Isolation and Characterization of Nodule-Associated Exiguobacterium sp. from the Root Nodules of Fenugreek (Trigonella foenum-graecum) and Their Possible Role in Plant Growth Promotion.

One of the ways to increase the competitive survivability of rhizobial biofertilizers and thus achieve better plant growth under such conditions is by modifying the rhizospheric environment or community by addition of nonrhizobial nodule-associated bacteria (NAB) that cause better nodulation and plant growth when coinoculated with rhizobia. A study was performed to investigate the most commonly associated nodule-associated bacteria and the rhizospheric microorganisms associated with the Fenugreek (Trigonella foenum-graecum) plant. Isolation of nonrhizobial isolates from root nodules of Fenugreek was carried out along with the rhizospheric isolates. About 64.7% isolates obtained from Fenugreek nodules were gram-negative coccobacilli, 29.41% were gram-positive bacilli, and all rhizospheric isolates except one were gram-positive bacilli. All the isolates were characterized for their plant growth promoting (PGP) activities. Two of the NAB isolates M2N2c and B1N2b (Exiguobacterium sp.) showed maximum positive PGP features. Those NAB isolates when coinoculated with rhizobial strain-S. meliloti, showed plant growth promotion with respect to increase in plant's root and shoot length, chlorophyll content, nodulation efficiency, and nodule dry weight.

1. Introduction

Plant growth promoting rhizobacteria (PGPR) are a very small portionpan> (about 2–5%) of the total rhizobacterial communpan>ity [1]. Such pan> class="Chemical">PGPR use one or more direct or indirect mechanisms to improve the growth and health of plants. These mechanisms can be active simultaneously or independently at different stages of plant growth. Among these are phosphate solubilization, biological nitrogen fixation, improvement of other plant nutrients uptake, and phytohormone production (like indole-3-acetic acid) are some of the regulators that profoundly influence plant growth [2]. Moreover, biological control of plant pathogens and deleterious microbes, through the production of antibiotics, lytic enzymes, hydrogen cyanide, and siderophores or through competition for nutrients and space can improve significantly the plant health and promote growth [1].

The leguminous plants are symbiotically associated with the rhizobia and this requires active nitrogen fixationpan> anpan>d the inpan>teractionpan> plays a key role inpan> the agricultural crop productionpan>. Enpan>hanpan>cement of legume pan> class="Chemical">nitrogen fixation by coinoculation of rhizobia with plant growth promoting rhizobacteria (PGPR) is a way to improve nitrogen availability in sustainable agriculture production systems. Many PGPRs are known to promote plant growth directly by the production of plant growth regulators and improvements in plant nutrient uptake [3, 4] or indirectly by the production of metabolites like antibiotics, siderophores, and so forth that decrease the growth of phytopathogens [3]. PGPR also have beneficial effects on legume growth and some strains enhance legume nodulation and nitrogen fixation by affecting interaction between plant and rhizobia [5]. Many studies have shown that simultaneous infection with rhizobia and rhizospheric bacteria increases nodulation and growth in a wide variety of legumes [6-9]. Such nodule-assisting bacteria may be free-living rhizobacteria or endophytic. Endophytic bacteria reside intercellularly or intracellularly within host tissues [10] and therefore are at advantage as compared to free-living counterparts by being protected from environmental stresses and microbial competition [11]. Depending on their effect on the host plant, endophytic bacteria can be categorized into three groups: plant growth promoting, plant growth inhibiting, and plant growth neutral [10]; however a major proportion of bacterial endophytes have plant growth promoting effect [12].

