Plant growth promoting characteristics of halophilic and halotolerant bacteria isolated from coastal regions of Saurashtra Gujarat

Halophiles are a class of microorganisms that thrive in environments with very high salt concentrations. The coastal regions of Saurashtra Gujarat host a diverse group of microorganisms including halophilic and halotolerant bacteria that may have plant growth promoting characteristics. Microorganisms with plant growth promoting characteristics are of immense importance in the field of agriculture and the present study was conducted to investigate the characteristics of halophilic and halotolerant bacteria isolated from agricultural soils of coastal regions of Junagadh and Porbandar districts of Saurashtra, Gujarat. A total of 15 isolated strains showed indole acetic acid production, solubilization of phosphate and potash, and nitrogen fixing capacity ranging from 18.77–33.48 μg ml−1, 50.10–106.10%, 180.42–239.92% and 0.170–0.480 g kg−1 of Jensen’s agar medium, respectively, while two isolates were also found positive for siderophore production. Besides, nine out of fifteen isolates also showed positive ACC deaminase activity ranging from 0.92-5.78 µM α-ketobutyrate mg−1 h−1. The isolates were further characterized by physiological, microscopic, and biochemical tests. The halophilic and halotolerant bacterial isolates were identified by 16S rRNA gene sequencing as belonging to Halomonas pacifica, H. stenophila, and Bacillus haynesii, B. licheniformis and Oceanobacillus aidingensis respectively. The 16S rRNA partial gene sequence of two isolates belonging to H. pacifica and H. stenophila were submitted to NCBI with accession number MK955347 and MK961217 respectively. The findings of the present investigation showed that isolated bacterial halophiles possess promising plant growth promoting characteristics. Their potential as bioinoculants to alleviate salinity stress in crops and for bioremediation deserves further investigation.

www.nature.com/scientificreports/ In contrast, non-halophilic microorganisms refer to those organisms that show optimum growth in media containing NaCl concentration less than 1% (0.2 M). However, those bacteria capable of growing irrespective of presence or absence of salt and capable of tolerating relatively high NaCl concentrations have been categorized as halotolerant or extremely tolerant if tolerance level exceeds 15% (2.5 M) NaCl. Thus, accordingly there are several categories of halotolerant microbes: Non-tolerant, those which tolerate only a small concentration of salt (about 1% w/v). Slightly tolerant, tolerating up to 6-8% (w/v). Moderately tolerant, up to 18-20% (w/v). Extremely tolerant, those microbes that grow over the whole range of salt concentrations from zero up to saturation 3 .
A considerable number of halophilic and halotolerant bacteria have been reported to possess plant growth promoting characteristics. Ramadoss et al. 4 showed that halotolerant bacteria isolated from saline habitats ameliorated the salt stress in wheat seedlings. Anbumalar et al. 5 investigated the plant growth promoting potentialities of IAA and phosphate solubilizing halobacterium strains and showed their effectiveness in plant seed germination and growth in various crops like cotton, tomato, lady's finger and maize under in vitro condition. Marakana et al. 6 also reported that plant growth promoting halotolerant bacteria serve as a potential tool for alleviating salinity stress in salt sensitive crops.
Saurashtra, also known as Sorath or Kathiawar, is a peninsular region of Gujarat, with natural saline habitat in western India, located on the Arabian Sea. The coastal areas of the region covering the entire sampling sites of the present investigation represent one of the natural saline microbial biodiversity hotspots in the country harboring a diverse group of microorganisms including halophilic and halotolerant bacteria that may have plant growth promoting characteristics. Previous reports on successful isolation and characterization of rhizospheric halotolerant bacteria from Bhavnagar district of Saurashtra also showed plant growth promoting potential as reported by Gontia et al. 7 and Jha et al. 8,9 . Symbiotic or non-symbiotic soil microorganisms that colonize the rhizosphere, inhabit plant roots and exert a positive effect to plants directly or indirectly. The use of microorganisms with the aim of improving nutrients availability for plants is an important practice and necessary for agriculture irrespective of their source of habitations throughout the world. Direct promotion of growth by PGPR occurs when the rhizobacteria produce metabolites that promote plant growth such as auxins, cytokinins, and gibberellins, ACC deaminase as well as through the solubilization of phosphate, potash, zinc minerals, nitrogen fixation etc. Indirect growth promotion occurs through the elimination of pathogens by the production of cyanide and siderophores. PGPR beneficial effects have been exploited in many areas including biofertilizers, microbial rhizoremediation and biopesticides 5 .
