Increased Production of the Exopolysaccharide Succinoglycan Enhances Sinorhizobium meliloti 1021 Symbiosis with the Host Plant Medicago truncatula

ABSTRACT The nitrogen-fixing rhizobial symbiont Sinorhizobium meliloti 1021 produces acidic symbiotic exopolysaccharides that enable it to initiate and maintain infection thread formation on host legume plants. The exopolysaccharide that is most efficient in mediating this process is succinoglycan (exopolysaccharide I [EPSI]), a polysaccharide composed of octasaccharide repeating units of 1 galactose and 7 glucose residues, modified with succinyl, acetyl, and pyruvyl substituents. Previous studies had shown that S. meliloti 1021 mutants that produce increased levels of succinoglycan, such as exoR mutants, are defective in symbiosis with host plants, leading to the hypothesis that high levels of succinoglycan production might be detrimental to symbiotic development. This study demonstrates that increased succinoglycan production itself is not detrimental to symbiotic development and, in fact, enhances the symbiotic productivity of S. meliloti 1021 with the host plant Medicago truncatula cv. Jemalong A17. Increased succinoglycan production was engineered by overexpression of the exoY gene, which encodes the enzyme responsible for the first step in succinoglycan biosynthesis. These results suggest that the level of symbiotic exopolysaccharide produced by a rhizobial species is one of the factors involved in optimizing the interaction with plant hosts.

S inorhizobium meliloti 1021 is a soil bacterium that establishes a nitrogen-fixing symbiosis with the host plants Medicago sativa (alfalfa) and Medicago truncatula cv. Jemalong A17 (reviewed in references 17 and 21). These plants are not only agriculturally important but are also key model organisms for studying the symbiotic interaction between rhizobial bacteria and their legume plant hosts. S. meliloti fixes dinitrogen gas to ammonia in root nodules formed by the host plant. Nodule development requires that several signals be exchanged between the plant and the rhizobial bacteria. Host plant flavonoid compounds signal S. meliloti to produce lipochitooligosaccharides called Nod factors (NFs) (39). NF activates multiple host plant responses, including tight curling of root hairs that traps bacterial cells within the curl and the induction of cell divisions in the root cortex which establish the nodule primordium (14,36). The bacteria invade and colonize the roots through "infection threads," which originate from microcolonies of bacteria trapped in the curled root hair cells (21,48). Infection threads are progressive ingrowths of plant cell membrane that contain a matrix composed of bacterial exopolysaccharides (EPSs) and plant cell wall material (14). Infection thread initiation and development require that S. meliloti propagate in the infection thread and produce both NF and the exopolysaccharide succinoglycan (25). New infection threads initiate at each cell layer, eventually delivering the bacteria to cells of the inner root cortex (48). There, the rhizobial bacteria are endocytosed by host cells within individual compartments of host cell membrane origin (6,17). Within these compartments, the low-oxygen environment and signals provided by the plant induce the bacteria to differentiate into a form called a "bacteroid" and to begin symbiotic nitrogen fixation (33,40).
Succinoglycan production by S. meliloti 1021 has been studied extensively (reviewed in reference 21). This exopolysaccharide is required for this strain to induce infection thread development on plant hosts, since it is the only symbiotically active exopolysaccharide that this strain produces in large quantities (18,28). The rea-sons that rhizobial exopolysaccharides are required for host plant invasion are not fully understood. S. meliloti 1021 strains that do not produce succinoglycan, such as the exoY mutant, are able to colonize plant surfaces and are trapped within curled root hairs, but they fail to initiate infection thread formation (8). These aborted infections are associated with gene expression responses (22) and cytological responses (34) characteristic of plant defense reactions. Several possible roles for succinoglycan in infection thread initiation and development have been proposed, including modulating factors such as pH, Ca 2ϩ ion concentration, or reactive oxygen species (ROS) that affect root hair elongation and/or plant defense responses (1, 23) by influencing cross-linking of infection thread matrix components and generating turgor pressure against the root hair cell membrane (4) or serving as a signal to the host plant through a plant receptor (37).