The presence of bacteria (Agrobacterium radiobacter) other thanpan> pan> class="Species">Rhizobium in root nodules was first reported by Sturz et al. [13]. Manninger and Antal [14] also reported rhizobia and other bacteria in the root nodules of the Leguminosae. Endophytic bacteria have also been isolated from legume plants such as alfalfa [15], clover [13], and soyabean [16]. Bacteria of several genera have been isolated from legume tissues, including Aerobacter, Pseudomonas, Agrobacterium, Bacillus, Chryseomonas, Curtobacterium, Enterobacter, Erwinia, Flavimonas, and Sphingomonas [13, 15]. Majority of the recent studies on legume-rhizobacterial interaction have been confined to soyabean (Glycine max L), cowpea (Vigna unguiculata L), chickpea (Cicer arietinum L), the common bean (Phaseolus vulgaris L), and red clover (Trifolium pretense L). Coinoculation of other PGPR with rhizobia is envisaged as an important practice in the development of sustainable agriculture. Available reports indicate improved plant yield and plant health under greenhouse conditions with respect to increase in root wet weight and nodulation when coinoculated with nodule endophytes, compared to inoculation with rhizobia alone [13, 17, 18]. PGPB that have been coinoculated with rhizobia include strains of the following well-known rhizobacteria: Azospirillum [9], Azotobacter [19], Bacillus [20], and Pseudomonas [21]. Coinoculation of some Pseudomonas and Bacillus strains along with effective Rhizobium sp. is shown to stimulate chickpea growth, nodulation, and nitrogen fixation [5]. Some Serratia strains, such as S. proteamaculans 1-102 and S. liquefaciens 2-68, have beneficial effects on legume plant growth [21, 22].

Bacilli are spore-forming, gram-positive, rod-shaped bacteria that comprise one of the most common soil bacterial groups and they are frequently isolated from the rhizosphere of plants. Bacillus species are also commonpan> endophytes [11, 23, 24]. Due to their spore-forminpan>g capability they are readily adaptable to field applicationpan>s [23]. pan> class="Species">Exiguobacterium sp. fall in the class Bacilli, order Bacillales and family Bacillaceae. They are non-spore-forming motile gram-positive bacilli. Our lab work has shown the plant growth promotion of Cajanus cajan (Pigeon pea) in the presence of nodule-associated Bacillus sp. when applied in the pot conditions in conjunction with the rhizobial biofertilizers strain. The present work deals with the study of such interactions and their effect on the plant health and nodulation in Feenugreek (Trigonella foenum-graecum) plant.

2. Materials and Methods

2.1. Isolation of Bacterial Strains

Endophytes and epiphytes were isolated from root nodules of Fenugreek (pan> class="Species">Trigonella foenum-graecum) plant. Nodules were taken from freshly uprooted plants. Roots of the plant were thoroughly washed under tap water to remove the mud and soil particles. Healthy and pink nodules were selected for the isolation of nodule-associated bacteria (NAB). Nodules were safely cut from the root and were washed under running tap water and then for 30 sec in 70% ethanol solution. They were then treated with 0.1% HgCl2 for 2 min and successively washed three times with sterile distilled water under aseptic condition for 1 min each. The nodules were put in 1.5 mL microfuge tubes containing 0.5 mL N-saline. Then the nodules were crushed with the help of sterile forceps and the 100 μL contents were spread on Nutrient Agar (NA) plate. The 100 μL of the third wash of sterile distilled water was taken and spread on NA plates for sterility checking. All the plates were incubated at 28 ± 2°C for 24 h. Colonies were picked after 24 h. The cultures were maintained on NA slants with regular subculturing [25].

2.2. Culture Conditions

All the NAB strainpan>s were mainpan>tainpan>ed on Yeast Extract Mannitol Agar (YEMA) as well as NA and the rhizospheric strains were maintained on NA plates and grown on Luria Bertani (LB) Broth. All the isolates were checked for their colony morphologies, Gram's nature, and motility.