The present study evaluated plant growth promoting characteristics of halophilic and halotolerant bacteria isolated from agricultural soils of coastal regions of Saurashtra, Gujarat.

Results
The results of preliminary soil analysis is presented in Table 1. The physico-chemical characteristics of the soil samples such as pH, E.C., organic carbon content, and available phosphorous and potash ranged from 7.4-8.  Table 2. The colony morphologies of isolates ranged from irregular to cir- cular in shape with a majority being small to medium in size with flat to raised and convex type of elevations, while some of them were pigment producing. Colony pigmentation among isolates included pale yellow, creamy, shiny, watery and pure white. Most of the colonies had entire to irregular margins, while a few had undulate margins. The isolates also displayed different cell sizes and morphologies when viewed under the microscope. The cells ranged from coccus to short or thin long rod shape in single or pairs to bunchy type organization, while few were also found to be filamentous in structure. Nine isolates were gram negative while the remaining six were gram positive. All isolates were motile and some were spore forming in nature.
Determination of salt, pH and temperature tolerance test. The results of tolerance to different NaCl, pH and temperatures by isolates are presented in Table 3. The isolates were capable of tolerating salt concentrations up to 25% with optimum growth between 10-15% NaCl, optimum pH ranged between 6-8 with tolerance towards extreme acidity and increased growth towards alkalinity, and temperature tolerance up to 45 °C with optimum temperature observed at 35 °C.

Biochemical characterization.
The results pertaining to various biochemical tests conducted are shown in Table 4. The biochemical tests were carried out in order to determine the different biochemical characteristics of the isolates as addressed in the discussion section.
IAA production. The results of indole acetic acid (IAA) production by isolates are shown in Table 5. The amount of IAA production by isolates ranged from 18.77 to 33.48 μg ml −1 (Fig. 1) shown by isolates S 2 and S 1 respectively.
Nitrogen fixation capacity. The results of nitrogen fixing capacity of isolates are presented in Table 5 which were found to range from 0.170 to 0.480 g kg −1 of Jensen's agar medium shown by isolate S 11 and S 4 respectively (Fig. 2). The statistical value of calculated F was greater than that of table F at both 1 and 5% respectively thus indicating a high level of significance at both 1 and 5%.
Qualitative phosphate solubilization test in solid medium. The results observed in qualitative phosphate solubilization capacity of isolates are presented in Table 6. Thirteen out of fifteen isolates showed positive test while two (S 5 and S 9 ) isolates were negative and did not show any zone of solubilization (ZOS) on the Sperber's agar media. The highest ZOS and thereby solubilization efficiency was shown by isolate S 8 with ZOS Quantitative phosphate solubilization test in liquid medium. The quantitative phosphate solubilization capacity of isolates were estimated by measuring the drop in pH and release of Pi (inorganic phosphorous) in TCP broth recorded at intervals of 3, 5, 7 and 10 DAI ( Table 7). The drop in broth pH of respective isolates were found to increase with incubation time for all the isolates and the maximum drop in pH (4.1 ± 0.09) was recorded in broth of isolate S 8 at 10 DAI followed by isolates S 11 , S 4 and S 10 with drop in pH of (4.3 ± 0.09), (4.4 ± 0.09), (4.5 ± 0.09), respectively. The amount of Pi released from TCP also increased with incubation time  Starch hydrolysis +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve Lipid hydrolysis +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve Gelatin hydrolysis +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve Indole production −ve −ve −ve −ve −ve −ve −ve +ve +ve −ve −ve −ve +ve +ve +ve Methyl Red +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve Catalase +ve +ve +ve −ve +ve +ve −ve +ve +ve +ve +ve −ve +ve +ve +ve Oxidase +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve Glucose utilization +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve +ve  Values are mean ± standard error of three replicates   Table 9. Only eight out of fifteen isolates were found positive for potash solubilization capacity in the Aleksandrow's media. The highest ZOS and thereby solubilization efficiency was shown by isolate S 4 with ZOS of 9.60, 12.70, 17.23 and 17.83 mm (Fig. 5), potash solubilization efficiency (KSE) of 202.97, 195.46, 241.13 and 239.92% on 3, 5, 7 and 10 DAI respectively. The E. coli which was included as a negative control showed no zone of solubilization even at 10 DAI. The KSE (%) was seen to increase rapidly from 3 to 7 DAI and then continued to increase slowly from 7 to 10 DAI for majority of the isolates.