Although succinoglycan is required for efficient S. meliloti 1021 invasion of its plant hosts, there has also been speculation that the production of higher than normal amounts of succinoglycan is detrimental in the invasion process (51). This was based on the observation that overproduction of succinoglycan (known as a "calcofluor-bright phenotype") is found in several mutant strains with symbiotic defects, including strains with mutations of exoR (12), bluB (5), cbrA (16), and relA (52). However, most of these mutations have been found to have pleiotropic effects on S. meliloti, in addition to succinoglycan overproduction (5,7,15,52,54). Therefore, a specific role of succinoglycan overproduction in the host invasion defects of these strains could not be determined. Other S. meliloti 1021 mutants that produce higher levels of succinoglycan than the reference strain are those that carry mutations in the exoX gene (41,57). These strains are able to induce the formation of nitrogen-fixing nodules on the host plant alfalfa (41,57). However, ExoX appears to exert its inhibitory effect on succinoglycan biosynthesis at the posttranslational level (41), and it is unknown whether mutations in exoX have other effects on the interactions of S. meliloti with host plants.
The goal of this study was to determine whether increased succinoglycan production by S. meliloti 1021 has a positive or negative effect on its symbiotic proficiency on host plants. Increased succinoglycan production was achieved by overexpression in the S. meliloti 1021 reference strain of the exoY gene in the absence of other mutations that might have pleiotropic effects. The exoY gene encodes an undecaprenyl-phosphate galactose phosphotransferase that performs the first step in succinoglycan biosynthesis (43). The expression of exoY under the control of the constitutive Smb21651 promoter has been shown to be sufficient to restore succinoglycan production in an exoY mutant, but the amount of succinoglycan produced by these strains was not quantified (58). In this study, S. meliloti 1021 strains that express exoY under the control of this promoter have been constructed. We find that succinoglycan levels are elevated in these strains and that the symbiotic productivity of the host plant M. truncatula A17 inoculated with these strains is enhanced.
Construction of the pstb-LAFR5 vector, the exoY overexpression vector pstb-LAFR5-exoY, and S. meliloti 1021 strains carrying these plasmids. A 725-bp fragment upstream of the putative plasmid stability ORF SMb21651 of S. meliloti 1021 was amplified from the genome using Phusion polymerase (New England BioLabs, Ipswich, MA) and primers from Eurofins MWG Operon (Huntsville, AL). This fragment has been demonstrated to have strong constitutive promoter activity in S. meliloti (58). It was cloned into the HindIII and PstI restriction sites in the broadhost-range plasmid pLAFR5 (24). The resulting plasmid was named pstb-LAFR5 (stb is an abbreviation for "stability protein"). The exoY ORF was amplified from the S. meliloti genome and the 5= end of the ORF was fused with the sequence 5= CTGCAGTAACGTAACGTAAATGGAGTCAC CTCT 3=, which contains a PstI site followed by 3 stop codons, as well as a  (35,58). This fragment was cloned into the PstI and BamHI restriction sites in pstb-LAFR5 to generate plasmid pstb-LAFR5-exoY. Plasmids were mobilized into S. meliloti by triparental mating as described previously, using E. coli strain MM294A (19). S. meliloti exconjugants were selected on LBMC medium containing 10 g/ml tetracycline and 1 mg/ml streptomycin. Each exconjugant strain that was used in these studies was isolated from a separate conjugation reaction.
Plant nodulation assays. The host plant Medicago sativa (alfalfa) cv. Iroquois was prepared for inoculation with S. meliloti as described by Leigh et al. (29) with modifications: seeds were sterilized for 5 min in 50% bleach, rinsed in sterile water, and germinated for 3 days on plant cell culture-tested 1% (wt/vol) agar-water (Sigma, St. Louis, MO) (29). Seedlings were then moved to individual 100-mm by 15-mm Jensen's medium plates (49) and inoculated with 100 l of S. meliloti or S. medicae of the appropriate strain at an optical density at 600 nm (OD 600 ) of 0.05. Plants were grown in a Percival AR-36L incubator (Perry, IA) at 21°C with 60 to 70% relative humidity and 100 to 175 mol m Ϫ2 s Ϫ1 light for 5 weeks.
The host plant Medicago truncatula (barrel medic) cv. Jemalong A17 was prepared for inoculation with S. meliloti by scarifying seeds in concentrated sulfuric acid for 10 min, rinsing 5 times in sterile water, soaking overnight at 4°C, and germinating for 3 days on plant cell culture-tested 1% (wt/vol) agar-water (38). Seedlings were then treated, inoculated, and maintained as for alfalfa (see above) for 7 weeks.
