Role of a Ferredoxin Gene Cotranscribed with the nifHDK Operon in N2 Fixation and Nitrogenase "Switch-Off" of Azoarcus sp. Strain BH72

doi:10.1128/JB.183.12.3752-3760.2001

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Journal of Bacteriology, June 2001, p. 3752-3760, Vol. 183, No. 12
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.12.3752-3760.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Role of a Ferredoxin Gene Cotranscribed with the nifHDK Operon in N₂ Fixation and Nitrogenase "Switch-Off" of Azoarcus sp. Strain BH72

Tanja Egener,¹^, Dietmar E. Martin,² Abhijit Sarkar,² and Barbara Reinhold-Hurek¹^,²^,^*

Symbiosis Research Group, Max Planck Institute for Terrestrial Microbiology, D-35043 Marburg,¹ and Laboratory of General Microbiology, Faculty of Biology and Chemistry, University of Bremen, D-28334 Bremen,² Germany

Received 16 January 2001/Accepted 27 March 2001

	ABSTRACT

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The endophytic diazotroph Azoarcus sp. strain BH72 is capable of infecting rice roots and of expressing the nitrogenase (nif)genes there. In order to study the genetic background for nitrogenfixation in strain BH72, the structural genes of nitrogenase (nifHDK)were cloned and sequenced. The sequence analysis revealed an unusualgene organization: downstream of nifHDK, a ferredoxin gene (fdxN;59% amino acid sequence identity to R. capsulatus FdxN) and openreading frames showing 52 and 36% amino acid sequence identityto nifY of Pseudomonas stutzeri A15 and ORF1 of Azotobacter vinelandiiwere located. Northern blot analysis, reverse transcriptase PCRand primer extension analysis revealed that these six genes arelocated on one transcript transcribed from a $sigma$ ⁵⁴-type promoter. Shorter transcripts sequentially missing genesof the 3' part of the full-length mRNA were more abundantly detected.Mutational analyses suggested that FdxN is an important but notthe essential electron donor for dinitrogenase reductase. An in-framedeletion of fdxN resulted in reduced growth rates (59% ± 9%) andnitrogenase activities (81%) in nitrogen-fixing pure culturesin comparison to the wild type. Nitrogenase activity was fullycomplemented in an fdxN mutant which carried a nifH promoter-drivenfdxN gene in trans. Also, in coculture with the ascomycete Acremoniumalternatum, where strain BH72 develops intracytoplasmic membranestacks, the nitrogenase activity in the fdxN deletion mutant wasdecreased to 56% of the wild-type level. Surprisingly, the fdxNdeletion also had an effect on the rapid "switch-off" of nitrogenaseactivity in response to ammonium. Wild-type strain BH72 and thedeletion mutant complemented with fdxN in trans showed a rapidreversible inactivation of acetylene reduction, while the deletionmutant did not cease to reduce acetylene. In concordance withthe hypothesis that changes in the redox state of NifH or electronflux towards nitrogenase may be involved in the mechanism of physiologicalnitrogenase switch-off, our results suggest that the ferredoxinmay be a component involved in thisprocess.

	INTRODUCTION

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In addition to the root surface, inner tissues of roots may also be colonized by bacteria. Endophytic diazotrophic bacteriainvade roots and shoots of grasses without causing symptoms ofplant disease (23, 46). Establishment in inner tissues ofagriculturally important crops such as sugar cane or rice hasbeen shown for several gram-negative bacteria, such as Herbaspirillumseropedicae (23, 24), Acetobacter diazotrophicus (25), andAzoarcus spp. (19).

Azoarcus sp. strain BH72, which was isolated from the endorhizosphere of Kallar grass in Punjab, Pakistan (45), is alsocapable of infecting roots of rice seedlings in the laboratory(19). Reporter gene studies have demonstrated that nitrogenase(nif) genes of Azoarcus spp. can be expressed endophytically inthe aerenchyma of these seedlings, suggesting that the interiorof rice roots provides a microenvironment suitable for nitrogenfixation (6). Expression of nifHDK genes (6) as well asnitrogenase activity (16) requires low concentrations of oxygenand ammonium (below 0.5 mM); however, anaerobic conditions donot permit nitrogen fixation in this strictly respiratorybacterium.

Azoarcus sp. strain BH72 is unusual in that it can shift into a state of "hyperinduction" under certain growth conditionsthat include extremely low oxygen concentrations (30 nM). Moreover,in contrast to other Proteobacteria, this strain harbors threeinstead of two copies of P_II-like proteins, the central signaltransmitters of nitrogen metabolism (37). Hyperinduction ofstrain BH72 is characterized by increased activity and efficiencyof nitrogen fixation (18), appearance of intracellular membranestacks (diazosomes), and association of the iron protein of nitrogenasewith diazosome membranes (20). Diazosome formation can be inducedreproducibly in the laboratory by cocultivating Azoarcus sp. strainBH72 with the ascomycete Acremonium alternatum, which was isolatedfrom the root interior of Kallar grass as well (17). The cellsattach to the fungal mycelium, and the fungal respiration mayprovide sufficiently microaerobic niches for diazosome formation.The association of nitrogenase with these membranes suggests thatthey are involved in efficient nitrogen fixation, possibly byproviding a more efficient electron flux to nitrogenase (20).

