained 2.5 g L−1 calcium phytate, was distributed in petri dishes under sterile conditions. Each petri dish was divided into six equal parts and the different fresh isolates were cultured by the dipping method in a separate petri dish, with three replicates, and stored in an incubator at 28 °C. The colony diameter grew, leaving different diameters of the transparent halos from the dissolution of the phosphate around each colony. The diameters were measured at intervals of 1, 2, 4, 8 and 10 days, and then the diameter of the halo was measured against the colony diameter in each isolate. Isolates which had halo-to-colony diameter ratios of more than 1.5 mm were evaluated by culture methods on liquid medium. At this stage, the modified Sp medium of 2.5 g L−1 calcium phytate was used. Phosphorus was measured in inoculated and control (un-inoculated) media. The preparation of the standard curve was similar to the mineral method. Amylase activity was performed using a modified version of Nack-Moon et al.16 method. After incubation at 30 °C for 5 days, the production of amylase, which was detected using soluble starch (1%), was screened by adding iodine to the culture. Liquid starch medium was used as control. Discoloration confirmed the presence of amylase production of bacterial isolates that decompose starch.
Siderophore and hydrogen cyanide production
The CAS method17 was used for quantitative measurement of siderophore produced by the strains. The reaction mixture included a cell-free extract of supernatant (0.1 ml) which was mixed with 0.5 ml of the CAS assay solution along with 10 μl of a shuttle solution (0.2 M 5-sulfosalicylic acid). The reaction mixture was stored at room temperature for 10 min, and then the absorbance was measured at 630 nm using a UV–VIS spectrophotometer (SL164, Systronics). For the control treatment, all of the compounds were used, except the extract which was obtained from the cell. Each siderophore unit was calculated using the following formula:
where Ar is the absorbance at 630 nm of reference (CAS assay solution + uninoculated media), and As is the absorbance at 630 nm of the sample (CAS assay solution + supernatant).
Production of HCN was done using a nutrient agar medium containing 0.44% glycine18. The surface of the agar was streaked with one-day culture and was coated with Whatman No. 1 filter paper. It was immersed in 2% sodium carbonate solution and 0.5% picric acid. This was followed by storage at 30 °C for 72 h. The changes observed in the color of the filter paper ranged from yellow to orange, red and brown. These colors indicate respectively the low, medium and high levels of HCN production by the strains. A quantitative analysis of HCN was done by analyzing strips of filter paper, which were changed by picric acid and sodium bicarbonate. After inoculating the tubes and keeping them at 30 °C for seven days, the strips were stored in double-distilled water and the changes in color were observed at 625 nm.
Estimations of Indole-3-acetic acid and gibberellins
Primarily, bacterial isolates were grown in NB for 72 h at 37 °C in a shaker. IAA was eluted by methanol according to a method described by Żur et al.19. The supernatant comprised formic acid (0.1%) aqueous solution (solvent A) and acetonitrile: methanol (1:1) mixture (solvent B). The MRM (Multiple Reaction Monitoring) mode was used for monitoring each analyzed compound in which the most abundant ion product functioned as the quantifier. Also, another abundant ion product was used for identifying the phytohormones. For the extraction of gibberellic acid (GA3), extracts were prepared with a mixture of iso-propanol/H2O/concentrated HCl (2:1:0.002, v:v:v). Then, they were centrifuged and purified within a series of steps. A re-dissolved operation was performed with a final concentration in 100 L methanol. Half of the volume was subjected to an ESI-triple quadrupole mass spectrometer device (HPLC-ESI-MS/MS, Applied Biosystems, USA) which was equipped with a reverse-phase C18 Gemini column (150 9 2.00 mm, 5-lm particle size, Phenomenex, USA)20.