Siderophore production potentiality. The results of siderophore production potentiality of isolates showed that only two out of fifteen isolates viz., S 2 and S 6 were positive for siderophore production (Fig. 6). The siderophore type produced by these two isolates were further confirmed by tetrazolium test as hydroxymate type ( Fig. 7) which was inferred by the instant appearance of deep red colour on addition of tetrazolium salt and NaOH to the test samples. The results of qualitative and quantitative ACC deaminase production by isolates are shown in Table 10. Nine out of fifteen isolates were found positive for ACC deaminase activity while remaining six isolates showed negative activity. The amount of ACC deaminase production by isolates ranged from 0.92 to 5.78 μM α-ketobutyrate (α-KB) mg −1 h −1 shown by isolates S9 and S15 respectively.   identified by 16S rRNA gene sequencing on capillary sequencer (Applied Bio Systems 3130) using a pair of 16S universal primers. The PCR purified bands of isolates total genomic DNA extracts has been shown in (Fig. 8).
The 16S rRNA gene sequences obtained were compared against the nucleotide sequences available in BLASTn Search in GenBank of NCBI. Comparative sequence analysis of BLASTn search on NCBI revealed that eight out of ten isolates designated as S 1 , S 3 , S 4 , S 5 , S 6 , S 7 , S 8 and S 11 belonging to genus Halomonas were identified as H. pacifica while two isolates designated as S 2 and S 9 were identified as H. stenophila. On the other hand, three out of four isolates designated as S 12 , S 14 and S 15 belonging to genus Bacillus were identified as B. haynesii while one isolate designated as S 13 was identified as B. licheniformis and the remaining one isolate designated as S 10 belonging to genus Oceanobacillus was identified as O. aidingensis. The partial 16S rRNA gene sequence of two isolates S 1 and S 2 were re-designated as Halomonas pacifica strain HPSB1 and Halomonas stenophila strain HPSB2 and submitted to NCBI with accession numbers MK955347 and MK961217 respectively. The Phylogenetic analysis of these two strains using NCBI BLAST pairwise alignments revealed their relatedness with other strains of respective species (Fig. 9) and similarly for remaining isolates ( Supplementary Fig. S1 to S13).

Discussion
Preliminary analysis showed that the soils from which the halophilic bacteria were isolated were slight to moderately alkaline, non-saline and low to medium with respect to availability of soil organic carbon, phosphorous and potash. These results agrees with the findings of Echigo et al. 10 who reported that isolation of extreme halophiles can also occur from environments in which they are not expected to be actively growing.
The morphological characteristics of isolates deduced from the observed colony characteristics recorded in terms of size, shape, elevation, margin, texture, opacity, pigment and microscopic features showed the typical halophilic like colonies on media after 24 h of inoculation. These findings are similar to those by Kambura 11 and Roohi et al. 12 .
The results of salt, pH and temperature tolerance showed that the isolates were moderate to extreme halophiles and moderate halotolerants, slightly acidophilic to alkaliphilic and mesophilic in nature with respect to their optimum growth and tolerance capacity at different levels of salt concentration, pH, and temperature.