Bacterial growth curves. Each strain to be tested was streaked to LBMC with 500 g/ml streptomycin and 10 g/ml tetracycline, and 3 single colonies of each were inoculated into precultures of the same medium and grown for 2 to 3 days. Cells from the LBMC preculture were washed in 0.85% saline and inoculated into a second preculture of the growth medium to be tested. After 2 to 3 days growth, cells from the second preculture were used to inoculate the growth curve cultures to an OD 600 of 0.01, except for Jensen's glutamate-mannitol medium, which was inoculated to an OD 600 of 0.05. All media for growth curves contained streptomycin at 500 g/ml and tetracycline at 10 g/ml.
Anthrone-sulfuric acid assays of polysaccharide production. Total polysaccharide in supernatants from cultures grown for 6 days in media lacking hexose sugars (GMS; M9 salts plus 12 mM mannitol, 5 mM glutamic acid, and sodium salt; or Jensen's medium plus 12 mM mannitol, 5 mM glutamic acid, and sodium salt) were quantified as follows: culture supernatants were collected from cultures by centrifugation and frozen at Ϫ80°C. Frozen culture supernatants were diluted 1/30 in Milli-Q H 2 O, and 0.325 ml of each diluted supernatant was mixed with 0.65 ml of 0.2% anthrone (wt/vol) in concentrated sulfuric acid (30) and boiled for 5 min. The OD 620 values of the boiled samples were measured and compared to a 2-fold dilution series of glucose (from 20 g to 0.31 g) dissolved in 1/30 of the appropriate culture medium. Anthrone assays performed on a 1/30 dilution of the appropriate culture medium served as the blanks. The microgram equivalents of glucose for each sample were normalized to the OD 600 of the cell pellet from that sample after resuspension of the pellet in 0.85% saline.
Calcofluor fluorescence quantitation of culture supernatants. Frozen culture supernatants were diluted 1/2 for LBMC and Jensen's GM media and 1/4 for GMS medium and were left undiluted for M9 and M9GM. For each culture supernatant, 175 l of the appropriate dilution (or of the appropriate dilution of uninoculated blank medium) was pipetted into a 96-well plate. Twenty-five microliters of a 0.14-mg/ml solution of calcofluor white M2R (dissolved in 0.04% Triton X-100 -400 mM Tris-HCl, pH 8.0) was added to each well. Fluorescence was read on a SpectraMax M5 plate reader (Molecular Devices, Sunnyvale, CA) at low sensitivity with excitation at 365 nm, emission at 435 nm, and cutoff at 435 nm. The appropriate blank was subtracted from each raw fluorescence reading, and the values were normalized to the OD 600 of the cell pellet from that sample after resuspension in 0.85% saline.

RESULTS AND DISCUSSION
Sinorhizobium meliloti strains with increased expression of the succinoglycan biosynthesis enzyme encoded by exoY produce elevated levels of the exopolysaccharide succinoglycan. The exoY gene, which encodes an undecaprenyl phosphate galactose phosphotransferase that attaches galactose to the lipid carrier on which succinoglycan is synthesized (43), was cloned into the plasmid pstb-LAFR5 (this study). pstb-LAFR5 carries a strong constitutive promoter from the region upstream of the SMb21651 ORF (58). Both the exoY overexpression construct pstb-LAFR5-exoY and the negative-control construct pstb-LAFR5 were conjugated into S. meliloti 1021 and tested for calcofluor fluorescence. Calcofluor white M2R fluoresces with maxima at ϳ420 nm and ϳ440 nm when bound to ␤-glucans (53). Succinoglycan is the only polysaccharide produced by S. meliloti 1021 that exhibits calcofluor fluorescence (18). Therefore, differences in calcofluor fluorescence between strains streaked onto this indicator are expected to be due to differences in succinoglycan production.