The electrons required to reduce N₂ are carried to nitrogenase by either flavodoxins or ferredoxins. Little is known aboutthe generation of reductant for N₂ fixation in nonphototrophicbacteria. While the NifJF pathway via a pyruvate:flavodoxin oxidoreductasewas characterized for Klebsiella pneumoniae (41), the generationof low-redox-potential electron carriers for nitrogenase reductionin many heterotrophic diazotrophs remains unclear. Nevertheless,the immediate molecule donating electrons to nitrogenase reductasehad been identified for many diazotrophs. While in gram-positivebacteria (10) and in cyanobacteria (53) [2Fe-2S] ferredoxinshave been shown to supply electrons to nitrogenase, the groupof Proteobacteria favors more or less nif-specific 2[4Fe-4S] ferredoxins(30, 52). Some of the genes encoding these ferredoxins havebeen found to be localized in an operon with nif genes (otherthan nitrogenase genes) and are therefore regulated in a nif-dependentmanner (26, 33).

In order to analyze nitrogen fixation in Azoarcus sp. strain BH72 genetically, nitrogenase structural genes were cloned andsequenced in the present study, revealing strong homologies withknown nif genes of other Proteobacteria. In contrast to most otherbacteria, strain BH72 was found to cotranscribe a ferredoxin genewith the structural nifHDK genes. Mutational analysis revealedthat the ferredoxin is not obligatory for nitrogen fixation. However,it is essential for the rapid "switch-off" of nitrogenase activityin response to ammonium addition and thus a newly identified componentinvolved in thisprocess.

	MATERIALS AND METHODS

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Bacterial strains and plasmids. The strains and plasmids used in this study are listed in Table 1. Azoarcus strain BH72 originated from roots of Kallar grass,Leptochloa fusca (L.) Kunth (45).

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TABLE 1. Bacterial strains and plasmids

Culture media and growth conditions. If not stated otherwise, Azoarcus sp. strain BH72 was grown at 37°C in VM medium supplemented with ethanol (47, 48). Fornitrogen fixation in pure culture, the cells were grown microaerobicallyin N-free SM medium (44) in a closed batch culture (32) or,for mixed-culture growth experiments, in a 2-liter fermentor (BiostatB; Braun Biotech, Melsungen, Germany) equipped with a regulatedoxygen supply set at 0.1% O₂ in N₂, and stirred at 600 rpm. Thecells were precultured overnight in SM medium supplemented with0.01% yeast extract and 0.05% ammonium chloride, washed threetimes in N-free SM medium, and inoculated at an optical densityat 578 nm (OD₅₇₈) of 0.02 in the fermentor. Cells were harvestedat the late exponential growth phase (OD₅₇₈ of 1.5) after sixgenerations. Cocultures with the ascomycete Acremonium alternatumwere carried out as described previously (20), with wild-typeand mutant cells added to the cultures in the same amounts. Theflasks were sealed with gas-tight rubber stoppers and incubateduntil the oxygen in the headspace had decreased from initiallyatmospheric concentrations to approximately 2%. This occurred5 to 8 days afterinoculation.

Analysis of bacterial growth and nitrogen fixation. To analyze the growth of the $Delta$ fdxN mutant strain compared to that of the wild type under exactly the same growth conditions,the strains were coinoculated in the fermentor in equal amounts.Growth parameters were as described above. Culture samples ofthe mixed culture were taken at different time points during exponentialgrowth, diluted in saline (0.9% NaCl), and plated on VM agar platesto give approximately 200 colonies per plate. These colonies wererestreaked on Hybond N membranes in six replicates of 30 randomlypicked colonies in the first experiment. Thus, 180 colonies totalfrom each time point were used for colony hybridization, usinga digoxigenin-labeled fdxN probe (fragment amplified with primersTE29 and TE30) to differentiate mutant colonies from the wildtype and thereby determine the ratio of both cell types (standarddeviations are given for the six replicates at 11 and 15 h inFig. 4). In two more independent fermentor experiments, only thefirst and the last time points were evaluated in this way (standarddeviations are given in Fig. 4 for all three independent experiments).Growth rates for individual strains were estimated from calculatingcell densities of the mutant and the wild type according to thepercentage of distribution obtained by colony hybridization atdifferent timepoints.

To analyze the mutant phenotype in cocultures with the ascomycete, independent cultures of wild-type and mutant strains weregrown. Nitrogen-fixing capacity was measured using the acetylenereduction assay (32) 5 to 8 days after inoculation as describedbelow, and the amount of ethylene formed per vial was determinedby gas chromatography. The oxygen concentration in the headspacewas also determined by gas chromatography (32). Cultures hadbeen inoculated with equal amounts of bacterial cells (8 × 10⁸ per ml [5]), which do not grow significantly in coculturebut adhere to the fungal mycelium (approximately 20 mg per culture),reduce acetylene, and form dumbbell-shaped, diazosome-containingcells which appear to be arrested in cell division (reference20 and unpublished results). Acetylene reduction of cultureswas estimated in three independent experiments with three to fivereplicates. To demonstrate an equal yield of bacterial proteinfrom both wild-type and mutant cultures in coculture with theascomycete, in which fungal mycelium and bacteria cannot efficientlybe separated from each other, equal volumes of cultures were harvestedand roughly disrupted in a kitchen blender (Braun) for 30 s. Thebacteria and fungal debris were sedimented by centrifugation at20,000 × g for 2 min and resuspended in sample treatment bufferto give 140 mg (fresh weight) per ml. After addition of 1% sodiumdodecyl sulfate, the cells were incubated at 95°C for 5 min andcentrifuged at 20,000 × g for 5 min to pellet DNA and cell debris.The clear protein-containing supernatant was used for sodium dodecylsulfate-polyacrylamide gel electrophoresis and Western blot analysis,using antibodies against the iron protein of nitrogenase (kindlyprovided by R. Ludden, University of Wisconsin, Madison) to differentiatebacterial from fungalprotein.