Results from various biochemical tests conducted on isolates indicated that they were all capable of producing alpha-amylase, lipase and gelatinase enzymes, while five isolates were positive for indole production. A positive methyl red test for all isolates indicated that they are glucose fermenters. Hence, all the isolates showed negative Voges-Proskauer test as bacteria can give only either of the test positive except for some gram negative bacteria in exceptional conditions that are reported to give positive test for both methyl red and Voges-Proskauer test. On the other hand only one isolate tested positive for hydrogen sulfide production implying that only one of the fifteen isolates has an ability to reduce sulfur containing compounds to hydrogen sulfide during metabolism. All fifteen isolates tested positive for oxidase test whereas only twelve and five out of fifteen isolates were found positive for catalase and urease tests respectively. Ten out of fifteen isolates were found positive for nitrate reduction test. Only one out of fifteen isolates was detected positive for phenylalanine deamination test. All isolates were found capable of using glucose as their carbon source for energy. The same goes for arabinose except one isolate which tested negative for utilizing it as carbon source. Eleven, eight, seven, four, and two isolates tested positive in utilizing lactose, lysine, sorbitol, ornithine and citrate as carbon source respectively. However, no isolates were found positive to utilize adonitol as carbon source for their energy.
The amount of IAA produced by the isolates were found to be slightly more than the range 1 to 23 μg ml −1 reported by Verma et al. 13 and Khamna et al. 14 . The results of mean comparison related to different isolates indicated that concentrations of IAA produced by the isolates under study are in agreement with the results of former studies reported by Padder et al. 15 and Nghia et al. 16 . In their reports, the minimum to maximum IAA production at varying concentration of tryptophan in the medium ranged from 16.21 to 32.41 μg ml −1 and 10.44 to 33.13 μg ml −1 respectively. However, the IAA production range of the isolates under study are much lower as compared to the range 78 to 101 μg ml −1 reported by Nabti et al. 17 . www.nature.com/scientificreports/ The positive nitrogen fixation capacity of the isolates quantified by micro Kjeldahl method even though in small quantity indicated the ability of the isolates to fix soil atmospheric nitrogen. Kanimozhi and Panneerselvam 18 also used the similar method and quantified the total amount of nitrogen fixed by Azospirillum isolates in nitrogen-free medium ranging from 3.3 to 15.6 mg N g −1 . Nitrogen fixation by free living organisms is a process that needs considerable amounts of organic matter to be effective. The free living organisms are said to be able to fix between 12 and 30 g N kg −1 of carbon source 19 . Thus the results of nitrogen fixation obtained from the isolates can be considered negligible to very low as compared to those of free living biological nitrogen fixers.
The solubilization of phosphates were confirmed from the formation of clear zones which is concerned with the P-solubilization by the isolates. These results implied that P-solubilization may be due to secretion of some substances into surroundings during the course of growing, which can solubilize phosphate or organophosphate. Phosphorous solubilization results are reported to vary depending on kinds of the metabolin, how quickly it   www.nature.com/scientificreports/ is released, and also the degree of its spread on the medium. Therefore, observational method of P solubilizing zone can only be used for qualitative assays 20 . In the present study, the expansion of diameter of ZOS of the isolates during the interval of 5 to 10 DAI were found to be much lower than the range of 25 to 30 mm reported by Zhu et al. 20 .