Molecular identification of the bacterial strains
Two strains were then selected for further molecular characterization and identification. For this purpose, amplification occurred through PCR reaction, followed by subsequent sequencing of the 16S rDNA gene. The cultures were grown in LB for DNA extraction at 26 °C on a shaker (250 rpm). DNA was extracted using the DNeasy Tissue Kit (Qiagen). DNA concentration and quality were determined using a spectrophotometer and by gel electrophoresis on agarose (1%). The thermal cycles of the PCR operated according to a protocol used by Rees and Li, 2004. The amplified products were sent to Macrogen (a South Korean company) for sequencing the samples in both directions. The NCBI database was used as a platform for the comparison of sequence data by the BLAST program. The sequences of representative strains were submitted to the GenBank database and accession numbers were obtained.
Results and discussion
The physical and chemical characteristics of soil samples from the rhizosphere of each genotype differed from another (Table 1). In total, 205 non-identical bacteria were found in the rhizosphere surrounding the walnut roots (Table 2). Morpho-biochemical detection methods revealed that 76, 67, 44 and 18 isolates belonged to Micrococcus, Bacillus, Pseudomonas and Arthrobacter, respectively. The genus Arthrobacter was only detected in the rhizospheres of ‘ZM1’, ‘Haward’ and ‘TT1’ genotypes. The rhizosphere of the ‘RS-ZM1’ genotype contained the highest number of isolates, i.e. 19, 12, 15 and 2 of Bacillus, Pseudomonas, Micrococcus and Arthrobacter genera, respectively, whereas the rhizosphere of the ‘RS-TT2’ genotype consisted of the least number of isolates, i.e. 6, 7, 9 and 0 of Bacillus, Pseudomonas, Micrococcus and Arthrobacter genera, respectively (Table 2). Rhizobacteria with PGP-activity are known to occur in several bacterial phyla (Firmicutes, Proteobacteria and Actinobacteria), including strains that belong to the genera Azospirillum, Bacillus, Azotobacter, Agrobacterium, Alcaligens, Pseudomonas, Arthobacter, Comamonas, Burkholde-ria, Rhizobium, Pantoea, Variovorax and Serratia21. In confirming a large range of diversity among the bacterial strains, our results were in agreement with previous findings reported by Vega et al.22 in a research that led to the isolation of large numbers of bacterial strains from the rhizosphere of coffee plants.
In the current study, the strains were primarily screened for their ability to tolerate drought stress, while considering important physiological and biochemical traits relevant to plant growth promoters. In the absence of drought stress, phosphate-solubilizing activity corresponded with high amounts of dissolved phosphorus, which were caused by strains ZM4 (256 mg L−1), ZM18 (239 mg L−1), ZM44 (237 mg L−1), Cha13 (236 mg L−1) and Cha27 (235 mg L−1) (Table 3). Meanwhile, drought stress led to high amounts of dissolved phosphorous in strains ZM39 (248 mg L−1), ZM18 (254 mg L−1), Cha15 (241 mg L−1) and Cha43 (269 mg L−1). High amounts of siderophore production were recorded in strains Cha38 (24.5%), Haw25 (23.7%), ZM4 (22.7%) and Haw20 (21.4%) under normal conditions, whereas drought stress induced high levels of siderophore production by Cha43 (28.6%), ZM39 (28.4%), Haw25 (25.8%) and ZM4 (24.6%), respectively.
The ability of microbes to release metabolites, such as organic acids, can be used as an index for determining phosphate-solubilizing activity23. The ability of bacteria to secrete organic acids is a function of mechanisms that are controlled by bacterial gene expression patterns which, in turn, can be influenced by environmental factors. Many phosphate-solubilizing bacteria (PSB) can forage Fe from the mineral complex into soluble Fe3+ which takes form through mechanisms of active transport carriers24. Siderophore production by PSB could improve the availability of P indirectly. Since siderophores are ligands that can extract Fe from ferric phosphate and ferric citrate25, PSBs tend to produce organic acid compounds that help to transform metal species into chelates, thereby reducing metal toxicity26.