For analysis of switch-off of nitrogenase activity, nitrogen-fixing cells were grown in closed batch culture overnight asdescribed above and then transferred to fresh N-free SM medium(5 to 15 ml of culture to give 30 ml total) in sealed Erlenmeyerflasks adjusted to 1% O₂ and 1% acetylene in the headspace. Acetylenereduction and optical density were monitored before and afteraddition of NH₄Cl (2 mM finalconcentration).

Statistical evaluations were carried out using the GraphPad Instat software, applying the Student t test or the Tukey-Kramermultiple comparisontest.

Techniques for DNA and RNA manipulation. General techniques for DNA analysis were carried out according to standard protocols (3, 47). Homologous DNA gene probesfor Southern and Northern blot analysis were digoxigenin labeledin a PCR using a digoxigenin labeling and detection kit (Boehringer,Mannheim, Germany). Primer sequences are given in Table 2. ForNorthern blot analysis, RNA was isolated from exponentially growingbacterial cells by the hot phenol method (1), and Northernblot analysis was carried out according to standard protocols(3, 47). Reverse transcriptase PCR (RT-PCR) was carried outwith 1.5 µg of RNA using Ready-To-Go RT-PCR beads (Amersham PharmaciaBiotech) according to manufacturer's instructions, using primersnifKfw and Fdxrev (Table 2) for the RT reaction at 42°C for 20min and inactivation at 95°C for 5 min, followed by the PCR with35 cycles of denaturation at 95°C for 1 min, annealing at 55°Cfor 1 min, and extension at 72°C for 1 min.

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TABLE 2. Primers used

Primer extension was carried out with a CY5-labeled primer (TH25rCy) (Table 2) according to standard protocols (3) with20 µg of RNA isolated from nitrogen-fixing cells, using an automatedsequencer (ALFexpress; Amersham Pharmacia Biotech) for productanalysis.

DNA sequencing and computational analysis. DNA sequencing was carried out as described by Sanger et al. (51). Primers were ³⁵S labeled and sequencing was carried out using the DNA sequencingkit Sequenase, version 2.0 (Amersham, Braunschweig, Germany).Products were separated on an 8% acrylamide gel (GENE-PAGE; Amresco,Solon, Ohio) and detected by autoradiography. Alternatively, CY5-labeledprimers were used for sequencing with an automated sequencer asdescribed by Hurek et al. (15).

Construction of fdxN mutants of Azoarcus sp. strain BH72. The construction of an fdxN in-frame deletion is depicted in Fig. 1. Plasmid pEN94, which carries the genomic region of thefdxN gene, was digested with BsmI and EcoRI. The sticky ends ofthe restriction fragments were blunted using Klenow large fragment,which removed the 3' overhang of the BsmI site and filled the5' overhang at the EcoRI site. The blunt ends were religated,yielding a stop codon that interrupted the translation of thefdxN gene after the seventh amino acid. The mutation was confirmedby sequence analysis and reintroduced into pEN9 by cloning theKpnI/BamHI insert of pEN94 $Delta$ fdxN into pEN9 digested with the samerestriction endonucleases, yielding pEN9 $Delta$ F. The mutation was introducedinto the Azoarcus sp. strain BH72 chromosome by allelic exchangemutagenesis. Specifically, the plasmid pEN9 $Delta$ F, which does notreplicate in Azoarcus spp., was integrated into the chromosomeby a single homologous recombination event after electroporation.Recombinants carrying the vector-borne Ap^r gene were used for a second recombination event: colonies werereplica plated on medium with and without antibiotic and screenedfor cells that had lost the vector-encoded resistance. Six in5,000 colonies tested which had lost the vector were tested forthe fdxN deletion by PCR with primers TE14 and TE18. These primersamplified a 609-bp fragment in the wild type, while the mutantshowed a 373-bp product. Two of six double recombinants had exchangedthe wild-type for the mutagenized gene (strain BH $Delta$ fdxN).

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FIG. 1. Gene organization of the nifHDK locus. The restriction map of the nifHDK operon in Azoarcus sp. strain BH72 shows nif gene-containing clones from a genomic library above and the construction of the fdxN deletion (pEN9 $Delta$ F) below the map. The bold arrow indicates the promoter region, and the light arrow shows the position of fdxN in plasmid pEN94. Sequences with inverted repeats for stem-loop formation are indicated by hairpins below the map. S, SalI; E, EcoRI; P, PstI; X, XhoI; K, KpnI; Bs, BsmI; Sm, SmaI; B, BamHI.

