Endophytic Colonization and In Planta Nitrogen Fixation by a Herbaspirillum sp. Isolated from Wild Rice Species

doi:10.1128/AEM.67.11.5285-5293.2001

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Applied and Environmental Microbiology, November 2001, p. 5285-5293, Vol. 67, No. 11
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.11.5285-5293.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Endophytic Colonization and In Planta Nitrogen Fixation by a Herbaspirillum sp. Isolated from Wild Rice Species

Adel Elbeltagy,¹^, Kiyo Nishioka,¹ Tadashi Sato,¹ Hisa Suzuki,¹ Bin Ye,¹ Toru Hamada,²^, Tsuyoshi Isawa,¹ Hisayuki Mitsui,¹ and Kiwamu Minamisawa¹^,^*

Institute of Genetic Ecology, Tohoku University, Katahira, Aoba-ku, Sendai 980-8577,¹ and Marine Biotechnology Institute, Kamaishi Laboratories, Kamaishi City, Iwate 026-0001,² Japan

Received 4 May 2001/Accepted 20 August 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Nitrogen-fixing bacteria were isolated from the stems of wild and cultivated rice on a modified Rennie medium. Based on 16Sribosomal DNA (rDNA) sequences, the diazotrophic isolates werephylogenetically close to four genera: Herbaspirillum, Ideonella,Enterobacter, and Azospirillum. Phenotypic properties and signaturesequences of 16S rDNA indicated that three isolates (B65, B501,and B512) belong to the Herbaspirillum genus. To examine whetherHerbaspirillum sp. strain B501 isolated from wild rice, Oryzaofficinalis, endophytically colonizes rice plants, the gfp geneencoding green fluorescent protein (GFP) was introduced into thebacteria. Observations by fluorescence stereomicroscopy showedthat the GFP-tagged bacteria colonized shoots and seeds of asepticallygrown seedlings of the original wild rice after inoculation ofthe seeds. Conversely, for cultivated rice Oryza sativa, no GFPfluorescence was observed for shoots and only weak signals wereobserved for seeds. Observations by fluorescence and electronmicroscopy revealed that Herbaspirillum sp. strain B501 colonizedmainly intercellular spaces in the leaves of wild rice. Colonycounts of surface-sterilized rice seedlings inoculated with theGFP-tagged bacteria indicated significantly more bacterial populationsinside the original wild rice than in cultivated rice varieties.Moreover, after bacterial inoculation, in planta nitrogen fixationin young seedlings of wild rice, O. officinalis, was detectedby the acetylene reduction and ¹⁵N₂ gas incorporation assays. Therefore, we conclude that Herbaspirillumsp. strain B501 is a diazotrophic endophyte compatible with wildrice, particularly O. officinalis.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Use of nitrogen fertilizer is of great importance in rice production, as nitrogen is the major factor limiting growth undermost conditions (7). Since agriculture is expected to movetoward environmentally sustainable methods (31), much attentionhas been paid to natural methods of biological nitrogen fixation.Several diazotrophic bacteria, including Klebsiella oxytoca (11),Enterobacter cloacae (11), Alcaligenes (33), and Azospirillum(4), have been isolated from the rhizosphere of wetland rice.However, a renewed interest in endophytic diazotrophs, such asAcetobacter, Azoarcus, and Herbaspirillum, in gramineous plantshas arisen because of their occurrence mainly within plant tissuesand evidence for significant nitrogen fixation (18, 25). Azoarcussp. from Kallar grass, abundantly colonize and express nif genesand nitrogenase protein inside the original host as well as inrice roots (8, 25). Acetobacter diazotrophicus, an endophyticdiazotroph from sugarcane, has been found mainly associated withsugar-rich plants, such as sugarcane, sweet potato and Cameroongrass (2). In nitrogen-deficient conditions, sugarcane plantsinoculated with wild-type A. diazotrophicus had a higher nitrogencontent than plants inoculated with nif mutant or uninoculatedplants (29). Diazotrophic Herbaspirillum seropedicae has beenfound in maize, sorghum, sugarcane, and other gramineous plants(3, 23). H. seropedicae strain Z67 colonized mainly subepidermalregions of rice roots (5).

Cultivated rice (Oryza sativa) originated from species of wild rice and was domesticated several thousand years ago (14,22, 28). Wild rice species are likely to harbor unique populationsof nitrogen-fixing bacteria that differ from those in extensivelybred modern varieties of cultivated rice (10). Nitrogen-fixingendophytes in rice were reported to be higher in stems than inroots, indicating that rice stems probably provide a suitableniche (5). Additionally, use of rice stems for isolation ofdiazotrophic bacteria can minimize the possibility of contaminationfrom soil, because the rice stems are completely covered withsuccessive leaf sheaths before heading (14). Once endophyticdiazotrophs such as Azoarcus sp. infect plants, they sometimesspread systemically and reach aerial tissues of the plant (25).Recent research has focused on the question of whether the bacteriareally fix nitrogen within the plants (8, 29) and establishmutual symbiosis (16).

