A Cytochrome cbb3 (Cytochrome c) Terminal Oxidase in Azospirillum brasilense Sp7 Supports Microaerobic Growth

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Journal of Bacteriology, November 1998, p. 5689-5696, Vol. 180, No. 21
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

A Cytochrome cbb₃ (Cytochrome c) Terminal Oxidase in Azospirillum brasilense Sp7 Supports Microaerobic Growth

Kathleen Marchal,¹ Jun Sun,¹ Veerle Keijers,¹ Huub Haaker,² and Jos Vanderleyden¹^,^*

F.A. Janssens Laboratory of Genetics, KULeuven, 3001 Heverlee, Belgium,¹ and Department of Biochemistry, Agricultural University, 6703 HA Wageningen, The Netherlands²

Received 25 March 1998/Accepted 17 August 1998

	ABSTRACT

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Spectral analysis indicated the presence of a cytochrome cbb₃ oxidase under microaerobic conditions in Azospirillum brasilenseSp7 cells. The corresponding genes (cytNOQP) were isolated byusing PCR. These genes are organized in an operon, preceded bya putative anaerobox. The phenotype of an A. brasilense cytN mutantwas analyzed. Under aerobic conditions, the specific growth rateduring exponential phase (µ_e) of the A. brasilense cytN mutantwas comparable to the wild-type specific growth rate (µ_e of approximately0.2 h¹). In microaerobic NH₄⁺-supplemented conditions, the low respiration of the A. brasilensecytN mutant affected its specific growth rate (µ_e of approximately0.02 h¹) compared to the wild-type specific growth rate (µ_e of approximately0.2 h¹). Under nitrogen-fixing conditions, both the growth rates andrespiration of the wild type were significantly diminished incomparison to those under NH₄⁺-supplemented conditions. Differences in growth rates and respirationbetween the wild type and the A. brasilense cytN mutant were lesspronounced under these nitrogen-fixing conditions (µ_e of approximately0.03 h¹ for the wild type and 0.02 h¹ for the A. brasilense cytN mutant). The nitrogen-fixing capacityof the A. brasilense cytN mutant was still approximately 80% ofthat determined for the wild-type strain. This leads to the conclusionthat the A. brasilense cytochrome cbb₃ oxidase is required undermicroaerobic conditions, when a high respiration rate is needed,but that under nitrogen-fixing conditions the respiration ratedoes not seem to be a growth-limiting factor.

	INTRODUCTION

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Azospirillum brasilense is a gram-negative soil bacterium that lives in the rhizospheres of various plants, such as maize,wheat, and rice. When combined nitrogen is available, this bacteriumis able to grow in anaerobic, microaerobic, or aerobic conditions.Under anaerobic conditions, when NO₃ is available, denitrification provides the energy for growth(28, 29). Under microaerobic conditions, A. brasilense canreduce molecular N₂ in the absence of combined nitrogen. In aerobicor microaerobic conditions, O₂ is used as terminal electron acceptor(17). Like many other bacteria, A. brasilense has a branchedrespiratory chain. The presence of a respiratory chain that efficientlycouples electron transfer with proton pumping at low oxygen concentrationsis inferred from the attraction of A. brasilense to low oxygenconcentrations. Under these conditions, a maximal proton motiveforce is generated (3, 53). The existence of a high-affinityterminal oxidase and a second oxidase with a significantly loweraffinity in A. brasilense Sp7 was previously noted (4). Moreover,depending on the O₂ status of the culture, A. brasilense Sp7 andCd showed marked differences in cytochrome content (6, 21,31, 34). For both strains spectral analysis revealed evidencefor the presence of cytochrome b ( $alpha$ peak at 560 nm in the reduced-minus-oxidizeddifference spectrum), cytochrome c ( $alpha$ peak at 552 nm in the reduced-minus-oxidizeddifference spectrum), and a CO-binding o-like cytochrome ( $alpha$ peakat 558 nm in the reduced-minus-oxidized difference spectrum anda trough at 560 nm in the CO-reduced-minus-reduced differencespectrum) (6, 21, 34). The amounts of cytochromes b andc increased as the O₂ concentration was lowered (6, 21, 31,34). In contrast to the case for A. brasilense Sp7, a cytochromed (peak at 628 nm in the reduced-minus-oxidized difference spectrum)was found in A. brasilense Cd (34). A cytochrome a ( $alpha$ peak at603 to 605 nm in the reduced-minus-oxidized difference spectrum),observed under high aeration, was present in A. brasilense Cd(31, 34), but in A. brasilense Sp7 spectral evidence for thisoxidase seemed to be less clear and even contradictory (6,21).