The ability of plants to produce auxin is one of the main traits by which plant growth promoters are generally measured. Auxins are a group of hormones which act as molecular signals that regulate plant growth, prolong cell proliferation, cell division and differentiation. While coexisting with plants, different bacteria produce various amounts of auxin and release them into the rhizosphere. Auxins are reportedly produced by Rhizobium, Bradyrhizobium and Nostoc species, as well as by other species which occur in the rhizosphere27. Among the strains in the current research, the ability to produce auxins differed significantly among the bacterial species. Bacillus strains Cha41 (24.7 μg mL−1), Cha21 (24.1 μg mL−1) and ZM7 (22.7 μg mL−1) had the highest performance in producing auxin under normal conditions. Under drought stress, however, IAA formation increased in the Bacillus strains Cha43 (29.4 μg mL−1), ZM39 (28.7 μg mL−1) and Cha21 (26.9 μg mL−1) (Table 3). The current results are in agreement with those previously reported by Beneduzi et al.28 regarding the ability of Bacillus strains to produce auxin in Luria and Berthani Bruce media. Similarly, Lwin et al.29 and Kaur and Sharma30 showed that rhizobacteria produced auxin (53.1–71.1 μg mL−1) under optimal growth conditions, whereas Husen et al.31 reported lower amounts of bacterial auxin production (33.28 μg mL−1). Shobha and Kumudini32 reported a wide range of IAA (35–217 μg mL−1) produced by bacteria, since IAA production by PGPB strains can be affected by different factors, including the species of the microorganisms, the conditions in which plants and bacteria coexist, the specificity of each growth stage in plants, and the availability of suitable substrates9,33.
The current study showed significant differences in the amounts of GA3 which were produced by the different strains. The highest gibberellin production was observed in strain Haw20 (80.9), followed by Cha28 (78.9) and Haw14 (77.9) (μg mL−1). In contrast, drought-stressed strains produced significantly higher amounts of GA3, as observed in Cha41 (94.3), Haw20 (86.7) and ZM39 (85.4) (μg mL−1) (Table 3). Previous studies reported that the maximum amount of gibberellin (65.3 μg mL−1) was produced by Pseudomonas sp. when the bacteria were isolated from the wastes of processed olive fruits in a culture medium of NB34.
One of the secondary metabolites produced by the PGPR is hydrogen cyanide, which plays an important role in the biological control of pathogens. In this study, all of the evaluated strains produced HCN, although their levels of production were not similar. Strains ZM39 and Cha43 produced the highest amounts of HCN, so much that the color of filter papers changed from pale yellow to brown. Also, these two strains showed starch hydrolysis activity along with other 134 strains (Fig. 1). Earlier research in the available literature suggested that HCN production by PGPR can promote plant growth by inactivating pathogens, but recent findings have argued that HCN indirectly increases P availability by metal chelation35. Increasing of soluble sugar contents in the leaves of Brachypodium distachyon (switchgrass) treated by some Bacillus strains has been reported39.
Based on morphological, biochemical and biological assessments, while considering plant response to drought stress, two promising strains were identified, ZM39 and Cha43, which caused high levels of resistance to drought. Thus, both strains were selected for further genetic identification by molecular markers. Upon completing the amplification and sequencing of their 16S rDNA gene sequences, and after using the BLAST-N program (NCBI), a complete identification showed > 99% similarity of their partial sequence with the available sequences from the NCBI database. The obtained sequences were submitted to NCBI and, together with other relevant information, their accession numbers were provided (Table 4). According to molecular assessments, ZM39 and Cha43 strains were identified as members of B. velezensis and B. amyloliquefaciens, respectively (Table 4). The current research identified these two rhizobacterial species, through DNA molecular analysis, in walnut rhizospheres for the first time. Previous reports indicated the presence of Azotobacter, Azospirillum, Bacillus, Pseudomonas, Aspergillus and Penicillium genera in walnut rhizospheres7.