The aims of this study were twofold: first, to isolate nitrogen-fixing bacteria from the stems of wild and cultivated ricespecies, and second, to investigate endophytic colonization andin planta nitrogen fixation of a selected diazotroph in orderto verify whether the bacteria function as nitrogen-fixingendophytes.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial growth media. For isolation of diazotrophic endophytes, we used a modified version of Rennie medium (26), Rennie medium supplemented withrice extract and malate (RMR medium). RMR medium was preparedfrom solutions A and B. Solution A consisted of 0.8 g of K₂HPO₄,0.2 g of KH₂PO₄, 0.1 g of NaCl, 28 mg of Na₂FeEDTA, 25 mg of Na₂MoO₄· 2H₂O, 100 mg of yeast extract (Difco), 3.0 g of mannitol, 5.0g of sucrose, 0.5 ml of 60% (vol/vol) sodium lactate, 2.0 g ofsodium malate, 2.0 g (for semisolid medium in test tubes) or 15g (for agar medium for plates) of Noble agar, and 900 ml of distilledwater (the final pH of solution A was adjusted to 7.0 before autoclaving).Solution B consisted of 0.2 g of MgSO₄ · 7H₂O, 0.06 g of CaCl₂· 2H₂O, and 100 ml of distilled water. The solutions were autoclavedseparately and mixed after cooling. Filter-sterilized biotin andpara-aminobenzoic acid (100 µl each) were added at final concentrationsof 5 and 10 µg/liter, respectively. The combined solution (approximately1 liter) was mixed with 1.25 ml of rice shoot extract that hadbeen extracted with ethanol and 1.25 ml of rice shoot extractthat had been extracted with water as described below. RMR mediumcontained rice extract derived from 1 g of rice shoots in 1liter.

To prepare rice extracts, shoots of field-grown O. sativa cv. Sasanishiki at maximum tillage stage were washed with tap water,wiped dry, and weighed. The rice shoots (200 g) were maceratedin 500 ml of distilled water at 4°C or in 500 ml of 80% ethanolat room temperature using a mortar and pestle. The macerated extractswere filtered and centrifuged at 15,000 × g for 10 min to eliminateall residual substances. The fine sap was filter sterilized andkept at $-$ 20°C untiluse.

Acetylene reduction of bacterial culture. The nitrogen-fixing activity of the bacterial culture was examined by acetylene reduction assay in a 27-ml test tube containing9 ml of RMR semisolid culture. Acetylene gas was injected intothe head atmosphere of the test tubes (18 ml) at a final concentrationof 5% (vol/vol) and incubated for 24 h at 30°C. Ethylene concentrationwas assayed on a Shimadzu GC7A gas chromatograph equipped witha flame ionization detector and a Porapack R column (internaldiameter, 2.2 mm; length, 2 m; Shimadzu, Kyoto,Japan).

Sources of rice and isolation of diazotrophic bacteria. Four species of wild rice (Oryza officinalis W0012, Oryza barthii W1407, Oryza rufipogon W1989, and Oryza glandiglumis W1194)and three varieties of cultivated rice (O. sativa cv. Nipponbare,cv. Kasalath, and cv. SC41) were used. The stock seeds of wildrice were provided by the National Institute of Genetics (Mishima,Japan) and the Institute of Genetic Ecology (IGE), Tohoku University(Sendai,Japan).

O. officinalis W0012, O. barthii W1407, and O. glandiglumis W1194 were grown in Akadama soil pots in a greenhouse of the Instituteof Genetic Ecology, Tohoku University. They had almost reachedthe heading stage when used for bacterial isolation. Stems ofO. barthii W1407, O. officinalis W0012, and O. glandiglumis W1194were separated from leaf sheaths. The stems were surface sterilizedwith 70% ethanol by shaking for 1 min and transferred into RMRsemisolid medium. After cultivation for 1 week at 30°C, the culturewas reinoculated into RMR semisolid medium in test tubes for theacetylene reductionassay.

O. rufipogon W1989, O. sativa (cv. Nipponbare, cv. Kasalath, and cv. SC41; Gemdjah Benton) were grown at the experimentalstation of the Institute of Genetic Ecology (Kashimadai city,Miyagi prefecture, Japan). Stem segments separated from leaf sheathswere simultaneously vigorously shaken and washed with sterile0.01% Tween 20 for 30 min to eliminate epiphytic bacteria. Thesurface-washed segments were aseptically macerated in a mortarwith 0.8% saline solution and quartz sand and then transferredto test tubes containing RMR semisolid medium. After 1 week ofincubation at 30°C, the cultures were assayed for acetylenereduction.

The pellicles from acetylene reduction-positive tubes were streaked on RMR agar plates. Single colonies aerobically grownat 30°C on the plates were transferred separately into test tubescontaining RMR semisolid medium, incubated at 30°C for 7 days,and assayed for acetylene reduction. The resultant diazotrophicbacterial culture was mixed with sterilized dimethyl sulfoxideat a final concentration of 10% (vol/vol) and stored at $-$ 80°C.

PCR amplification and sequencing of the 16S rRNA gene. Cell lysate from each isolate for the PCR template was prepared by the method of Hiraishi et al. (13). 16S rRNA gene wasamplified by PCR using universal primers pr0R (5'-AGAGTTTGATCCTGGCTCAG-3')corresponding to positions 8 to 27 (forward primer) and 9rev (5'-AAGGAGGTGATCCAGCC-3')corresponding to positions 1543 to 1525 (reverse primer) of theEscherichia coli numbering system (35). The PCR operating conditionswere as described by Suzuki and Yamasato (32). The PCR productswere visualized by electrophoresis on ethidium bromide-stained1.0% agarose gels (SeaPlaque GTG FMC Bioproducts) and purifiedby using QIAquick (Qiagen) following the manufacturer's instructions.Sequencing was performed with an ABI PRISM Big Dye TerminatorCycle Sequencing Kit and a 377 DNA sequencer (Perkin-Elmer) accordingto the manufacturer's instructions. Six primers, f1 (5'-AGCCATGCCGCGTGTATG-3'),f2 (5'-GGGAGCAAACAGGATTAGAT-3'), f3 (5'-GAAATGTTGGGTTAAGTCCC-3'),r1 (5'-TGCAATATTCCCCACTGC-3'), r2 (5'-TTCCTCCACATCTCTACG-3'),and r3 (5'-CGCTCGTTGCGGGACTTA-3'), as well as the two PCR primers,were used to sequence both strands of the16S rRNA gene. FASTA(DDBJ, Mishima, Japan) was used to compare the resulting sequenceswith those identified in the DDBJ, EMBL, and GenBank DNA databases.The neighbor-joining method (27) and the Clustal W program wereused to construct a phylogenetictree.