To complement the mutation, the fdxN gene was genetically fused to the original nifH promoter and provided in trans. The codingsequence and the promoter region were both amplified by PCR usingPfu polymerase (Stratagene) and the primers (Table 2) fdxpro2(PstI)and fdxprorev(BamHI) at 64°C with 1.5 mM MgCl₂ for the promoterregion or fdxvor(BamHI) and TE36(EcoRI) at 53°C with 1.5 mM MgCl₂for the coding sequence. The two amplified fragments were restrictiondigested with PstI/BamHI or EcoRI/BamHI, respectively, and clonedinto PstI/EcoRI-digested vector pUC19, the two PCR fragments beingfused at the BamHI site. A clone of the correct sequence was subclonedinto the broad-host-range plasmid pLAFR3 (56) after EcoRI/PstIdigestion, yielding plasmid pfdxN, which was conjugated into strainBH72 by triparental mating. Since the fragments provided in transwere very short (400 to 600 bp), a double recombination eventof fdx into the chromosome wasunlikely.

Nucleotide sequence accession number. The sequences of the nifHDK operon were submitted to GenBank (accession no. AF200742).

	RESULTS

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Characterization of the nifHDK-fdxN region of Azoarcus sp. strain BH72. The nitrogenase genes of Azoarcus sp. strain BH72 were obtained by screening a genomic library in pUC19 (Sau3A1-digested DNAcloned into the BamHI site [47]) with a heterologous nifH geneprobe of Azorhizobium caulinodans. The resulting plasmids carryingthe nifHDK region and results of the sequence analysis of 6.5kb are shown in Fig. 1. Southern hybridization assays at low stringencywith either a homologous nifH or nifK probe indicated that thesenif genes are present in a single copy on the chromosome of Azoarcussp. strain BH72 (data not shown). Nitrogenase structural geneproducts showed the highest homology to the FeMo nitrogenase fromAzotobacter spp., with 88% identity to NifH of Azotobacter chroococcum(27) and 82% identity to NifD and 77% identity to NifK of Azotobactervinelandii (21). Downstream of the nif genes, a sequence codingfor a 2[4Fe-4S] ferredoxin was detected which was most closelyrelated to the ferredoxin FdxN from Rhodobacter capsulatus, with59% amino acid identity (11, 29). Downstream of this fdxNgene, a nifY homologue (52 and 42% amino acid identity to NifYof Pseudomonas stutzeri A15 and A. vinelandii, respectively) andan open reading frame (ORF1) with weak amino acid identity (36%)to an open reading frame (named ORF1) from the A. vinelandii nifregion (21) werefound.

The upstream untranslated region of the nifHDK region harbored sequence homologies to the consensus of $sigma$ ⁵⁴-dependent promoters (Fig. 2A). Sequences for putative NifA bindingsites (or putative upstream activating sequences) were detectedapproximately 120 and 140 bp upstream of the $sigma$ ⁵⁴ promoter. Putative ribosome binding sites (RBS) in Azoarcus sp.strain BH72 contained a minimal consensus of four or five bases(aGGAG) at a 6- or 7-base distance from the possible start codon(Fig. 2A), which is ATG. The transcriptional start site was verifiedby primer extension studies (Fig. 2B).

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FIG. 2. Promoter region of nifHDK. (A) Sequence of the genomic region upstream of nifH and of the fusion of the promoter region of nifH fused to fdxN in plasmid pfdxN. The arrow indicates the putative transcription start site, and the unlabeled box indicates the possible start codon. Regulatory sequences are boxed and labeled: UAS, putative upstream activating sequence; $-$ 12/ $-$ 24 region, putative $sigma$ ⁵⁴-dependent promoter region; RBS, putative Shine-Dalgarno sequence of nifH. The putative RBS of the other genes of the nifHDK region are given at the bottom, as well as the sequence of the fusion region in plasmid pfdxN. (B) Primer extension analysis localizing the transcriptional start at minute 158.6, corresponding to nucleotides 541/542 (159 and 158.2 min). Top, sequencing reaction; bottom, primer extension.

Analysis of the nifHDK mRNA. Nitrogenase genes in Azoarcus sp. strain BH72 are clustered in a region of approximately 6.3 kb (Fig. 1) covering six openreading frames. Since putative promoter sequences were detectedonly upstream of the nifH gene, these genes are likely to be partof the sameoperon.

In order to analyze whether the six genes formed one transcriptional unit, Northern blot analysis of RNA extracted from Azoarcussp. strain BH72 was carried out with gene probes targeted to differentgenes of the nifHDK region (Fig. 3). All four probes hybridizedonly to RNA extracted from N₂-fixing cells, where they detectedseveral apparently overlapping transcripts. A fragment of approximately6 kb which is the same size as the entire nifH-orf1 region wasdetected with an orf1 probe; however, the signal was weak, requiringlong exposure times. An RNA fragment of the same length hybridizedwith the fdxN probe; however, with this probe a stronger hybridizationsignal appeared at approximately 5 kb, corresponding in size tothe nifH-fdxN region (Fig. 3). A nifK probe hybridized with threefragments of 6.5, 5, and 4.3 kb, the latter corresponding in sizeto the nifH-nifK region, which was most intensely stained. Lowestexposure times were required for the nifH probe, which hybridizedmost strongly with a 1.15-kb band (corresponding to nifH alone)and less intensely with the 4.3-kb fragment (Fig. 3). This mRNAhybridization pattern indicated that all genes are localized onone large transcript, which occurs, however, at low abundance.Shorter transcripts sequentially missing genes of the 3' partof the region were more abundant, which might be due to multipletranscriptional termination sites or sequential degradation ofthe original transcript from its 3' end in defined steps.