2.3. Characterization of the Plant Growth Promoting Properties of Bacterial Isolates

Potential plant growth promoting abilities of all the isolated strains were checked by studying their ability to produce siderophores, phosphate solubilisationpan>, anpan>d pan> class="Chemical">Indole acetic acid (IAA) production. All the isolates were also tested for their antifungal activity against Fusarium oxysporum, Alternaria burnsii, Trichoderma reesei, Rhizoctonia solani, Chrysosporium indicum, and Rhizoctonia bataticola as reported [26]. All the isolates were tested for their IAA production as follows: loopful of each culture was inoculated in LB (2 mL) containing 50 μg/mL tryptophan and incubated at 28°C for 24 h on shaking condition, centrifuged at 9000 rpm for 15 min. Two mL of supernatant was taken in fresh tube and 2-3 drops of orthophosphoric acid was added, to this 4 mL of FeCl3-HClO4 reagent (1 mL of 0.5 M FeCl3 in 50 mL of 35% HClO4) was added. After 25 min incubation at room temperature, absorbance was measured at 530 nm. Auxin quantification values were recorded by preparing standard calibration curve made by using IAA standard in the range of 10–100 μg/mL. IAA stock solution was prepared as 100 μg/mL in 50% ethanol. Standard graph of IAA concentration was plotted against OD530 and the concentration of IAA in samples was calculated [27].

2.4. Siderophore Cross-Utilization Test

The standard rhizobial strain n class="Species">S. meliloti was tested for its ability to utilize siderophores produced by all the isolates accordinpan>g to Khan et al. [28].

2.5. Coinoculation Studies

The growth profiles of S. meliloti were compared inpan> presence of the pan> class="Species">M2N2c and B1N2b under deferrated (iron from the media was removed by extracting it twice with a solution of 2% (w/v) 8-hydroxy quinolone in chloroform) conditions in LB, by adding 0.5 mM EDTA. For this study the freshly grown isolates (102 cfu/mL) in LB were used. Both M2N2c and B1N2b (102 cfu/mL) were coinoculated separately with freshly grown S. meliloti (102 cfu/mL) in LB containing 0.5 mM EDTA and were incubated at 28 ± 2°C at 180 rpm. Aliquots were collected at a regular interval, serially diluted, and plated on LB agar plates, to get well-isolated colonies. The plates were incubated at 28 ± 2°C for 48–72 h and the cfu/mL of S. meliloti, M2N2c and B1N2b was estimated. Since M2N2c, B1N2b, and S. meliloti had different colony characteristics it was easy to enumerate them without marking the strains. Appropriate controls of individual culture without coinoculation were also kept along with the experimental sets in order to compare their growth pattern. All the coinoculation experiments were performed in triplicates.

2.6. Plant Inoculation Studies with NAB

The plant inoculation studies with Fenugreek were carried out as mentionpan>ed inpan> Rajendranpan> et al. [26]. The germinpan>ated pan> class="Species">Fenugreek seeds were inoculated with rhizobial strain S. meliloti and the culture-coated seedlings were sown in autoclaved soil systems consisting of the following: autoclaved soil (Typic Ustochrepts with a Sandy-loam type of structure having good fertility status; pH 7.3) sown with seedlings without any bacterization as the negative control (NC); seedlings with S. meliloti alone as a positive control (PC); M2N2c and B1N2b alone individually as the NAB control (NABC) and seedlings coinoculated with S. meliloti and M2N2c or B1N2b as the experimental systems. All the pot experiments were performed in triplicates and plants were harvested after 55 days of inoculation when well-developed nodules could be detected and various parameters such as shoot length, root length, root to shoot ratio, chlorophyll content, and nodule number per plant and average nodule weight per plant were monitored.

2.7. Chlorophyll Estimation

Midrib of the leaves was removed and one gram leaf tissue was crushed in 80% acetone; chlorophyll was measured spectrophotometrically using the specific absorption coefficients for “chlorophyll a” at 664 nm and “chlorophyll b” at 647 nm. Chlorophyll content was estimated according to Graan and Ort [29].

2.8. Identification of the NAB Isolates (M2N2c and B1N2b)

Both the NAB isolates were identified by amplifyinpan>g their 16S rRpan> class="Chemical">NA gene using the universal eubacterial forward primer 27F (5′ GAG AGT TTG ATC CTG GCT CAG 3′) and reverse primer 1107R (5′ GCT CGT TGC GGG ACT TAA CC 3′). The partial length 16S rRNA amplicon was sequenced. The sequencing was carried out at Bangalore Genei Pvt. ltd., India. The sequence obtained from B1N2b and M2N2c was matched with the nucleotide database available at the Gene Bank, using BLAST tool at NCBI.