Phenotypic characterization of diazotrophic bacteria. Gram staining, motility, and production of pectinase and cellulase were assayed as described previously (9). Three isolatesthat were close to Herbaspirillum sp. on the phylogenetic treeconstructed based on 16S ribosomal DNA (rDNA) sequences were furthercharacterized. Cell shape and width were observed by phase-contrastmicroscopy. Catalase and oxidase assays were performed by themethod of Smibert and Krieg (30). The ability of the bacteriato grow on various carbon substrates was assayed in M70 minimalmedium (12) supplemented with 1% (wt/vol) of the appropriatecarbonsubstrate.

Fluorescent labeling of diazotrophic bacteria. To confirm the endophytic features of Herbaspirillum sp. strain B501, we incorporated DNA sequences encoding the green fluorescentprotein (GFP) into the bacteria. Plasmid pUTgfpx2 (34) containingthe gfp minitransposon, which expresses gfp genes downstream ofa constitutive promoter, PpsbA, was transferred into strain B501isolated from wild rice. This plasmid carried two tandem copiesof gfp and kanamycin resistancegenes.

Competent cells were prepared and electroporated by the methods of Unge et al. (34). Herbaspirillum sp. strain B501 wascultured in 10 ml of nutrient broth medium (Difco). Samples (1ml) of the subculture were transferred to 1,000-ml flasks containing200 ml of nutrient broth medium and incubated at 30°C with shaking.Cells at stationary phase were chilled on ice separately and harvestedby centrifugation at 3,000 × g for 10 min at 4°C. Each pelletwas then washed twice with 200 ml of cold, sterilized distilledwater and resuspended in 500 µl of cold, sterile 10% glycerol-water.The cell suspension was dispensed in 100-µl aliquots and storedat $-$ 80°C until use. The competent cells (100 µl) were thawed onice, and 200 ng of purified gfp delivery plasmid pUTgfpx2 wasadded to the cells and mixed quickly. The mixture was incubatedon ice for 15 min and transferred to a sterile, prechilled cuvette(0.2-cm interelectrode gap) and placed in the Gene Pulser II apparatusequipped with a Pulser Controller (Bio-Rad Laboratories, Tokyo,Japan). The electroporation unit was used at the following settings:12.5 kV/cm, 25 µF, and 200 $Omega$ . Following the pulse, the cells wereimmediately diluted with 1 ml of nutrient broth medium (Difco),transferred to the sterilized tubes, and incubated at 30°C for3 to 4 h. From each tube, 100 µl was plated onto selective nutrientagar plates containing 100 µg of kanamycin per ml. After the plateswere incubated at 30°C, green fluorescence emission was examinedwith an Olympus SZX12 fluorescence stereomicroscope with GFP band-passfilter unit SZX-FGFPA (excitation wavelength ,460 to 490 nm; emissionwavelength, 510 to 550nm).

Rice growth media. Nitrogen-free medium (20a) was used for colonization and nitrogen fixation studies. The medium contained the following: 0.6mM NaH₂PO₄ · 2H₂O, 0.3 mM K₂SO₄, 0.3 mM CaCl₂ · 2H₂O, 0.6 mM MgCl₂· 2H₂O, and 0.045 mM FeEDTA as macroelements; 50 µM H₃BO₃, 9 µMMnSO₄ · 5H₂O, 0.3 µM CuSO₄ · 5H₂O, 0.7 µM ZnSO₄ · 7H₂O, and 0.1µM Na₂MoO₄ · 2H₂O as microelements; and 0.325% (wt/vol) agar.The pH was adjusted to 5.5. The macroelement and microelementsolutions were sterilized separately and then poured into plantboxes (350 ml) (CUL-JAR300; Iwaki, Tokyo, Japan) beforesolidification.

Rice cultivation and inoculation with Herbaspirillum sp. Dehulled seeds of O. officinalis W0012, O. rufipogon W2008, O. sativa cv. Sasanishiki, and O. sativa cv. Nipponbare were surfacesterilized with 70% ethanol for 1 min and shaken in 10% (wt/vol)calcium hypochlorite solution (high granules; Wako Pure ChemicalCo. Ltd., Osaka, Japan) for 30 min at 28°C. Seeds were then washedthree times with sterilized distilled water with shaking (15 mineach). To ensure the sterilization efficiency, seeds were subjectedto sterility checks on RMR and nutrient agar (Difco)media.

For seed inoculation, GFP-tagged Herbaspirillum sp. strain B501 was grown on nutrient broth medium (Difco), harvested at thelogarithmic phase when the turbidity (A₆₆₀) reached approximately0.9, and washed twice with sterilized distilled water. An inoculumwas prepared by resuspending the pellet in sterile saline solution,and cell density was determined by direct counting with a Thomahemocytometer. The sterilized seeds were transferred into plantboxes containing 100 ml of semisolid rice growth medium and theninoculated with GFP-tagged Herbaspirillum sp. strain B501 (10⁵ cells/seed). The plant boxes containing the inoculated seedswere then incubated in a plant growth cabinet (LH300; NK SystemCo. Ltd., Osaka, Japan) under a light-dark cycle (16 h of lightfollowed by 8 h of dark) at 25°C.