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FIG. 3. Analysis of the nifHDK mRNA. (A) Northern blot analysis with RNA from Azoarcus sp. strain BH72 cells grown aerobically (lanes a) in VM medium containing combined nitrogen and microaerobically (lanes b) on N₂. Hybridization was carried out with probes directed against nifH, nifK, fdxN, and ORF1 as indicated above the lanes. Blank areas in lanes are of the sizes of rRNA. (B) RT-PCR using RNA of N₂-fixing cells of strain BH72 and primers annealing to nifK and fdxN, spanning 384 bp. Products were separated on a 1.5% agarose gel. Lane 1, size marker (lambda DNA digested with PstI); lane 2, negative control (no RNA added); lane 3, RT inactivated by incubation at 95°C for 5 min prior to addition of 1.5 µg of RNA; lane 4, 1.5 µg of RNA added without heat inactivation; lane 5, 60 ng of chromosomal DNA of strain BH72 added to the RT-PCR mixture.

To prove that the nifHDK operon was transcriptionally linked with downstream genes, a PCR involving an RT step was carriedout with RNA of the nitrogen-fixing strain BH72. The first primerfor the RT reaction and the PCR was designed to anneal to the5' end of the ferredoxin gene, while the second primer was targetedto nifK. An RT-PCR product of the expected size was detected onlyin the presence of RNA and active RT (Fig. 3B, lane 4) and notafter heat inactivation of RT (control for DNA contamination)(lane 3) or without addition of RNA (lane2).

Role of the ferredoxin FdxN in nitrogen fixation. In order to investigate the role of the nif operon-encoded ferredoxin in nitrogen fixation, we constructed an in-frame deletionmutant of fdxN in Azoarcus sp. strain BH72. The mutant (BH $Delta$ fdxN)was still able to fix nitrogen in semisolid (0.2% agar) N-freemedium. Whether nitrogen fixation reached wild-type levels waselucidated by quantitation of growth rates under nitrogen-fixingconditions.

To subject the wild type and the $Delta$ fdxN mutant of Azoarcus to exactly the same growth conditions, the strains were cultivatedin a mixed culture on N₂ in an oxygen-controlled bioreactor atinitially identical cell numbers. The culture was grown to anOD₅₇₈ of ~1.5, corresponding to six generations of bacterial growth(Fig. 4A). In three independent experiments, cultures were testedfor the distribution of the different genotypes at the first andthe last time points by colony hybridization with a probe directedagainst the fdxN gene of strain BH72; in one experiment this wastested at several time points (Fig. 4B). While the proportionsof wild-type and mutant strains were approximately 50% in thebeginning of the experiment, the relative amount of the $Delta$ fdxNmutant decreased during the course of the experiment (Fig. 4B).After 20 h or six generations, the wild type dominated the cultureby a ratio of 4:1. Calculations of individual growth rates fromthese data revealed that the mutant BH $Delta$ fdxN had only 59% ± 9%of the growth rate of the wild type.

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FIG. 4. Growth comparison of the wild type and the fdxN deletion mutant in mixed culture. The wild type and the fdxN deletion mutant were grown in an oxygen-controlled bioreactor on N₂ in mixed culture. (A) Growth measured as turbidity (OD₅₇₈). (B) Relative amount of each of the two strains at different time points during exponential growth of the mixed culture, determined by colony hybridization. Black bar, wild type; white bar, fdxN deletion strain. Values are means with standard deviations. For details of the calculations, see Materials and Methods.

To investigate whether this growth deficiency was due to a decreased electron flux to nitrogenase or to other cellular processes,quantitative measurements of nitrogenase activity were carriedout. To verify that the deficiency was due solely to the lackof FdxN and not to the destabilization of the nifHDK transcript,we complemented the fdxN gene in trans under the control of thenifH promoter of strain BH72, which was cloned into the mobilizablebroad-host-range plasmid pLAFR3 to create pfdxN. Wild-type andmutant cells were precultured on N₂ in separate closed batch culturesand then transferred to fresh medium in microaerobic flasks (1%O₂) at 37°C (two experiments with three replicates each); after3 h of incubation, acetylene (5%) was added, and the ethyleneformation was quantified by gas chromatography after 1 h of incubation.While the wild type reduced 29.4 ± 2.4 µmol of acetylene/h/mgof protein, the fdxN deletion mutant reached significantly lowervalues (P < 1%) of 23.9 ± 1.5 µmol of acetylene/h/mg of protein.This corresponded to approximately 81% of the wild-type nitrogenaseactivity rate. The complemented strain BH $Delta$ fdxN(pfdxN) restoredthe rates to 32.3 ± 1.7 µmol/h/mg of protein (110%, not significantlydifferent from the wild-type value). Thus, a decrease in nitrogenaseactivity was observed which could be fully complemented by addingthe fdxN gene in trans, suggesting that nitrogenase activity andthus also growth on N₂ were specifically affected by an impairedelectron flow due to the lack of fdxN in strainBH72.