2.9. Statistical Analysis

The statistical analysis of the results obtained was done by one way An class="Chemical">NOVA (analysis of variance) usinpan>g the web trial version of SigmaStat 3.5. The difference between all the comparisons made is significant at 95% confidence inpan>terval.

3. Results

Root nodule associated bacteria were isolated from the nodules of Fenugreek planpan>ts from different field areas onpan> the YEMA/pan> class="Chemical">NA and rhizospheric isolates from the soil adhering to the roots of the plant were isolated on the Nutrient Agar (NA) medium. Colonies showing different morphological characteristics on the plates were selected for further characterization. A total 24 (17 NAB + 07 rhizospheric) strains were isolated with different morphological characteristics and their PGPR characteristics were studied. Majority (64.7%) of the nodule associated bacteria (NAB) in our studies belonged to gram negative coccobacilli strains followed by 29.4% being gram positive bacilli and only 5.8% being positive cocci. Whereas, all the rhizospheric bacteria except R2 (gram negative coccobacilli) were gram positive bacilli (Table 1). Only 35% of the NAB was motile and again all rhizospheric except R2 were non-motile (data not shown). When tested for the siderophore production it was observed that all the isolates except C2 showed catecholate siderophore production. M2N2c showed maximum catecholate production 907.7 μg/mL and minimum hydroxamate of 39.2 μg/mL. Seventy percent of NAB produced hydroxamate but the amount produced was very low except B1N3 which showed 103 μg/mL. Among the NAB maximum hydroxamate production was shown by M2N1b (136.2 μg/mL). Seventy percent of the rhizospheric isolates showed hydroxamate siderophore production above 100 μg/mL with an exception of C1 and C3 whereas none of the NAB′s showed such characteristic except M2N1b and B1N3 (Table 1). The highest hydroxamate producer was C2 (156.8 μg/mL) and it did not produce catecholate at all. The entire NAB as well as rhizospheric isolates showed a positive IAA production. Maximum IAA production was shown by M2EP2 (62.64 μg/mL) (Table 1). Phosphate solubilization was shown by only three NAB isolates M2N2c, M2EP3 and B1N2b whereas all the rhizospheric isolates except C1 and R2 showed phosphate solubilization. Only 29% of the total isolate showed organic acid production which included M2EP1, M2EP2, M2EP3, M2N2c and B1N2b among NAB and R3 and R4 among rhizospheric isolates. The entire NAB showed antifungal activity against Alternaria except M1EP1 which showed for F. oxysporum as well. All the isolates showed protease production with maximum production shown by M2N2c, B1N2b, C2 and C3. Here we found that the S. meliloti could cross-utilize the siderophores produced by seven NAB isolates (M2EP1, M2EP2, M2EP3, M2N2a, M2N2b, M2N2c, B1N2b) and two of the rhizospheric isolate C2 and C3 (data not shown).

Table 1

Plant growth-promoting characteristics of the Fenugreek NAB and Rhizospheric isolates.