Fluorescence microscopy. Seven-day-old seedlings of wild and cultivated rice plants that were either inoculated or not inoculated were taken from theplant box, washed lightly with sterilized distilled water, andplaced separately on petri dishes. These intact seedlings werethen observed and photographed using an Olympus SZX12 fluorescencestereomicroscope. Each field was photographed under three differentconditions: optical light microscopy and fluorescence microscopywith a GFP filter unit (Olympus SZX-MGFP/Em510-) and GFP band-passfilter unit (Olympus SZX-MGFP/Em510-550).

To determine the localization of the inoculant bacteria in plant tissues, root and shoot segments of 7-day-old rice plantswere fixed for 4 h in 4% paraformaldehyde in phosphate buffersolution (10 mM sodium phosphate buffer [pH 7.2], 150 mM NaCl)at room temperature and rinsed with the phosphate buffer. Thefixed shoots and roots were cut into 80-µm-thick slices with amicroslicer (DTK-1000). The specimen was observed by a confocallaser scanning fluorescence microscope (Zeiss LSM510; Carl Zeiss,Tokyo, Japan) with a laser emitting 488-nm-wavelength light andwith a 514-nm barrier filter cutoff. Confocal images were reconstructedwith Zeiss LSM imagesoftware.

Electron microscopy. Seedlings (1 to 2 weeks old) inoculated with Herbaspirillum sp. strain B501 were observed with an Olympus SZX12 fluorescencestereomicroscope, and the infection zones were identified. Slices(1 to 2 mm thick) were taken from coleoptiles, leaves, and rootsand fixed in 2% glutaraldehyde in 0.2 M Na-cacodylate buffer (pH6.8) at room temperature in a vacuum for 2 h, washed four timeswith the same buffer, and postfixed in 1% osmium tetroxide in0.1 M Na-cacodylate buffer (pH 6.8) for 2 h. Samples were rinsedthree times with distilled water and suspended in 2% uranyl acetatefor 2 h. Samples were then rinsed again with distilled water,dehydrated through a series of ethanol solutions, embedded inSpurr's low-viscosity epoxy resin, and polymerized at 60°C for24 h. Ultrathin sections were restained with uranyl acetate andlead citrate and observed with a JEOL 100SX transmission electronmicroscope.

Inoculant population in surface-sterilized rice. To estimate the population of GFP-tagged Herbaspirillum sp. inside rice tissues, 7-day-old seedlings of O. officinalis W0012,O. rufipogon W2008, and O. sativa cultivars Sasanishiki and Nipponbareinoculated with the bacteria were surface sterilized in 1% NaOClfor 30 s. The seedlings were then quickly washed with sterilizeddistilled water and then with saline solution. The shoots, roots,and seeds of five seedlings were excised, weighed, and maceratedseparately in 0.8% saline solution. The macerate was seriallydiluted and plated on nutrient agar plates containing 50 µg ofkanamycin per ml. The green fluorescent colonies that appearedon the plates after incubation at 30°C were counted with the aidof an Olympus SZX12 fluorescencestereomicroscope.

Acetylene reduction assay of inoculated plants. Nitrogenase activity of seedlings with and without inoculation was evaluated using the acetylene reduction assay. Seven-day-oldseedlings of O. officinalis W0012 and O. sativa cv. Sasanishikiinoculated with Herbaspirillum sp. strain B501 were washed withsterilized distilled water. Each seedling was then placed in aseparate 13.8- or 33.2-ml bottle sealed with rubber septa, andthe bottles were injected with 10% (vol/vol) pure acetylene (17).Ethylene concentrations were measured at 8-h intervals for 24h using a Shimadzu GC-18A gas chromatograph as described above.We drew a graph showing ethylene concentrations over time andexamined the linearity of increase of ethylene concentrations.Ethylene evolution from uninoculated seedlings in the presenceof 10% acetylene and inoculated seedlings in the presence of airwas also assayed to discriminate acetylene reduction activityof the inoculant in planta from the background ethylene emissionof rice as a planthormone.

¹⁵N₂ gas incorporation. Ten-day-old seedlings of O. officialis W0012 inoculated with Herbaspirillum sp. strain B501 were surface sterilized in 1%NaOCl for 30 s and washed with sterilized distilled water. Theseedlings were placed into 120-ml bottles sealed with butyl rubbersepta. A gas phase composed of 40% (vol/vol) ¹⁵N₂ (99.7 atom%), 40% (vol/vol) Ar, and 20% (vol/vol) O₂ was attainedin the bottle after several replacements of 80% (vol/vol) Ar and20% (vol/vol) O₂ using a vacuum line. After 24 h at 30°C in thedark, the seedlings were taken from the bottles, dried at 70°C,and powdered using a mortar and pestle. ¹⁵N concentrations were determined in duplicate using a Thermo QuestDELTA plus XL mass spectrometer (Bremen,Germany).