The results in Figure 1 show that strains carrying the exoY overexpression construct have much brighter calcofluor fluorescence (calcofluor-bright phenotype) than the S. meliloti 1021 reference strain or this strain carrying the negative-control construct pstb-LAFR5 on the rich medium LBMC (Fig. 1A). (A comparison of the calcofluor fluorescence of S. meliloti 1021 with that of the exoY::Tn5 mutant, which cannot make succinoglycan, is shown in Fig. S1 in the supplemental material.) The exoY overexpression strains are also brighter on glutamate-mannitol salts medium (GMS), which is a low-osmolarity medium that is commonly used in studies of succinoglycan production (55, 56) (Fig. 1B), and on Jensen's medium (49) supplemented with glutamate and mannitol (Jensen's GM) as the nitrogen and carbon source, respectively. Jensen's is the plant growth medium used for host plant nodulation assays (29). On either M9 medium containing NH 4 Cl as the nitrogen source and sucrose as the carbon source or M9 containing glutamate as the nitrogen source and mannitol as the carbon source (M9GM), the calcofluor fluorescence of the exoY overexpression strains is not brighter than that of the reference strain or the negative-control strains ( Fig. 1C and D). Also, the growth of the exoY overexpression strains on M9 and M9GM media was somewhat reduced relative to the growth of the reference strain and the negative-control strains, regardless of which carbon source and nitrogen source were used ( Fig. 1C and D; also see  Table S1 in the supplemental material.) The overall increase in calcofluor fluorescence of the reference strain and the negative-control strains seen in M9 medium versus their calcofluor fluorescence levels in other media probably reflects the high (ϳ200 mM) phosphate concentration of this medium. High levels of phosphate have been shown to lead to an increase in succinoglycan production in S. meliloti (32). Most importantly, however, the calcofluor fluorescence assay demonstrates a strong calcofluor-bright phenotype of exoY overexpression strains grown on Jensen's plant medium, indicating that these strains overproduce succinoglycan under conditions that most closely approximate those used for host plant nodulation assays.
The exopolysaccharide production of the exoY overexpression strains grown in liquid medium was measured using the anthrone-sulfuric acid assay for hexose sugars (Fig. 2) (30). Since the carbon source mannitol is not detected by this assay, all the hexose sugars quantified in supernatants of cultures grown in M9GM, GMS, and Jensen's GM should be of bacterial origin. Since succinoglycan is the most abundant exopolysaccharide produced by the S. meliloti 1021 reference strain (18,28), most of the sugars detected by the anthrone-sulfuric acid assay are from succinoglycan. A standard curve of glucose (Fig. 2) was used to calculate the quantity of polysaccharide in each culture supernatant, and these values were normalized to the cell OD 600 of the cultures. In M9GM, GMS, and Jensen's GM media, the exoY overexpression strains produced, respectively, 2.3-fold, 2.5-fold, and 2.4-fold more exopolysaccharide than strains carrying the negative-control constructs (Fig. 2).
To confirm that the increase in exopolysaccharide production detected by the anthrone method was due to an increase in succinoglycan production, a quantitative calcofluor fluorescence microplate assay was devised based on that of Schmitt and Budde for wort ␤-glucan (45). The calcofluor fluorescence of culture supernatants was quantified in a fluorescence plate reader with excitation at 365 nm and emission at 435 nm and blanked against uninoculated media (see Materials and Methods for details). The fluorescence value for each culture supernatant was normalized to the cell OD 600 of the culture. The average relative fluorescence for the exoY overexpression strains and the negative-control strains for each growth condition is presented in Fig. 3. The calcofluor fluorescence of the exoY overexpression strains is increased relative to that of the negative-control strains in all media tested. In LBMC and M9 media, which could not be tested for exopolysaccharide production by the anthrone-sulfuric acid method due to the presence of hexose sugars, the exoY overexpression strains have, respectively, a 2.5-fold (Fig. 3A) and a 4.4-fold (Fig. 3C) increase in calcofluor fluorescence. The 4.4-fold increase in calco-fluor fluorescence of exoY overexpression strains grown in M9 medium is higher than expected, given that very little difference in calcofluor fluorescence between these strains and the negativecontrol strains was observed on M9 agar plates. It is possible that more succinoglycan is produced by negative-control strains  grown on M9 solid medium than in liquid medium or that the presence of calcofluor in the plates during growth on M9 solid medium affects succinoglycan production.
The calcofluor fluorescence of the exoY overexpression strains grown in GMS is 2.4-fold greater than that of the negative-control strains (Fig. 3B). This value is very close to the 2.5-fold increase in exopolysaccharide production in GMS medium measured by the anthrone-sulfuric acid method (Fig. 2). The calcofluor fluorescence of the exoY overexpression strains grown in M9GM medium (Fig. 3D) and Jensen's GM medium (Fig. 3E) is also greater than those of the negative-control strains. In M9GM medium, the exoY overexpression strains have 2-fold greater calcofluor fluorescence than the negative-control strains (Fig. 3D), while in Jensen's GM medium, the exoY overexpression strains have 1.6-fold greater calcofluor fluorescence than the negative-control strains (Fig. 3E). The calcofluor differences in M9GM and Jensen's GM are not as great as the difference in total polysaccharide production between these strains measured by the anthrone-sulfuric acid method (Fig. 2). It is possible that some of the difference in total exopolysaccharide production (Fig. 2) is due to production of non-calcofluor-fluorescent exopolysaccharide such as EPSII (18) or cyclic ␤-glucans (50) or that succinoglycan produced in M9GM medium and Jensen's medium is more refractory to calcofluor binding and thus is not apparent in the calcofluor fluorescence microplate assay.