The halophilic and halotolerant bacteria studied in the present investigation lowered the pH of the TCP broth. The maximum drop in pH in TCP broth recorded in isolates were in accordance with those found in halophilic bacterium strain Kushneria sp. YCWA18 by Zhu et al. 20 . However, the maximum release of soluble Pi from TCP broth in culture supernatant accompanied by the significant drop in pH i.e., acidification of TCP broth by isolates were significantly higher than that reported in the latter. This indicated the implication of organic acid production in isolates. The negative correlation between drop in pH and Pi release, on the other hand, corroborates a  www.nature.com/scientificreports/ similar observation made even with rhizobium species 21 and other bacteria mobilizing P from rock phosphate 22,23 . Several mechanisms like the process of acidification, chelation and exchange reaction or the production of low molecular weight organic acids have been implicated to render insoluble phosphates into soluble form 24 . The Duncan's Multiple Range Test (DMRT) showed varying degree of significant differences in the treatment mean of potash solubilization efficiency between the isolates tested as shown in Table 9. The maximum potash solubilization efficiency (KSE) of the isolates were found to be lower by half than that reported in potash solubilizing bacteria by Sun et al. 25 . However, they were within the range of 169-423% reported in the latter. Similarly, the maximum potassium solubilization index (KSI) of isolates were also slightly lower but in compliance with the range of 2.37-5.25 accounted in potash solubilizing bacteria by Fatharani and Rahayu 26 . The measure of ZOS range of isolates studied were also within the range of 20.7-28.1 mm recorded on 7 DAI in potash solubilizing bacteria by Saha et al. 27 . The potash solubilization capacity of isolates indicated their potential to solubilize potash in agricultural soils thus making them available to the plants. This solubilization could be attributed to excretion of organic acids which either directly dissolves rock K or chelate silicon ions to bring K into solution [28][29][30][31] . Therefore, the application of K solubilizing halophilic bacteria could be of promising approach for increasing K availability in soils cultivated for high-K-demanding crops [32][33][34] .
Siderophores are said to be produced especially in an environment where the iron is deficient thus causing the bacteria to excrete siderophore in the extracellular environment to sequester and solubilize iron. The inability of the isolates under study to produce siderophores can thus be attributed to the possible sufficiency of iron in their habitual environments. An investigation about connection between iron homeostasis and the osmostress response in the halophiles also reported a decrease in the requirement for both iron and histidine and a lower level of siderophore synthesis at high salinity 5 . This report also correlates with the nature of isolates in the present study being high salt requiring and hence very low to no siderophore production in such high salinity.
The amount of ACC deaminase enzyme produced by the isolates were found to be three to six folds higher than the range 325-997 nmol mg −1 protein h −1 reported in halophilic and halotolerant bacterial strains by Mukhtar et al. 35 but two folds lower than 11,172.1 nM mg −1 protein h −1 reported in halotolerant bacterial isolates by Tiwari et al. 36 . However, the ACC deaminase production of the isolates under study are in compliance with the range 0.69-4.90 μmol α-ketobutyrate mg −1 protein h −1 reported in halotolerant bacterial strains by Siddikee et al. 37 . Penrose and Glick 38 described that different organisms with a wide range of ACC deaminase activity can act as PGPR. A low level of ACC deaminase activity, approximately ≥ 20 nmol α-ketobutyrate mg −1 h −1 is sufficient to permit a bacterium to grow on ACC and to act as a PGPR. Organisms with higher levels of ACC deaminase activity that is from 300 to 400 nmol α-ketobutyrate mg −1 h −1 do not necessarily promote root elongation to any greater extent than the strains that contain less enzyme activity 38 . The positive ACC deaminase activity of the isolates thus implies their ability to irreversibly cleave ACC molecules (intermediate precursor formed by the conversion of S-Adenosyl Methionine (SAM) (itself converted from main 'precursor of ethylene' called methionine by SAM synthase) by ACC-synthase which is further converted by ACC-oxidase into ethylene 39 ) into α-ketobutyrate and ammonia 40 , and may thereby promote plant growth by alleviating stress by lowering ethylene levels 41 under various stress conditions.

Methods
The study was carried out at "Department of Biotechnology, College of Agriculture, Junagadh Agricultural University, Junagadh" during the academic year 2018-2019. A total of fifteen isolates was used for studying the various plant growth promoting activities with three replication each for each experiment using a completely randomized design (CRD).
Soil sample collection. The soil samples were collected from coastal regions of Saurashtra, Gujarat viz., Junagadh and Porbandar districts located at coordinates 21.52°N 70.47°E and 21°37′48″N 69°36′0″E respectively. The names of the sites within the respective districts from which the soil samples were collected with due consultation and permissions have been shown in Table 11. A total of 15 soil samples (approximately 100 g each) were collected from agricultural fields from a depth of 5 cm around the crop rhizospheres with the help of an agricultural soil sampler.