Nucleotide sequence accession numbers. We deposited the sequences of diazotrophs isolated in this work under the following accession numbers to DDBJ: AB049133(strain B501), AB049103 (strain B65), AB049104 (strain B512),AB049105 (strain B508-1), AB049106 (strain B511), AB049107(strain B513), AB049108 (strain B509), AB049109 (strainB52), AB049110 (strain B506), AB049111 (strain B510), andAB049112 (strainB518).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Isolation and characterization of nitrogen-fixing bacteria from rice. From surface-washed or sterilized stems of wild and cultivated rice plants, we obtained 11 gram-negative isolates of nitrogen-fixingbacteria grown on a modified Rennie (RMR) semisolid medium (Table1; Fig. 1). They consistently showed acetylene reduction activityin the medium during isolation steps. The diazotrophic isolateswere closely related to Herbaspirillum, Ideonella, Enterobacter,and Azospirillum within Proteobacteria (Fig. 1). Isolates B65,B501, and B512 from wild rice species Oryza barthii, O. officinalis,and O. rufipogon, respectively, were closely related to Herbaspirillumspp. in $beta$ -Proteobacteria, which are known to be diazotrophic endophytesfrom sugarcane and other gramineous plants (3, 20, 23).Conversely, isolates B508-1, B511, and B513 from indica and javanicatypes of cultivated rice plants (O. sativa cultivars Kasalathand SC41, respectively) were closely related to Ideonella dechloratans(21) in $beta$ -Proteobacteria. Isolates B52, B506, B510, and B518apparently fell into an Azospirillum cluster within $alpha$ -Proteobacteria(Fig. 1). Isolate B509 clustered close to Enterobacter. All diazotrophicisolates in this study were motile and showed pectinase and cellulaseactivities except for cellulase activity of strain B511 (Table1). These traits were found when nondiazotrophic bacteria wereisolated and characterized from the stems of wild and cultivatedrice varieties previously (9).

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TABLE 1. Diazotrophic bacteria isolated from stems of wild rice and cultivated rice

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FIG. 1. Phylogenetic tree showing relatedness of nitrogen-fixing bacteria isolated from rice and their relatives in the Proteobacteria by neighbor-joining grouping of the aligned sequences of the 16S rRNA gene. Strains B4 and B29 are nitrogen-fixing bacteria previously isolated using nutrient agar medium from surface-sterilized culms of wild rice (9). To construct the phylogenetic tree, we used the 16S rRNA sequences in the DDBJ/EMBL/GenBank database from the following bacteria (accession numbers given in parentheses): Rhodococcus rhodochrous (X79288), Rhodocyclus purpureus (M34132), Herbaspirillum rubrisubalbicans (AB021424), Herbaspirillum seropedicae (Y10146), Comamonas terrigena (AB021418), Rhodoferax fermentans (D16211), Variovorax paradoxus (D30793), Aquaspirillum delicatun (AF078756), Pseudomonas saccharophila (AB021407), Leptothrix mobilis (X97071), Rubrivivax gelatinosus (D16213), Ideonella dechloratans (X72724), Citrobacter freundii (M59291), Citrobacter amalonaticus (AF025370), Citrobacter farmeri (AF025371), Enterobacter cloacae (AJ251469), Klebsiella pneumoniae (AF130981), Enterobacter asburiae (AB004744), Enterobacter cancerogenus (Z96078), Rhizobium leguminosarum (X67227), Bradyrhizobium japonicum (X87272), Rhodopseudomonas palustris (D25312), Sphingomonas paucimobilis (U37337), Azospirillum irakense (Z29583), Azospirillum amazonense (X79735), Azospirillum halopraeferens (X79731), Azospirillum brasilense NCIMB 11860T (Z29617), Azospirillum brasilense sp7 (X79739), Azospirillum lipoferum PA1 (X79738), Azospirillum largomobile (X90759), Azospirillum lipoferum ATCC 29707T (M59061), and Azospirillum lipoferum NCIMB11861T (Z29619). Bar, 0.01 base substitution per nucleotide.

Comparison of Herbaspirillum spp. with bacterial isolates from wild rice. Three nitrogen-fixing species of Herbaspirillum have previously been identified. H. seropedicae was first reported as a nitrogen-fixingbacterium associated with the roots of rice, maize, and sorghum(3). Subsequently, a mild plant pathogen in sugarcane was reclassifiedas Herbaspirillum rubrisubalbicans (1). Recently, a new species,Herbaspirillum frisingense, isolated from C₄ fiber plants wasproposed (20). We then examined whether diazotrophic isolatesB65, B501, and B512 from wild rice could be classified as anyof the known species of Herbaspirillum (Table 2).

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TABLE 2. Comparison of wild-rice-derived diazotrophic bacteria B65, B501, and B512 with nitrogen-fixing Herbaspirillum spp.^a

Basic properties including cell shape, cell size, and production of catalase and oxidase of the tested isolates were similarto those of the known species of Herbaspirillum. Utilization ofcarbon sources such as meso-erythritol and N-acetylglucosaminehas been used as criteria for species identification of Herbaspirillum(1, 3, 20). Isolates B65, B501, and B512 differed fromH. seropedicae, H. rubrisubalbicans, and H. frisingense in theutilization of meso-erythritol, N-acetylglucosamine, L-rhamnose,and meso-inositol (Table 2). Kirchhof et al. (20) developedseveral diagnostic probes of a 16S rRNA-targeted oligonucleotide(18 bp) that are specific for the genus Herbaspirillum and Herbaspirillumspecies. Complementary sequences of the diagnostic probes werecompared with DNA sequences of our 16S rRNA genes, and identitywas expressed as percentage similarity in Table 2. In terms ofthe diagnostic probe sequences, isolates B65, B501, and B512 werenot identical to H. seropedicae, H. rubrisubalbicans, and H. frisingense,although the sequences of genus-specific probes, HERB 86 and HERB1432, showed strong conservation even in the tested isolates.The results of basic properties, carbon source utilization, andthe diagnostic probe sequences (Table 2) indicated that isolatesB65, B501, and B512 cannot be classified as any known speciesof Herbaspirillum but do belong within this genus. They may benew species of Herbaspirillum, although DNA-DNA hybridizationand further description are required for accurate classification.Isolates B65, B501, and B512 are thus called Herbaspirillum sp.in thiswork.