The exoY overexpression strains clearly produce higher levels of exopolysaccharide and more calcofluor-fluorescent material than the negative-control strains, indicating the production of more succinoglycan. Most importantly, the exoY overexpression strains grown in Jensen's GM plant medium produce culture supernatants with higher levels of exopolysaccharide and greater calcofluor fluorescence than the negative-control strains, indicating that these strains overproduce succinoglycan under conditions that approximate those used for host plant nodulation assays.
Exopolysaccharide overproduction is not deleterious to S. meliloti growth in most media tested. To determine the physiological effects of increased succinoglycan production on free-living cells, the growth rates of the strains described were compared. The exoY overexpression strains, which have been shown as described above to produce an excess of exopolysaccharide, have a growth pattern that is indistinguishable from the growth of the negative-control strains in LBMC (see Fig. S2A in the supplemental material), GMS (see Fig. S2B), or Jensen's GM plant growth medium (see Fig. S2E). Therefore, it is not expected that any symbiotic plant phenotypes conferred by exoY overexpression would be due to effects on cell growth. In M9 medium (see Fig. S2C) or M9GM medium (see Fig. S2D), the exoY overexpression strains had slightly reduced growth, similar to the reduced growth on M9 medium observed on agar plates ( Fig. 1C and D). (The detailed compositions of M9, GMS, and Jensen's GM media are listed in Table S1 in the supplemental material.) The addition of the trace element mixture from GMS medium (Fig. 4B) or from Jensen's medium (Fig. 4C) to M9 agar medium alleviates the growth defect of the exoY overexpression strains, suggesting FIG 4 Adding the GMS medium trace elements or Jensen's medium trace elements to M9 medium or adjusting the pH of M9 medium to pH 7 alleviates the growth defect of the exoY overexpression strains. When grown on M9 medium (A), the exoY overexpression strains had reduced growth on solid medium relative to the growth of the S. meliloti 1021 reference strain and the negative-control strains. In contrast, when the trace element mixture from GMS medium (B) or the trace element mixture from Jensen's medium (C) was added to M9 medium, the growth of the exoY overexpression strains was similar to the growth of the negative-control strains and the S. meliloti 1021 reference strain. Also, when M9 medium, which is normally buffered to pH ϳ7.3, is buffered to pH 7 (D), the growth defect of the exoY overexpression strains is eliminated. Panel A in this figure is the same image as panel C in Fig. 1. All exposures were 0.5 s on a 302-nm UV light box. that one or more of these trace elements is limiting in the presence of increased levels of the ExoY protein, increased activity of enzymes of the succinoglycan biosynthesis pathway, or increased levels of succinoglycan.
Medium additives that M9 lacks that are provided by the addition of either GMS trace elements or Jensen's trace elements are Fe 3ϩ , Zn 2ϩ , Cu 2ϩ , Mn 2ϩ , MoO 4 2Ϫ , and BO 3 3Ϫ (see Table S1 in the supplemental material). Among these, the addition of MnSO 4 has been shown to increase the growth rate of S. meliloti 1021 in M9 medium (10), and Mn 2ϩ is known to function as a glycosyltransferase cofactor (26), although the concentrations of Mn 2ϩ that might be required by ExoY or the other enzymes of the succinoglycan biosynthesis pathway are unknown. Also, anionic bacterial exopolysaccharides are known to chelate divalent cations (46), so one possibility is that high levels of these polysaccharides could interfere with bacterial growth when one or more divalent cations are limiting.
Another thing that differentiates M9 medium from GMS and Jensen's GM is that M9 is phosphate buffered to pH ϳ7.3, while both GMS and Jensen's GM have a final pH of 7 (see Table S1 in the supplemental material). We found that buffering of M9 medium to pH 7 instead of 7.3 also alleviates the relative growth defect of the succinoglycan-overproducing strains, even without the addition of trace elements (Fig. 4D). One possible explanation for this is a decrease in exopolysaccharide chelation of cations at lower pH. Recent studies suggest that exopolysaccharides with ionizable functional groups bind lower levels of some positively charged metals as a function of decreasing pH (9,20,27). Growth on lower-pH medium might make higher concentrations of positively charged metals available for use by bacterial cells.