Because the diazotrophic growth was not completely abolished by the deletion of fdxN, we speculated that other electron donors,either other ferredoxins or flavodoxins, may be present in Azoarcussp. strain BH72. In search of other, related ferredoxin geneschromosomal DNA was hybridized with a fdxN gene probe at low stringency.Specific hybridization signals were not observed at a hybridizationtemperature of 40°C with subsequent washing in 6× SSC (1× SSCis 0.15 M NaCl plus 0.015 M sodium citrate) (data not shown).Thus, highly related ferredoxins were not detectable under theseconditions. Whether flavodoxins may be alternatively used remainsto be tested in thefuture.

Role of the ferredoxin FdxN for N₂ fixation of diazosome-containing cells. Coculture of Azoarcus sp. strain BH72 with the ascomycete Acremonium alternatum 2003 leads to formation of diazosomes, whichoccur in strain BH72 in a state of augmented activity and efficiencyof nitrogen fixation (18, 20). Therefore, the effect of thefdxN mutation on nitrogen fixation was also analyzed in cocultures.The total ethylene formed per flask, measured when oxygen in theheadspace had decreased to 2% at days 5 to 7, was determined inthree independent experiments with five flasks each of strainBH72 and BH $Delta$ fdxN. Acetylene reduction of the mutant (6.9 ± 2.0µmol of ethylene formed per flask) was significantly (P < 0.0001)different from that of the wild type (12.2 ± 2.6 µmol), correspondingto 56.6% of the wild-type fixation rate. A decreased acetylenereduction activity of the mutant was observed throughout the incubationperiod (Fig. 5A), when ethylene accumulates while the oxygen concentrationdecreases from 21 to 2% due to fungal and bacterial respiration(20, 32). Western blot analyses showed that comparable amountsof nitrogenase Fe protein were present in both cultures at theend of the experiment (Fig. 5B), indicating that the differencewas caused not by decreased bacterial growth but by decreasednitrogenase activity. In both mutant and wild-type cells, diazosomeswere detected (data not shown). Accordingly, an iron protein ofnitrogenase of higher apparent molecular weight was observed (Fig.5B), which is a covalently modified protein formed in diazosome-containingcells (20).

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FIG. 5. Nitrogen fixation of the wild type and the fdxN deletion mutant in coculture. (A) Nitrogen fixation was measured as the amount of acetylene reduction per flask of Acremonium alternatum 2003 cocultured with Azoarcus sp. strain BH72 (circles) or with the mutant BH $Delta$ fdxN (squares). (B) Western blot analysis of cocultures with BH72 (lanes a) or BH $Delta$ fdxN (lanes b). Total protein extract of the coculture was diluted 2-fold (lanes 1) and 10-fold (lanes 2) and used for Western blot analysis with antibodies directed against the Fe protein of nitrogenase (34 and 37 kDa).

Effect of FdxN on rapid switch-off of nitrogenase in response to ammonium addition. Addition of 2 mM NH₄Cl to a nitrogen-fixing culture of Azoarcus sp. strain BH72 led to fast and complete (100%) inhibitionof acetylene reduction, while cultures in N-free medium continuedreducing acetylene. This nitrogenase switch-off was reversible,because nitrogenase activity was recovered within 30 to 50 minwhen only 0.2 mM ammonium was added (Fig. 6A), which was rapidlyconsumed to values below the detection limit (approximately 1µM) by the bacteria within this time (data not shown). To assesswhether the ferredoxin FdxN is involved in the process of nitrogenaseinhibition, the deletion mutant BH $Delta$ fdxN with and without complementationof fdxN in trans was tested in switch-off experiments using 2mM NH₄Cl. The complemented fdxN mutant showed almost wild-type-levelinhibition of nitrogenase activity, while the fdxN mutant continuedreducing acetylene (Fig. 6B). A rapid, complete switch-off wasthus not observed in the fdxN mutant, but a slow retardation ofnitrogenase activity which might be due to the repression of transcriptionof nifHDK genes by ammonium was observed.

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FIG. 6. Effects of ammonium addition on nitrogenase activity (acetylene reduction) of N₂-fixing cultures. (A) Reversible, fast, and complete inhibition (switch-off) of nitrogenase activity in Azoarcus sp. strain BH72 upon addition of 0.2 (closed circles) or 2 mM (open circles) NH₄Cl (final concentration). (B) Influence of ammonium addition (2 mM) on nitrogenase activity of BH72 (wild type; open circles), BH $Delta$ fdxN(pfdxN) (complemented mutant; triangles), and BH $Delta$ fdxN (deletion mutant; closed circles). Results are from one representative of three independent experiments where similar kinetics were observed.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Structural genes for the nitrogenase enzyme complex are often cotranscribed in one operon in bacteria. The structural nitrogenasegenes nifHDK in Azoarcus sp. strain BH72 occur in a single copyon a large transcript that includes three more putative open readingframes, as shown by Northern hybridization and RT-PCR. While inA. vinelandii and K. pneumoniae the nifHDK genes are followedby nifT, a gene of unknown and nonessential function for nitrogenfixation (21, 55), the downstream gene in strain BH72 showedhigh sequence identities to bacterial 2[4Fe-4S] ferredoxins. Downstreamof the fdxN gene, the operon structure resembles the situationin A. vinelandii with a nifY homologue and an open reading framewith weak homology to ORF1 (21). NifY is known to be involvedin the maturation of nitrogenase (14) or may have a role insensing and signaling the activity status of nitrogenase withrespect to regulating nifHDK mRNA stability in K. pneumoniae (54),while a mutation in ORF1 had no obvious phenotype in A. vinelandii(21).