Endophytic colonization of Herbaspirillum sp. strain B501 from wild rice. To examine endophytic behavior of Herbaspirillum sp. strain B501 isolated from O. officinalis W0012 in the original wild riceand cultivated rice plants, the gfp gene encoding GFP was introducedinto the bacteria with a gfp minitransposon pUTgfpx2 by electroporation(34). Several transformants that showed strong GFP fluorescencewere picked up, and their growth and acetylene reduction activitywere compared with the parent strain Herbaspirillum sp. strainB501. Controls not exposed to electric pulse or foreign DNA didnot produce any transformants. Consequently, we selected Herbaspirillumsp. strain B501gfp1, which showed the same growth curve in nutrientbroth medium and acetylene reduction activity in RMR semisolidmedium as the parent strainB501.

Herbaspirillum sp. strain B501gfp1 partially colonized the coleoptiles, leaves, seeds, and roots of 7-day-old seedlings ofO. officinalis W0012 and was distributed in patches (Fig. 2A andB, lanes III). Conversely, no GFP fluorescence was observed inthe seedlings of O. sativa cv. Sasanishiki, except for a weaksignal in the seed (Fig. 2C and D, lanes III). When a filter thatpasses over 510-nm-wavelength light was used (lane II), chlorophyllsemitted red autofluorescence in shoots. Yellow fluorescence mixedwith red and green fluorescence was observed exclusively in shootsof wild rice O. officinalis (Fig. 2A and C, lanes II). These observationssuggested that Herbaspirillum sp. strain B501gfp1 exclusivelycolonizes just the seedlings of wild rice O. officinalis.

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FIG. 2. Fluorescence micrographs showing distribution of GFP-tagged Herbaspirillum sp. strain B501gfp1 in 7-day-old seedlings of wild rice (O. officinalis W0012) (A and B), cultivated rice (O. sativa cv. Sasanishiki) (C and D), and intercellular colonization of the bacterium in shoots (coleoptiles) of wild rice (O. officinalis W0012) (E) when seeds were inoculated with B501gfp1. Bars = l mm (A to D) and 10 µm (E). The seedlings were observed under conditions of light field (lanes I) and fluorescence fields with a GFP filter unit (Em510-) (lanes II) and GFP band-pass filter unit (Em510-550) (lanes III). Panel E shows a confocal image by laser scanning fluorescence microscopy.

Localization of Herbaspirillum sp. strain B501 in tissues of wild rice. GFP-tagged cells of Herbaspirillum sp. strain B501gfp1 were apparently localized in intercellular spaces of shoot tissuesof 7-day-old seedlings of O. officinalis W0012 (Fig. 2E).

Transmission electron microscopy demonstrated that Herbaspirillum sp. strain B501gfp1 colonized intercellular spaces in youngtertiary leaves before the leaves expanded (Fig. 3A, B, and C)and in coleoptiles that were easily seen at this stage (Fig. 3D).Interestingly, the bacteria penetrated into very young tissuesof quaternary leaves (Fig. 3F) before leaf tissue differentiation,although they did not enter into the five-cell leaf tip (Fig.3E). No bacteria were observed in vascular tissues in shoots.Bacteria were often found outside the exodermis of roots but wererarely seen within the tissues. According to these observations,the majority of cells of Herbaspillium sp. strain B501 invadedand colonized intercellular spaces of rice shoots.

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FIG. 3. Transmission electron micrograph of transverse section through rice plant of O. officinalis W0012 seven days after seed inoculation with Herbaspirillum sp. strain B501gfp1. (A) The bacteria have invaded the shoot tissue which is a unexpanded third leaf (indicated by the two top arrows), and some bacteria were outside the leaf tissue (the lowest arrow). Bar = 10 µm. (B) High-magnification view of panel A showing bacteria colonizing the intercellular space within the rice tissue. Bar = 10 µm. (C) The bacteria colonizing the intercellular space of the third leaf of rice. Bar = 1 µm. (D) Section from rice coleoptile, showing the bacteria colonizing the intercellular space but not densely populated. Bar = 1 µm. (E) Cross section from the tip of a fourth leaf of rice shoot, showing little invasion of the undifferentiated leaf, which has only five cells. Bar = 10 µm. (F) A lower cross section from the same fourth leaf tip seen in panel E. The bacteria have entered the young fourth leaf and colonized the intercellular space (arrow). Bar = 10 µm.

Endophytic populations in surface-sterilized rice. After 7-day-old seedlings of O. officinalis W0012, O. rufipogon W2008, O. sativa cv. Sasanishiki, and O. sativa cv. Nipponbareinoculated with the bacterium were surface sterilized, the endophyticpopulations of the bacterium were measured by a colony count methodon nutrient agar medium containing kanamycin (Table 3). Therewere significantly more endophytic bacteria in the shoots of wildO. officinalis W0012 and O. rufipogon W2008 than in those of cultivatedO. sativa cultivars Sasanishiki and Nipponbare (Table 3). Thedensity of Herbaspirillum sp. strain B501 was higher in seedsof O. officinalis W0012 than in seeds of other rice varieties(Table 3). No endophytic bacteria were detected in root tissuesin this study. These results are consistent with the observationsfrom fluorescence stereomicroscopy (Fig. 2) and indicate thatHerbaspirillum sp. strain B501 prefers wild rice and particularlyprefers O. officinalis over O. sativa.