Preliminary soil analysis. The preliminary analysis of soil samples were carried out to determine the soil chemical properties viz., soil pH by potentiometry and electrical conductivity by conductometry method 42 , and soil organic carbon content by back titration method 43 , available soil phosphorous by colorimetric method 44 and potash by flame photometry method 42 .
Isolation of halophilic bacteria from soil samples. Halophilic bacteria were isolated from 15 different soil samples and inoculated by streak plate method on freshly prepared halophilic agar plates containing in grams per litre: 10 g casein acid hydrolysate, 10 g yeast extract, 5 g proteose peptone, 3 g tri-sodium citrate, 2 g potassium chloride, 25 g magnesium sulphate and 20 g agar supplemented with 10% NaCl adjusted to pH 7.2 ± 0.2 (at 25 °C) and incubated at 35 °C for 5 days.

Morphological characterization.
Morphological characterization of all isolates were studied by plating on halophilic agar plates and incubating at 35 ± 2 °C for 24 h in BOD incubator. The morphological and cultural characteristics such as size, shape, elevation, margin, texture, opacity and pigment with regard to colonial characters were then observed and recorded from the growth on halophilic agar plates. In addition it also included microscopic characterization by Gram's staining, motility and scanning electron microscopic observation. These tubes were inoculated with 0.1 ml (having 10 7 CFU ml −1 ) previously grown culture of all isolates. A tube without inoculation served as the negative control for each range of salt, pH and temperature respectively. The isolates were inoculated and incubated at 35 ± 2 °C for 8-10 days. The strain that could grow at particular range of salt, pH and temperature were considered as tolerant by observing the presence or absence of growth and comparing it with negative control respectively for each isolates.
Biochemical characterization. Biochemical characterization of isolates were carried out by using a HiPure Bacterial Identification Kit obtained from HiMedia for biochemical tests viz., glucose, adonitol, lactose, arabinose, sorbitol, citrate, lysine and ornithine utilization, urease detection, phenyl alanine deamination, nitrate reduction and H 2 S production tests. Other biochemical tests viz., starch, lipid and gelatin hydrolysis, indole production, methyl red, Voges-Proskauer and catalase tests were carried out manually according to the standard protocol followed by Nezami et al. 45 while oxidase test was based on the method described by Nyakeri 46 .
IAA production. In vitro IAA production of isolates were determined following the protocol described by Khalid et al. 47 on a freshly prepared 10 ml Glucose Phosphate Broth (GPB) medium prepared in 100 ml Erlenmeyer flasks. l-Tryptophan was added at desired concentration to the liquid medium by filter sterilization and passing through 0.2 μm membrane filter. 1.0 ml of 3-days old isolates broth (10 7 CFU ml −1 ) were then inoculated into each flasks and incubated at 30 ± 2 °C for 48 h. A flask containing the same broth medium without inoculation was kept as negative control for comparison. Following incubation, the isolates' broth culture contents were filtered through Whattman filter paper No.2 and 3.0 ml of culture filtrate were taken in test tubes and 2.0 ml of Salkowski's reagent was added for measuring IAA production. The test tubes containing the contents were then allowed to stand for 1/2 h for color development. The colour development were observed in both standard solutions and culture filtrate of IAA and the intensity of color developed were measured by spectrophotometer at 530 nm and recorded. The concentration of IAA produced by the bacterial isolates were then deduced by calculation from the IAA standard curve.
Nitrogen fixation capacity. The nitrogen fixing capacity of the selected halophilic bacterial isolates were studied on a nitrogen free Jensen's agar medium. The plates were inoculated by streaking the isolate culture onto the plates and incubated at 35 ± 2 °C for 5 days. The nitrogen fixation capacity of the bacterial isolates were then determined by micro Kjeldahl digestion and distillation method 48 . The uninoculated plate of the same media was used as negative control. The nitrogen content in the nitrogen free media which is equivalent to the amount of nitrogen fixed by the isolates were then determined by calculating with the following formula: where, 0.05 = Normal concentration of H 2 SO 4 used; 0.014 = Conversion factor.