The nifHDK operon in Azoarcus sp. strain BH72 is transcribed only under N-limiting and microaerobic conditions (6). Thisis a common feature of free-living nitrogen-fixing bacteria, mediatedby $sigma$ ⁵⁴-dependent promoters (39). Also in this Azoarcus strain, thetranscriptional start of the nifHDK mRNA corresponded in distanceto $-$ 12/ $-$ 24 promoter regions typical for $sigma$ ⁵⁴-dependent promoters. Initiation of transcription from a $sigma$ ⁵⁴-bound RNA polymerase needs to be facilitated by additional transcriptionalactivators (e.g., NifA or NtrC). Putative binding sequences forNifA were detected 120 and 140 bp upstream of the promoter region,suggesting a NifA-mediated regulation of nitrogen fixation inAzoarcus sp. strain BH72, as is commonly found in diazotrophicProteobacteria (39).

In Northern blot analysis of the nifHDK fdxN nifY ORF1 operon of strain BH72, several different transcripts were observed,the full-length transcript appearing to be least abundant. Asobserved for Azospirillum brasilense (4), the nifH transcriptappeared to be most abundant. Multiple transcripts of nifHDK mRNAwere also observed for A. vinelandii (22) and R. capsulatus(57). Inverted repeat sequences potentially capable of formingstable stem-loop structures were detected in the intergenic regionsof the latter two bacteria and also in strain BH72 between nifHD,nifK fdxN, and fdxN nifY. They might lead to differential terminationof the transcript, or, as speculated for R. capsulatus (57),they may be a target for intramolecular processing of the nifHDKmRNA. Subsequent degradation of the full-length transcript fromthe 3' end, giving stable intermediates that resisted RNA degradation,would be an alternative explanation for the transcript patternobserved in strain BH72. Formation of stem-loop structures mayassist to protect RNA from 3'-end degradation (2). Differentialstability of mRNA as a form of regulation was also demonstratedfor other bacterial gene clusters, such as the malEFG operon inEscherichia coli (40) and the puf operon in R. capsulatus (34).

The close transcriptional linkage of the ferredoxin gene fdxN with the structural nif genes may imply a role for electrontransport to nitrogenase in Azoarcus sp. strain BH72. 2[4Fe-4S]ferredoxins as electron carriers with a strong negative redoxpotential of $-$ 400 mV are known to play various roles in cellularelectron transport. Ferredoxins and flavodoxins are proposed tobe electron donors for nitrogenase in bacteria. In some organisms,such as A. vinelandii (26), R. capsulatus (52), or Sinorhizobiummeliloti (33), nif-specific ferredoxins that are encoded innif regions other than nifHDK have been identified. The S. melilotiferredoxin was shown to be essential for symbiotic N₂ fixationwith legumes. Localization of a ferredoxin gene in an operon ofstructural nitrogenase genes, which we describe here for an Azoarcussp., has been reported only for A. vinelandii, where a ferredoxin-likegene is localized downstream of vnfH, which encodes the iron proteinof vanadium nitrogenase (50).

Mutational and genetic complementation experiments in Azoarcus sp. strain BH72 showed that FdxN plays an important but notessential role in nitrogen fixation. The in-frame deletion ofthe fdxN gene reduced nitrogenase activity and diazotrophic growthin pure culture as well as nitrogen fixation of diazosome-containingcells in coculture with the ascomycete Acremonium alternatum 2003to a comparable degree (81, 59, and 56% of the wild-type rate,respectively). This defect is most likely due to a less efficientelectron transport to dinitrogenase reductase in the absence ofFdxN and not to destabilization of the nitrogenase gene mRNA,since nitrogenase activity could be fully restored by complementationof fdxN in trans. A similar nonessential role of a ferredoxinas an electron donor to nitrogenase was found, e.g., in Anabaenasp. (38), while in S. meliloti (33) and R. capsulatus (30)one ferredoxin was essential for nitrogen fixation. As no otherferredoxin gene with high sequence identity could be detectedin Azoarcus sp., it is not clear whether the residual electrontransport to nitrogenase is due to alternative ferredoxins orflavodoxins. As for Azoarcus sp., for most heterotrophic bacteriait is not yet known how ferredoxins are reduced. For R. capsulatus,the set of membrane-bound and Fe-S cluster-containing proteinsof the rnf operon has been discussed as a candidate for electrondonation to ferredoxins involved in N₂ fixation (28). The proteinsshow homology to NADH:ubiquinone oxidoreductase from Vibrio alginolyticus.(35). Analogous operons are also present in the fully sequencedgenomes of E. coli and Haemophilus influenzae and suggest a generaloccurrence in bacteria (28).