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TABLE 3. Colonization of Herbaspirillum sp. strain B501 tagged with gfp and kanamycin resistance genes in wild and cultivated rice 7 days after inoculation^a

Acetylene reduction assays of rice seedlings inoculated with Herbaspirillum sp. strain B501. Nitrogen fixation of free-living bacteria in media is quite different from their ability to fix nitrogen in planta (8,29). Therefore, the next question is whether Herbaspirillumsp. strain B501 has the ability to fix nitrogen in planta. Inthe presence of 10% acetylene, the seedlings of O. officinalisW0012 inoculated with Herbaspirillum sp. strain B501 showed significantacetylene reduction activity compared with the activity in uninoculatedplants and in inoculated plants in air (controls) (Table 4).Conversely, no significant acetylene reduction activity was observedfor O. sativa cv. Sasanishiki inoculated with B501 (Table 4).This result is perhaps not surprising, as the bacteria colonizedO. sativa cv. Sasanishiki to a lesser degree than O. officinalisW0012 (Table 3).

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TABLE 4. Acetylene reduction activity of rice seedlings inoculated with Herbaspirillum sp. strain B501gfp1^a

¹⁵N₂ gas incorporation. The acetylene reduction assay is an indirect method to verify nitrogen fixation in planta of endophytes, and the possibilityof ethylene emission from plants could not be completely excluded.Therefore, we designed a ¹⁵N dinitrogen incorporation experiment to follow ¹⁵N₂ gas into rice plants through endophytic Herbaspirillum sp.strain B501. No incorporation of ¹⁵N was detected in O. officinalis without inoculation (Table 5).Nevertheless, significant ¹⁵N incorporation from ¹⁵N gas was detected in the rice plants with inoculation. This resultclearly demonstrated that Herbaspirillum sp. strain B501 in O.officinalis fixed nitrogen within the rice plants.

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TABLE 5. Incorporation of ¹⁵N₂ into O. officinalis W0012 inoculated with Herbaspirillum sp. strain B501^a

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Many workers have isolated diazotrophic bacteria from gramineous plants using nitrogen-free media such as semisolid NFb (3).Rennie medium was proposed as a more efficient nitrogen-free mediumfor isolation of nitrogen-fixing bacteria (26). Use of a modifiedRennie medium in this study probably enabled us to isolate newnitrogen-fixing bacteria, such as close relatives of genera Herbaspirillumand Ideonella. In particular, Ideonella is a monospecific genus(I. dechloratans), which is capable of growing anaerobically withchlorate as an electron acceptor, although any ability to fixnitrogen is as yet unknown (21).

When the acetylene reduction activities of original rice seedlings inoculated with the corresponding diazotrophic bacteriawere preliminarily assayed, the combination of bacterial isolateB501 and O. officinalis W0012 showed the highest activity (datanot shown). Moreover, Herbaspirillum spp. have been found in sugarcaneand other gramineous plants (3, 23) and are possibly capableof nitrogen fixation in planta (3, 16, 25). Thus, we havefocused on the three isolates (B65, B501, and B512) that wereclosely related to Herbaspirillum spp. based on the 16S rDNA sequences.However, isolates B65, B501, and B512 did not cluster with anyknown species of Herbaspirillum but were determined to belongwithin this genus by characterization of basic properties, carbonsource utilization, and the diagnostic probe sequences (Table2), suggesting a great diversity of Herbaspirillum sp. residingin wild rice species and other gramineousplants.

Considerable progress has been made in recent years in nitrogen fixation of Acetobacter diazotrophicus (17, 29) and Azoarcussp. (8, 15, 25) using nitrogenase antibodies and severalreporter genes behind nif genes. Herbaspirillum is expected tobe responsible for nitrogen fixation in sugarcane, rice, and sorghum(16, 19, 23). Except for some acetylene reduction activityin inoculated sugarcane (17) and reaction with a nitrogenaseantibody in sorghum (19) however, there has been no direct evidenceof nitrogen fixation in rice plants. In this study, the inoculationof wild rice, O. officinalis W0012, with Herbaspirillum sp. strainB501 apparently increased ¹⁵N concentration from ¹⁵N₂ gas into the rice plants. To our knowledge, this is the firstdirect evidence that Herbaspirillum sp. fix nitrogen in Oryzaspecies. Interestingly, the degree of nitrogen fixation in plantais likely to depend on rice species (Table 4) due to variableendophytic colonization of Herbaspirillum among rice species (Table3). This suggests the presence of host specificity or preferenceof diazotrophic endophytes similar to those in microbe-plant mutualismsfound with Rhizobium and legumes (24).

James et al. (17, 19) have reported that A. diazotrophicus, H. rubrisubalbicans, and H. seropedicae colonized xylem vesselsof host plants. However, Dong et al. (7a) postulated that xylemis an unsuitable habitat for A. diazotrophicus in sugarcane fromthe anatomical and physiological points of view. In this work,Herbaspirillum sp. strain B501 never entered vascular tissues,apparently preferring the apoplast of shoot tissues, colonizingintercellular spaces. Conversely, microscopic observation andenumeration of surface-sterilized roots suggests that the bacteriumprobably colonized the root surface. Endophytic distributionsand penetration of young leaf tissues (Fig. 2 and 3) suggest thatHerbaspirillum sp. strain B501 spread in aerial parts of wildrice via apoplastic spaces. Motility and pectinase and cellulaseproduction by Herbaspirillum sp. strain B501 might be involvedin the spreading throughout shoottissues.