exoY overproduction in Sinorhizobium meliloti 1021 enhances symbiotic proficiency with the host plant M. truncatula cv. Jemalong A17. It has previously been shown that on the plant meliloti 1021 on the host plant M. truncatula A17 is improved slightly, but statistically significantly, by exoY overexpression. Symbiotic productivity is measured as (A) shoot length in cm and (B) shoot fresh weight in grams. However, the symbiotic improvement due to exoY overexpression does not bring the S. meliloti 1021 symbiotic productivity on this plant host up to the level of that of S. medicae strains WSM419 and ABS7. This indicates that factors other than the level of succinoglycan production are responsible for the superior symbiotic efficiency of S. medicae strains on M. truncatula A17. Asterisks over graph bars denote a statistically significant difference from the reference strain in an unpaired t test. Plants inoculated with an exoY::Tn5 null mutant that does not produce any succinoglycan had similar shoot lengths and fresh weight to uninoculated plants. ref., reference. Error bars show standard errors of the means.
host Medicago truncatula cv. Jemalong A17, the S. meliloti 1021 reference strain is not as effective a symbiont as wild-type S. medicae ABS7 or S. medicae WSM419 (47). One possible reason for this is a difference in succinoglycan production. Both S. medicae ABS7 and S. medicae WSM419 produce more calcofluor-fluorescent material than the S. meliloti 1021 reference strain (Fig. 5). Exopolysaccharide from S. medicae WSM419 has been demonstrated by proton nuclear magnetic resonance to contain succinyl, acetyl, and pyruvyl substituents, which suggests it may be similar in structure to succinoglycan produced by S. meliloti 1021 (11).
To determine whether increased succinoglycan production could enhance the symbiotic effectiveness of S. meliloti 1021 with M. truncatula A17, the symbiotic proficiency of the exoY overexpression strains was compared with that of the S. meliloti 1021 reference strain, the negative-control strains, S. medicae ABS7 wild type, and S. medicae WSM419 wild type. On this plant host, exoY overexpression was sufficient to confer a significant symbiotic enhancement to S. meliloti 1021, as measured by shoot length (Fig. 6A) and shoot fresh weight (Fig. 6B). However, exoY overexpression did not increase the symbiotic productivity of S. meliloti 1021 on this plant host to the level of either S. medicae ABS7 or S. medicae WSM419. This indicates that there are probably addi-tional factors that make the S. medicae strains more effective symbionts than S. meliloti 1021 on M. truncatula A17.
On the host plant alfalfa, the shoot length (Fig. 7A) and shoot fresh weight (Fig. 7B) of plants inoculated with the exoY overexpression strains were not significantly different from those of plants inoculated with the S. meliloti 1021 reference strain or with the negative-control strains. This demonstrates that overproduction of succinoglycan in itself is not detrimental to the symbiosis with alfalfa and, therefore, is unlikely to be one of the factors that contribute to symbiotic failure of S. meliloti mutants, such as relA and exoR. This also demonstrates that the level of succinoglycan production of the S. meliloti 1021 reference strain is not a limiting factor for symbiosis on the plant host alfalfa.
Our results also show that increased production of succinoglycan is sufficient to increase the productivity of the symbiosis between S. meliloti 1021 and the host plant M. truncatula A17. This suggests that the native level of succinoglycan produced by S. meliloti 1021 is a limiting factor for invasion of this plant host. In the future, it might be beneficial to modify rhizobial strains that are used in the inoculation of legume host crop plants so that they produce higher levels of symbiotic exopolysaccharides and to determine if this can increase crop yields.

FIG 7
The symbiotic productivity of alfalfa plants inoculated with S. meliloti 1021 strains overexpressing exoY is not significantly different from that of plants inoculated with control strains. exoY-overexpressing strains of S. meliloti 1021 were inoculated onto the host plant alfalfa. Symbiotic productivity is measured as (A) shoot length in cm and (B) shoot fresh weight in grams. This indicates that an increased level of succinoglycan production by the S. meliloti 1021 reference strain does not reduce the efficiency of the symbiosis with the host plant alfalfa. Also, since there is not a significant improvement in symbiotic productivity in exoY overexpression strains, it indicates that succinoglycan production is not a limiting factor for the S. meliloti 1021 reference strain in establishing a functional symbiosis on the host plant alfalfa. Plants inoculated with an exoY::Tn5 null mutant that does not produce any succinoglycan had similar shoot lengths and fresh weight to uninoculated plants. Asterisks over graph bars denote a statistically significant difference from the reference strain in an unpaired t test. ref., reference. Error bars show standard errors of the means.