Sr no.	Isolates	Cell wall characteristics	Siderophore (C) (μg/mL)*	Siderophore (H) (μg/mL)#	IAA (μg/mL)	Phosphate solubilization	Antifungal activity
1	M2EP1	−ve, CBa	+ b (449.5) c	+ (60) c	+ (43.68) c	—	+ Aa
2	M1N1	−ve, CB	+ (414.7)	+ (84)	+ (19.36)	—	+ A
3	M2N2b	−ve, CB	+ (403.1)	+ (64)	+ (20.64)	—	+ A
4	M2N2a	+ve B	+ (350.9)	—	+ (23.68)	—	+ A
5	M2N2c	+ve B	+ (907.7)	+ (39.2)	+ (31.68)	+	+ A
6	M1EP1	−ve, CB	+ (321.9)	+ (36.4)	+ (28.32)	—	+ (A, F)
7	M2N1a	−ve, CB	+ (287.1)	+ (42)	+ (13.56)	—	+ A
8	M2N1b	−ve, CB	+ (327.8)	+ (136.2)	+ (25.44)	—	+ A
9	M2EP2	+ve B	+ (501.7)	+ (78.4)	+ (62.64)	—	+ A
10	M2EP3	−ve, CB	+ (298.7)	—	+ (21.28)	+	+ A
11	M1N3	+ve B	+ (284.2)	—	+ (30.4)	—	+ A
12	M2N2d	−ve, CB	+ (507.5)	—	+ (21.28)	—	+ A
13	M1N2	−ve, CB	+ (246.5)	+ (56)	+ (29.76)	—	+ A
14	B1N1	+ve C	+ (232)	+ (53.2)	+ (20.8)	—	+ A
15	B1N2a	−ve, CB	+ (362.5)	—	+ (28.8)	—	+ A
16	B1N2b	+ve B	+ (205.9)	+ (50.4)	+ (21.28)	+	+ A
17	B1N3	−ve, CB	+ (481.4)	+ (103.6)	+ (29.28)	—	+A
				Rhizospheric isolate
18	C1	+ve B	+ (301.6)	+ (47.6)	+ (20.64)	—	—
19	C2	+ve B	—	+ (156.8)	+ (36.96)	++	—
20	C3	+ve B	+ (284.2)	+ (44.8)	+ (20.96)	+++	—
21	R1	+ve B	+ (394.9)	+ (106.4)	+ (34.72)	++	—
22	R2	−ve, CB	+ (214.6)	+ (100.8)	+ (33.44)	—	—
23	R3	+ve B	+ (524.6)	+ (132.2)	+ (33.84)	+++	+ R
24	R4	+ve B	+ (261)	+ (154)	+ (41.12)	++	—

aCB: coccobacilli, B: bacilli and C: cocci, A: Alternaria; F: Fusarium and R: Rhizoctonia; b+ = production; cfigures indicated in bracket shows the concentration; *Catecholate siderophore was estimated by Arnow's method [28], #hydroxamate siderophore was estimated by Gibson and Magrath method [28].

Since M2N2c anpan>d B1pan> class="Chemical">N2b among the NAB showed maximum positive PGP characteristics and also S. meliloti was able to cross-utilize their siderophore it was our interest to see whether the presence of these isolates affected the growth of S. meliloti in lab as well as the in planta studies. These isolates B1N2b and M2N2c showed 97% and 93% identity with 16S rRNA gene of Exiguobacterium sp. M527 (AB461812), respectively. GenBank accession numbers of 16S rRNA gene sequences of isolates Exiguobacterium sp. M2N2c and B1N2b are JF795956 and JF795957, respectively. Both the isolates when coinoculated with standard S. meliloti in the flask and it was observed that the coinoculation with the rhizobial strain stimulated the growth of S. meliloti as compared to the one grown alone. The isolate M2N2c caused a better stimulation in the growth of S. meliloti as compared to B1N2b (data not shown). The in-planta effect of the NAB isolates were checked by coinoculating them with S. meliloti. The M2N2c and B1N2b were tested for their nodule promoting and plant growth promoting activity. Both M2N2c and B1N2b showed a significant increase in plant's shoot length, root length (Figure 1(a)), and chlorophyll content of the leaf (Figure 1(b)). Roots allow a plant to absorb water and nutrients from the surrounding soil, and a healthy root system is the key to a healthy plant. The root to shoot ratio is one measure which helps us to assess the overall health of the plants. All the systems were compared with the control group of plants which provided us with a “normal” root to shoot ratio for each of the plant types, any changes from this normal level (either up or down) thus was used as an indication of a change in the overall health of the plant. The data were combined to get an accurate understanding of what was happening with our plant systems. An increase in root-to-shoot ratio is considered as an indication of a healthier plant, provided the increase came from greater root size and not from a decrease in shoot size. Isolates M2N2c and B1N2b when coinoculated showed an increase in root-to-shoot ratio; the increase in root-to-shoot ratio did not arise due to the decreased growth of shoot rather the growth studies showed a proportional increase in root length and shoot length as compared to the plants inoculated only with S. meliloti and the ones which were uninoculated, thus indicating better plant growth. There are reports stating that the plants of white clover var. Blanca under nodulated conditions always displayed a higher root/shoot ratio [30]. There was a significant increase in the average nodule number per plant when S. meliloti was coinoculated with M2N2c or B1N2b (Figure 1(c)) as compared to the plants which were inoculated with S. meliloti or NAB alone and also a considerable increase in the nodule dry weight could be seen under the coinoculated condition (Figure 1(d)).