The cytochrome cbb₃ cytochrome c oxidase, encoded by the fixNOQP operon in rhizobial species (18, 23, 32, 38, 50)or by a similar cco(cyt)NOQP operon in other bacteria (7, 39,43, 45), appears to be a cytochrome c terminal oxidase belongingto the heme-copper oxidase superfamily (14). In most rhizobialspecies this oxidase is essential for nitrogen-fixing endosymbiosis(18, 32, 50) and is characterized by an extremely high O₂affinity (16, 33). In the bacteria Magnetospirillum magnetoaceticumand Agrobacterium tumefaciens, and in Azorhizobium caulinodansgrowing nonsymbiotically, the cbb₃-type cytochrome c terminaloxidase seems to be at least partially responsible for the microaerobicrespiration (23, 39, 43). In Rhodobacter capsulatus, however,this oxidase drives aerobic respiration and does not functionas the obligate oxidase during microaerobic nitrogen fixation(45). Proton pumping activity of the cytochrome cbb₃ oxidasewas demonstrated in Paracoccus denitrificans (7).

The purpose of this study was the characterization of the terminal oxidase active during microaerobic growth in A. brasilense.In particular, we were interested in assessing the role of thisoxidase during nitrogen fixation.

	MATERIALS AND METHODS

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Bacterial strains, plasmids, and culture conditions. The bacterial strains used and plasmids described in this work are listed in Table 1. Escherichia coli strains were grownin Luria-Bertani medium at 37°C. To grow Azospirillum, minimalmedium (MMAB) was used (49). The nitrogen-free medium used fornitrogen fixation was the MMAB medium, devoid of NH₄Cl. Solidmedium contained 15 g of agar per liter. For conjugation YEP medium(containing 10 g of Bacto Peptone, 5 g of NaCl, and 10 g of yeastextract per liter) was used, and transconjugants of Azospirillumwere selected on MMAB medium. Antibiotics were used at the followingconcentrations: ampicillin, 100 µg/ml; kanamycin, 25 µg/ml; andtetracycline, 10 µg/ml.

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TABLE 1. Bacterial strains and plasmids

A. brasilense was grown in a chemostat of 1.8-liter capacity (Applitek). The parameters of fermentation (pH, temperature,dissolved oxygen [DO], and air flow) were controlled by the ML-4100fermentor control system (New Brunswick). All data from the ML-4100system were transmitted into a computer loaded with the ASF 2.0software (New Brunswick). DO levels were monitored with an autoclavableO₂ electrode (Ingold). During aerobic growth, the airflow ratewas set at 1.8 liters/min. According to the optimal values indicatedin the literature (30, 46, 48), a DO concentration of 2.5µM (2.5 µM DO at 30°C in sterile medium = a pO₂ of 0.006 atm)was used for growth under nitrogen-fixing conditions. In orderto maintain the DO at a constant level of 2.5 µM (microaerobicgrowth), the fermentor was sparged with a gas mixture of N₂ andair. The N₂ flow rate was set to 1.27 liters/min. The airflowrate was controlled by the ML-4100 system through a mass flowcontroller and automatically adapted according to the DO concentrationvalues. The culture was stirred at a constant rate of 400 rpm.The growth temperature during fermentation was 30°C. The pH wasmaintained at 6.8 and adjusted with an H₃PO₄ (1 M) solution duringfermentation according to the pH values measured by a pH probe(Ingold). A preculture of 100 ml, used to inoculate the fermentor,was grown in a flask of 250 ml of MMAB with NH₄⁺ at 200 rpm and 30°C until an optical density at 578 nm (OD₅₇₈)of 1.5 was reached. If cells were intended for growth in nitrogen-fixingconditions, the preculture was washed to remove residual NH₄⁺. Samples of 5 to 10 ml, used for analyzing turbidity, proteinconcentration in the cells, and residual malate and NH₄⁺ in the supernatant, were withdrawn automatically by a Biosampler(New Brunswick) during fermentation. Samples for acetylene reductionactivity were taken anaerobically at the late exponential phaseand transferred into gas-tight flasks which had been flushed withthe headspace gas of the fermentor to adjust the DO concentrationand with 10% (vol/vol) of C₂H₂ added. After an initial incubationof 30 min at 30°C and 200 rpm, the amount of ethylene producedwas measured as previously described (48). Values for the specificnitrogenase activity presented in Results are the averages fromat least three independent samples, each assayed at least fivetimes. Data were analyzed by analysis of variance.