That a ferredoxin can be essential for the physiological nitrogenase inactivation as detected in the Azoarcus sp. is a novelobservation. Certain bacteria fixing N₂ react to a supply of ammoniumrapidly by inactivation of nitrogenase activity (43, 49).The so-called nitrogenase switch-off by ammonium depends on twodifferent mechanisms. In some diazotrophs, such as Rhodospirillumrubrum (43), R. capsulatus (31), and Azospirillum brasilense(9), the iron protein of nitrogenase (NifH) is subject to posttranslationalmodification, a reversible mono-ADP-ribosylation at a specificarginine residue. Additionally, a physiological switch-off mechanismwhich does not involve this covalent modification of nitrogenaseexists in some bacteria (42). The mechanism is still unknown.Here we report that such a rapid reversible physiological switch-offmechanism also occurs in Azoarcus sp. strain BH72, similar tothose in R. capsulatus and Azospirillum brasilense in terms ofspeed and extent of nitrogenase inhibition. Nitrogenase activitywas almost completely abolished within a few minutes upon additionof ammonium. In contrast, nitrogenase switch-off in Rhodospirillumrubrum occurs more slowly and is incomplete (60). In Rhodospirillumrubrum, ammonium-induced switch-off was shown to be absolutelydependent on ADP ribosylation of NifH (36, 61), whereas inR. capsulatus and Azospirillum brasilense, modification of NifHis not absolutely required, indicating a second mechanism of regulation(7, 8, 42, 58, 61). Surprisingly, the rapid completeswitch-off in response to ammonium was abolished in the fdxN deletionmutant of Azoarcus sp. strain BH72; only a slow decrease of nitrogenaseactivity was still observed. This suggested that the ferredoxinmay be part of the mechanism of the process of rapid switch-off.This would be in concordance with the hypothesis that changesin the redox state of NifH or electron flux towards nitrogenasemay be factors involved (12, 42), but no sensor or signaltransduction proteins have been identified up to now. The essentialrole of FdxN for nitrogenase switch-off also suggests that itis the major electron donor for nitrogenase in wild-type BH72:putative alternative electron donors are apparently not able tocompensate for the switch-off function in the deletion mutant,although they still allow approximately 50% of the nitrogen fixationactivity. Therefore, they are unlikely to operate in the wildtype but might be more abundant in the deletion mutant, as speculatedfor R. capsulatus (30).

	ACKNOWLEDGMENTS

We are grateful to P. W. Ludden for the kind gift of antibodies to dinitrogenase reductase of Rhodospirillum rubrum, to ThomasHurek (Max-Planck-Institut für marine Mikrobiologie, Bremen,Germany) for electron-microscopic inspection of cells for diazosomes,and to Jan Gielen in Marc Van Montagu's Laboratorium Genetika,Ghent, Belgium, for help with sequencing parts of the nifHDKoperon.

We thank the Deutsche Forschungsgemeinschaft, who supported this work (Re756/5-1/2).

	FOOTNOTES

^* Corresponding author. Mailing address: University of Bremen, Faculty of Biology and Chemistry, Laboratory of General Microbiology,P.O. Box 33 04 40, D-28334 Bremen, Germany. Phone: (49) 421-218-2370.Fax: (49) 421-218-4042. E-mail: breinhold{at}uni-bremen.de.

Present address: Freiburg University, Plant Biotechnology, D-79104 Freiburg,Germany.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Aiba, H., S. Adhya, and B. de Crombrugghe. 1981. Evidence for two functional gal promoters in intact Escherichia coli cells. J. Biol. Chem. 256:11905-11910[Abstract/Free Full Text].
2.	Alifano, P., C. B. Bruni, and M. S. Carlomango. 1994. Control of mRNA processing and decay in procaryotes. Genetica 94:157-172[CrossRef][Medline].
3.	Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.). 1987. Current protocols in molecular biology. John Wiley & Sons, New York, N.Y.
4.	De Zamaroczy, M., F. Delorme, and C. Elmerich. 1989. Regulation of transcription and promoter mapping of the structural genes for nitrogenase nifHDK of Azospirillum brasilense Sp7. Mol. Gen. Genet. 220:88-94[Medline].
5.	Dörr, J., T. Hurek, and B. Reinhold-Hurek. 1998. Type IV pili are involved in plant-microbe and fungus-microbe interactions. Mol. Microbiol. 30:7-17[CrossRef][Medline].
6.	Egener, T., T. Hurek, and B. Reinhold-Hurek. 1999. Endophytic expression of nif genes of Azoarcus sp. strain BH72 in rice roots. Mol. Plant-Microb. Interact. 12:813-819.
7.	Fedorov, A. S., O. U. Troshina, T. V. Laurinavichene, V. M. Glazer, M. M. Babykin, V. V. Zinchenko, A. F. Yakunin, and A. A. Tsygankov. 1998. Regulatory effect of ammonium on the nitrogenase activity of Rhodobacter sphaeroides and Rhodobacter capsulatus is not mediated by ADP-ribosylation of the Fe-protein of nitrogenase. Microbiology 67:610-615.
8.	Förster, B., K. Maner, F. Fassbinder, and J. Oelze. 1999. Reversible inactivation of nitrogenase in Rhodobacter capsulatus strain W107I deleted in the draTG gene region. FEMS Microbiol. Lett. 170:167-171[CrossRef].
9.	Fu, H., A. Hartmann, R. G. Lowery, W. P. Fitzmaurice, G. P. Roberts, and R. H. Burris. 1989. Posttranslational regulatory system for nitrogenase activity in Azospirillum spp. J. Bacteriol. 171:4679-4685[Abstract/Free Full Text].
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