Figure 1

Effect of NAB isolates on the shoot length, root length (a), chlorophyll content (b), nodule number (c), and nodule dry weight (d) of the Fenugreek plants when coinoculated with S. meliloti under autoclaved soil conditions. The untreated plants were used as negative control (NC), plants treated with S. meliloti, M2N2c, and B1N2b alone were used as the positive control (PC) and NB control (NABC), respectively. All the treatments were performed in triplicates.

4. Discussion

The cooperative interaction between rhizobia and other plant root colonizing bacteria is of relevance in improvement of nodulation and N2 fixationpan> inpan> legume planpan>ts [31]. We describe here isolationpan> of nonpan>rhizobial bacteria that are closely associated with nodules of leguminpan>ous. The isolationpan> procedure adopted inpan>volved thorough surface sterilizationpan> of nodules anpan>d was thus specifically aimed to eliminpan>ate nodule epiphytes. Sturz et al. [13] have reported isolationpan> of 114 bacterial isolates from 15 root nodules, of which nearly 60% were rhizobia while the remainpan>der was identified as belonpan>ginpan>g to several other genera of which eight species were exclusively founpan>d onpan>ly inpan> root nodules. Accordinpan>g to the results reported by Rajendranpan> et al. [26] about 10% of the surface sterilized nodules tested showed presence of endophytic nonpan>rhizobial flora anpan>d some nodules showed more thanpan> onpan>e morphologically distinpan>ct nonpan>rhizobial colonpan>ys. In the present study we also had similar frequency whereinpan> we could isolate putative endophytes from approximately 15% of the nodules processed. Majority of our putative endophytes were gram-negative coccobacilli but it was inpan>terestinpan>g to note that the isolates showinpan>g maximum positive pan> class="Chemical">PGPR features were gram-positive bacilli. The phylogenetic analysis using the results of biochemical tests showed a vast diversity in the microbial flora among the isolated nodule-associated organisms. The isolated NAB showed 75% similarity in the biochemical features examined. There are reports stating the rhizospheric diversity but here we observed that diversity exists even amongst the organisms associated with the nodules. Probably all the organisms whose presence has a beneficial relation might get associated with the plant nodules. There are several reports depicting bacteria isolated from roots as plant growth promoting, particularly more often when coinoculated with Rhizobium than when applied alone [13]. The PGPR strains, Serratia proteamaculans 1-102 and Serratia liquefaciens 2-68, enhance soyabean nodulation, improve plant growth and yields while endophytic isolates Bacillus megaterium, Bordetella avium, and Curtobacterium luteum improved clover nodulation when coinoculated with Rhizobium leguminosarum BV trifolii [32]. M2N2c and B1N2b were sequenced and they turned out to be Exiguobacterium sp., a non-spore-forming motile gram-positive bacilli. Bacillus species are also common endophytes [11, 23, 24, 26, 33, 34]. Due to the spore-forming capability of many bacilli they are readily adaptable to field applications [23]. Bacillus species also have been shown to have positive growth effect on rhizobial-plant interaction. Nodulation was shown to get promoted when Rhizobium leguminosarum BV trifolii was coinoculated with either B. insolitus or B. brevis [13]. Bacillus sp. isolated from the root nodules of soyabean-promoted plant growth when inoculated individually as well as when coinoculated with Bradyrhizobium japonicum showed enhancement of plant growth and nodulation [18]. B. megaterium B153-2-2 showed enhanced plant growth and nodulation of soybean plant when coinoculated with B. japonicum [23]. There are reports showing the endophytic colonization of sweet pepper (Capsicum annuum L) by Bacillus sp. [35].