Qualitative phosphate solubilization test in solid medium. Qualitative phosphate solubilization test in Sperber's medium was carried out as per standard protocol followed by Nosrati et al. 49 . To examine Pi (Inorganic phosphorus) solubilization capabilities, 10 μl of the bacterial suspensions (~ 10 4 CFU ml −1 ) was spotted with the help of sterile inoculating needle onto the center of Sperber medium plate containing insoluble Pi. The inoculated plates were incubated at 28 °C. A Sperber agar plate spotted with E. coli was kept as the negative control. The zone of solubilization was recorded at 3, 5, 7 and 10 days after inoculation. The Solubilization Index (SI) was determined by measuring the ratio of halo (clear zone) diameter (mm) and the colony diameter as per the formula followed by Nautiyal 50 . And the Solubilization Efficiency (SE) was calculated by the formula followed by Nguyen et al. 51 .   52 . Erlenmeyer flasks (250 ml) containing 50 ml of phosphate solubilization estimation medium (containing per litre: 0.5 g yeast extract, 10 g dextrose, 5 g CaCl 2 , 0.5 g (NH 4 ) 2 SO 4 , 5 g Ca 3 (PO 4 ) 2 , 0.2 g KCl, 0.1 g MgSO 4 , 0.0001 g MnSO 4 and 0.0001 g FeSO 4 , pH 7.0) were inoculated with 100 μl of bacterial suspension (approx. 10 7 CFU/ml) in triplicates and incubated on rotary shaker (180 rpm) at 28 °C. After an intervals of 3, 5, 7 and 10 days, samples were drawn aseptically and centrifuged at 5000×g for 10 min to pellet the cell biomass and insoluble phosphate and the supernatants were used for the measurement of pH using pH meter for the determination of acidity and liberated Pi following phosphomolybdic blue color method 42 . The amount of Pi released in respective broths were estimated from three flasks each after incubation (DAI) in comparison with a set of uninoculated control. The concentration of Pi released were then calculated by plotting a graph of OD versus concentration of phosphates released in μg for standard and samples followed by their comparisons.
Estimation of pH change in broth culture. The supernatant obtained after centrifugation of each isolate culture at 3, 5, 7 and 10 DAI were examined for change in pH for determining acidity using a digital pH meter. The drop in pH in supernatants of each respective culture broth were recorded by comparing with the initial pH kept at 7.0.
Estimation of Pi released from culture supernatant. The available phosphorous content in the broth supernatant of each respective isolates were estimated by following phosphomolybdic blue color method 42 . A known varying concentration of potassium dihydrogen phosphate was used to prepare the standard curve. One ml supernatant of each isolates and control were then taken in 50 ml volumetric flask and 10 ml of chloromolybdic acid was added to it and the contents were mixed thoroughly. The volume was adjusted to three fourth with distilled water and 0.25 ml chlorostannous acid was added followed by immediate adjustment of volume to 50 ml with distilled water. After 15 min, the intensity of blue color developed were measured in UV spectrophotometer at 610 nm using reagent blank.
Potash solubilization capacity. The potash solubilization capacity of the selected halophilic bacterial isolates were tested qualitatively on an aleksandrow agar plates. A loopful of bacterial cells were picked from the respective fresh isolate culture broth and spotted in the middle of the plates containing solidified medium. The inoculated plates were then incubated in the incubator by placing them upside down at 30 °C for 4 days. An Aleksandrow agar plate spotted with an E. coli culture in the centre served as the negative control. The different bacterial isolates showing ability to solubilize potash by forming zone around their colony growth were considered as positive potash solubilizing bacteria. The diameter of zone of clearance or solubilization (halo) observed around the bacterial colony and the diameter of colony were measured after 3, 5, 7 and 10 days of inoculation in triplicates. Potash solubilization index (KSI) was then calculated as the ratio of diameter of halo (mm)/diameter of colony (mm) as per the formula followed by Nautiyal 50 . And the Solubilization Efficiency (SE) was calculated by the formula followed by Nguyen et al. 51 .