The increase in ¹⁵N concentration in rice plants for 24 h (0.135 atom% excess) was low compared to the concentration of ¹⁵N₂ gas used (99.7 atom%), indicating that 0.14% of total nitrogenwas derived from ¹⁵N₂ gas after the exposure for 24 h (Table 5). This value is similarto that reported in a combination of sugarcane and A. diazotrophicus.Sugarcane plants inoculated with A. diazotrophicus PA15 and PPe4showed that 0.1 to 0.5% of total nitrogen was derived from ¹⁵N₂ for 24-h spot exposure to ¹⁵N₂ in a nitrogen-deficient condition (29). However, ¹⁵N isotope dilution studies have shown that sugarcane can fix substantialamounts of N₂, up to 70% of nitrogen requirements of the plant,although the amount of fixed nitrogen is dependent on environmentalconditions (6, 16). Therefore, it is possible that plantstage and environmental conditions affect the amount of nitrogenfixation by endophytes. In this work, young seedlings of the inoculatedrice plants were evaluated for nitrogen fixation. Therefore, furtherexperiments of ¹⁵N incorporation and ¹⁵N isotope dilution using mature rice plants with and without inoculationof Herbaspirillum sp. strain B501 would shed light on the realcontribution of nitrogen fixation by thebacterium.

	ACKNOWLEDGMENTS

This work was supported in part by grants (to K.M.) from PROBRAIN, the Ministry of Education, Science, Sports and Cultureof Japan (grant 98460), Mayekawa MFG Co., and the Joint ResearchProgram of the Institute of Genetic Ecology, Tohoku University(grant 981002). A.E. was supported by a research fellowship foryoung scientists from the Japan Society for the Promotion of Science,for which we aregrateful.

We thank K. Yuhashi (Plant Biotechnology Institute, Ibaraki Agricultural Center) and M. Saito (National Institute of Livestockand Grassland Science) for their help with confocal laser scanningmicroscopy, J. K. Jansson (Stockholm University) for kindly providingplasmid pUTgfpx2, and S. Harayama (Marine Biotechnology Institute,Kamaishi Laboratories) for his continuing interest andencouragement.

	FOOTNOTES

^* Corresponding author. Mailing address: Institute of Genetic Ecology, Tohoku University, Katahira, Aoba-ku, Sendai 980-8577,Japan. Phone: 81-22-217-5684. Fax: 81-22-263-9845. E-mail: kiwamu{at}ige.tohoku.ac.jp.

Present address: Faculty of Agriculture, Minufiya University, Minufiya, Shebin Elkom,Egypt.

Present address: Laboratory of Plant Molecular Genetics, Nara Institute of Science and Technology, 8916-5 Takayama, Ikoma630-0101,Japan.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Baldani, J. I., B. Pot, G. Kirchhof, E. Falsen, V. L. D. Baldani, F. J. Olivares, B. Hoste, K. Kersters, A. Hartmann, M. Gillis, and J. Döbereiner. 1996. Emended description of Herbaspirillum; inclusion of [Pseudomonas] rubrisubalbicans, a mild plant pathogen, as Herbaspirillum comb. nov.; and classification of a group of clinical isolates (EF group 1) as Herbaspirillum species 3. Int. J. Syst. Bacteriol. 46:802-810[Abstract/Free Full Text].
2.	Baldani, J. I., L. Caruso, V. L. D. Baldani, S. Goi, and J. Dobereiner. 1997. Recent advances in BNF with non-legume plants. Soil Biol. Biochem. 29:911-922[CrossRef].
3.	Baldani, J. I., V. L. D. Baldani, L. Seldin, and J. Dobereiner. 1986. Characterization of Herbaspirillum seropedicae gen. nov., sp. nov., a root-associated nitrogen-fixing bacterium. Int. J. Syst. Bacteriol. 34:451-456.
4.	Baldani, V. L. D., and J. Dobereiner. 1980. Host-plant specificity in the infection of cereals with Azospirillum spp. Soil Biol. Biochem. 12:433-439[CrossRef].
5.	Barraquio, W. L., L. Revilla, and J. K. Ladha. 1997. Isolation of endophytic bacteria from wetland rice. Plant Soil 194:15-24[CrossRef].
6.	Boddy, R. M. 1995. Biological nitrogen fixation in sugarcane: a key to energetically biofuel production. Crit. Rev. Plant Sci. 14:263-279.
7.	Dawe, D. 2000. The potential role of biological nitrogen fixation in meeting future demand for rice and fertilizer, p. 1-9. In J. K. Ladha, and P. M. Reddy (ed.), The quest for nitrogen fixation in rice. International Rice Research Institute, Los Banos, Philippines.
7a.	Dong, Z., M. E. McCully, and M. J. Canny. 1997. Does Acetobacter diazotrophicus live and move in the xylem of sugarcane stems? Anatomical and physiological data. Ann. Bot. 80:147-158[Abstract/Free Full Text].
8.	Egener, T., T. Hurek, and B. Reinhold-Hurek. 1998. Use of green fluorescent protein to detect expression of nif genes of Azoarcus sp. BH72, a grass-associated diazotroph, on rice roots. Mol. Plant-Microbe Interact. 11:71-75[Medline].
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