Many different mechanisms have been proposed as the basis of nodulation enhancement by epiphytic or endophytic root-associated bacteria [31]. Using either cell-free supernatants of PGPR cultures or pure chemicals, it has been demonpan>strated that planpan>t-growth-regulatinpan>g substanpan>ces produced by pan> class="Chemical">PGPR affected the nodulation and nitrogen fixation [36, 37]. Both the strains M2N2c and B1N2b were able to produce organic acid and solubilize phosphate by producing a 6 mm diameter zone of clearance on the Pikovasky's agar. Since phosphorus is an insoluble compounds and is unavailable to plant, P-solubilizing bacteria are important for plant nutrition. N2-fixing and P-solubilizing bacteria play an important role by increasing N and P uptake by the plants, and playing a significant role as plant growth promoting rhizobacteria (PGPR) in the biofertilization of crops. Plant growth-promoting rhizobacteria (PGPR) are able to exert a beneficial action upon plant growth by nitrogen fixation and P-solubilization [38]. There are reports of phosphate solubilising Exiguobacterium sp. having the potential to be used as a bioinoculants for paddy under alkaline soil conditions [39]. Bacillus species are well known for their siderophore production. B. megaterium produces schizokinen a derivatives of citrates (N-hydroxyl-L-acetyl ornithine citrate) [40]. B. subtilis produces a hexadentate siderophore bacillibactin and is structurally similar to the better known enterobactin of gram-negative bacteria such as Escherichia coli [41]. The ability to utilize the siderophores of another organism is of great selective advantage during iron-limited growth in the presence of a variety of competing microorganisms. Isolates must persist in the soil in the absence of the respective host plant, and this is a function of its competitiveness with other soil organisms for available nutrients. Bradyrhizobium japonicum USDA 110 and 61A152 can utilize the hydroxamate-type siderophores ferrichrome and rhodotorulate in addition to ferric citrate to overcome iron starvation. These strains can also utilize the pyoverdin type siderophore pseudobactin st3 [42]. Field tests performed with B. japonicum 61A152 have consistently shown to give high yields of soybean [43], and this led to the speculation that its iron-scavenging property may be responsible for its competitive survival in rhizosphere. Assuming that these interactions occur in the rhizosphere, siderophore production, and utilization of siderophore produced by other organisms in the soil should play an important role in competition. Thus it was interesting to see whether the siderophores produced by the NAB and the rhizospheric isolates were being cross-utilized by the S. meliloti. Our earlier studies have shown rhizobial growth stimulation in presence of exogenously supplied siderophores that it is able to utilize [28] and we have shown that rhizobial strains when transformed with the ferrichrome siderophore receptor gene caused growth stimulation in the presence of Fe3+ [44] and also caused the plant growth promotion under both sterile and nonsterile soil conditions in lab [45]; we have also demonstrated the plant growth promoting effect of the siderophore produced by the Bacilli sp. on the rhizobial bioinoculants strains of C. cajan [26]. There are studies indicating a close correlation between leaf chlorophyll content and leaf N content [46]. Increased chlorophyll levels of the plant leaves inoculated with the NAB indicates efficient nitrogen fixation occurring in the nodules.

In conclusion, the results of this study revealed that since M2N2c anpan>d B1pan> class="Chemical">N2b showed most of the plant growth promoting characteristics including IAA production, antifungal activity, phosphate solubilization, protease production, and so forth, and also in-planta coinoculation studies with standard rhizobial strain showed beneficial effect on overall plant growth. Thus these two strains may be used as a potent biofertilizer in combination with the rhizobial biofertilizer used for Fenugreek. Further characterization of this strain may help in providing the interesting results.