Large number of strains of Bacillus spp. have been isolated from and characterized in relation to plants. Recent phylogenomic studies have demonstrated that Bacillus methylotrophicus, Bacillus velezensis, Bacillus oryzicola and Bacillus amyloliquefaciens subsp. plantarum can be considered as heterotypic synonyms36. Among the strains of the B. velezensis clade, secondary metabolites are diversely created by bacterial cells, which could exhibit antibacterial and anti-stress activities37. In the current study, with respect to the 16S rDNA gene sequence, phenotypic and molecular characteristics of B. velezensis were similar to those of B. amyloliquefaciens. In previous research, gyrB gene sequences confirmed that B. velezensis and B. amyloliquefaciens had similarities in heterotypic terms38.
Strains of the Bacillus genus have reportedly enhanced drought-tolerance in switchgrass through upregulation of drought-responsive genes and the modulation of the DNA methylation process39. Other strains can also make close associations with host plants and produce phytohormones, along with several well-characterized lipopeptide toxins40. These characteristics suggest that these strains have strong potential to act as bio-inoculants and can increase biomass in fruit trees, while assisting the defense system in plants against abiotic stress. PGPR can ultimately contribute to the production of plant growth regulators such as gibberellins41, auxins42,43, cytokinins and ABA44, thereby mitigating the adverse effects of abiotic stress on the physiological and biochemical processes of plants. Hormone levels in plant tissues could be modulated by microbial regulators via mechanisms that mimic the modes of exogenous phytohormone application45,46.
Conclusion
A large outlook of research potential is envisaged to explore walnut trees in terms of microbial populations in their rhizospheres. In this work, a significant diversity of PGPRs was confirmed in walnut rhizospheres. In addition, drought stress induced the ability of the identified PGPRs to solubilize phosphates and produce siderophore, IAA, gibberellic acid and HCN. Thus, there is scope that these PGPRs can be used as bio-fertilizers for sustainable crop production. Such improvements in the capabilities of plants may protect them against various forms of biotic and abiotic stress. Two promising strains (ZM39 and Cha43) were identified based on the current morpho-biochemical assays upon drought stress treatment. These strains were molecularly identified as B. velezensis and B. amyloliquefaciens, respectively. An ongoing project involves specifying their roles in improving tolerance against drought stress in walnut seedlings.
Data availability
Sequencing-data were generated during the current study and are available at NCBI as follows: Bacillus velezensis strain ZM39 16S ribosomal RNA gene, partial sequence; GenBank No. MK757975.1 (https://www.ncbi.nlm.nih.gov/nuccore/MK757975.1/). Bacillus amyloliquefaciens strain Cha43 16S ribosomal RNA gene, partial sequence; GenBank No. MK757976.1 (https://www.ncbi.nlm.nih.gov/nuccore/MK757976.1/).
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Acknowledgements
We are grateful to the University of Zanjan, the University of Urmia, the Atatürk University of Turkey and Iranian National Science Foundation for their supports. We acknowledge Urmia University for providing greenhouse supplies during the practical stages of this research. We also thank Mohsen Hamedpour-Darabi for reviewing the English language of the manuscript.
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N.L. Conceptualization, Methodology, Formal analysis, Writing-Original draft preparation, Writing-Reviewing and Editing. A.S. Conceptualization, Supervision, Writing-Reviewing and Editing. R.Ç. Advisor, Methodology, Investigation. K.V. Advisor, Writing-Reviewing and Editing. P.M. Methodology, Investigation.
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Lotfi, N., Soleimani, A., Çakmakçı, R. et al. Characterization of plant growth-promoting rhizobacteria (PGPR) in Persian walnut associated with drought stress tolerance. Sci Rep 12, 12725 (2022). https://doi.org/10.1038/s41598-022-16852-6
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DOI: https://doi.org/10.1038/s41598-022-16852-6
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