Siderophore production potentiality. The siderophore production potentiality of isolates were determined by following qualitative plate assay on Chrome Azurol S blue agar medium (CAS) to detect the siderophore production by isolates as per method described by Bhatt 53 . The CAS agar media was prepared according to the step-by-step procedure described by Louden et al. 54 . The individual CAS plates were then spot inoculated by overnight grown cultures of respective isolates and incubated at 30 ± 2 °C for 24 h. The isolates showing yellow to orange colored ring around the colonies were then considered as positive siderophore producing strains. The siderophore types produced were further identified as hydroxymate, catechol or carboxylate type by Tetrazolium, Arnow's, and Carboxylate test respectively as per the standard protocol described by Bhatt 53 .
Qualitative ACC deaminase production. Qualitative ACC deaminase production test was carried out using a simple plate assay following the standard protocol 38  www.nature.com/scientificreports/ Quantitative ACC deaminase production. The ACC deaminase activity of isolates were estimated by performing quantitative test as described hereafter. The bacterial isolates were cultured first in rich medium and then transferred to minimal medium with ACC as the sole nitrogen source in order to create culture conditions that favors the induction of isolates ACC deaminase activity. The isolates exhibiting positive ACC deaminase activity in the qualitative test were cultured first in a 15 ml fresh TSB broth and incubated at 35 ± 2 °C for 24-48 h on a shaker incubator at 150-200 rpm. After incubation, the accumulated biomass of the respective isolate cultures were harvested by centrifugation at 8000 rpm for 10 min at 4 °C and supernatants were discarded. The cell pellet of each isolates were then washed with 5 ml of either 0.1 M Tris-HCl (pH 7.6) or fresh DF salts minimal medium and centrifuged again and pellets resuspended in 15 ml DF minimal salt medium containing ACC at a final concentration of 3 mM in triplicates and incubated at 32 °C for another 36-72 h on a shaker incubator. The bacterial cells were then harvested again by centrifugation at 8000 rpm for 10 min at 4 °C and the supernatants were discarded and the cell pellet of each isolates were washed twice with 5 ml of 0.1 M Tris-HCl (pH 7.6) to ensure the pellets were free of the bacterial growth medium 38  The content mixture were then vortexed and incubated at 30 °C for 30 min. Then 2 ml of 2 N NaOH were added to the sample mixture prepared above and the absorbance were measured at 540 nm in spectrophotometer 57 . Finally, the ACC deaminase activity of isolates were determined by measuring the amount of α-ketobutyrate formed by the cleavage of ACC by ACC deaminase in each samples by comparing their absorbance at 540 nm to a standard curve generated by α-ketobutyrate.
Molecular identification by 16S rRNA gene amplification. The DNA for 16S rRNA gene amplification were isolated using Qiagen's DNA extraction DNeasy ® Blood and Tissue kit (250) and the 16S rRNA gene amplification were carried out on capillary sequencer (Applied Bio Systems 3130) with the help of a pair of universal oligonucleotide primers viz., forward and reverse primers designated as 005F and 907R with sequences 5′-TGG AGA GTT TGA TCC TGG CTCAG-3′ and 5′-CCG TCA ATTCMTTT RAG TTT-3′ respectively. The partial 16S rRNA gene sequence obtained from studied bacteria were analyzed and identified with nucleotide BLAST search in Gene Bank of NCBI.
Consent to participate/publish. I, as the main corresponding author of this paper hereby state that the entire research work was carried out with the appropriate consent of all the concerned authors and that all the concerned authors in relation to this work described has given their approval for participation into this publication process.

Conclusions
From the present study it was concluded that the halophilic and halotolerant bacterial isolates from agricultural soils of coastal regions of Saurashtra, Gujarat exhibited a very good plant growth promoting characteristics and represent a potent source of biofertilizers as plant growth promoting halobacteria and may help contribute to sustainable agriculture in such adverse conditions through reclamation and recovery of saline soils by supporting crop growth and metabolisms. However, the reported activities of the isolated halotolerant and halophilic bacteria represent only a potential for plant growth promotion. Further inoculation with the candidate PGPbacteria and salt stressed plants in salt affected soil are necessary for a more complete assessment of plant growth promotion abilities.

Data availability
The main author hereby declare with the consent of all concerned co-authors that data and materials related with the work described would only be made available at request.