Analyses of cells and growth medium during fermentation. Protein concentrations were determined with the bicinchoninic acid assay (42) with bovine serum albumin as a standard. Proteinvalues are the averages from two independent samples, each measuredtwice. Cell density was monitored by measuring turbidity (OD₅₇₈)on an LKB 4057 UV-visible spectrophotometer. The specific growthrate was defined as µ = ln(x₂/x₁)/(t₂ $-$ t₁), where x is OD₅₇₈,t is elapsed fermentation time (EFT), and subscripts 1 and 2 indicatedifferent sampling times. The values for µ_e (hours¹) mentioned in Results are the average values of µ during exponentialgrowth phase. L-Malate and NH₄⁺ concentrations in the supernatant were determined with test kitsfrom Boehringer Mannheim (27). The O₂ concentration in the mediumwas measured by the Winkler method (Aquamerck oxygen test combination;Merck) (24).

Isolation of membranes. Bacterial cultures grown in an oxystat under aerobic, microaerobic NH₄⁺-supplemented, and nitrogen-fixing conditions were harvested atthe beginning of the stationary phase (OD₅₇₈ of approximately1.2). Cells were subsequently centrifuged and suspended in 3 mlof 25 mM TES [N-tris(hydroxymethyl)methyl)methyl-2-aminoethanesulfonicacid]-KOH-5 mM MgCl₂ buffer (pH 6.8) containing 10 µg of RNaseper ml, 10 µg of DNase I per ml, and 1 mM phenylmethylsulfonylfluoride. Membrane vesicles were prepared as described by Haakeret al. (16).

Visible difference absorbance spectra. Visible light spectra were recorded on a dual-wavelength scanning spectrophotometer (Aminco DW2). Scanning was performed from400 to 700 nm with a 3-nm bandwidth and from 500 to 700 nm witha 1-nm bandwidth at a scan speed of 1 nm/s. For reduced-minus-oxidizedspectra, the membranes were reduced with dithionite. For the COplus dithionite-reduced-minus-dithionite-reduced difference spectra,dithionite-reduced membranes were sparged for 5 min with 100%CO. Measurements were taken after 15 min.

Recombinant DNA techniques. Standard protocols were used for cloning, restriction mapping, plasmid isolation, transformation, Southern blotting, and hybridization(36). Genomic DNA was isolated as described previously (2).PCR was performed on single colonies from A. brasilense Sp7. Theprimers used for the amplification of the cytN gene were cytplus(5'-TAGAATTCARTGGTGGTAYGGNCAYAAYGC-3') and cytminus (5'-CAGAATTCCRTTRATCATNCCSCCCCA-3').Both primers were provided with EcoRI recognition sites (boldface)to facilitate cloning procedures. The PCR was carried out in aTRIO-thermoblock (Biometra) with 0.2 mM deoxynucleoside triphosphates,1 µM each primer, and 0.025 U of Taq DNA polymerase (Boehringer)per µl. The following PCR protocol was used: a denaturation periodof 6 min at 94°C; followed by 35 cycles of 1 min at 94°C, 1 minat 52°C, and 1 min at 72°C; followed by an extension reactionof 7 min at 72°C.

A 300-bp PCR fragment was cloned in the EcoRI site of the vector pEMBL18, and it revealed an open reading frame (ORF) whosededuced product had similarity to known fixN gene products. This300-bp EcoRI insert was used as probe to screen a previously constructedgenomic library of A. brasilense Sp7 in pLAFR1 (25). One hybridizingclone (pFAJ853) with an insert of approximately 16 kb was digestedwith KpnI, and the 6-kb fragment hybridizing with the probe wassubcloned in pUC18, resulting in pFAJ860 containing the entirecytNOQP operon.

The KpnI fragment of pFAJ860 was further subcloned into pUC18 or pUCBM20 to obtain the overlapping fragments covering theentire cytNOQP operon (approximately 4 kb). All subclones weresequenced on both strands by the chain termination dideoxynucleosidetriphosphate method (37) with the AutoRead Sequencing Kit (Pharmacia-LKB)on an automated sequencer (ALF; Pharmacia-LKB), using fluorescein-labeleduniversal and synthetic oligonucleotide primers. Sequence datawere assembled and analyzed with the DNA-analyzing program PC-Gene(Intelligenetics). Sequence data banks were screened for similaritiesby using the BLAST program (1).

Mutant construction. To construct cytN insertion mutants, a 1.8-kb BamHI fragment was subcloned into pUC18, resulting in plasmid pFAJ861. A 2.5-kbaphII cassette (encoding Kanamycin resistance [Km^r]) of pHP45 $Omega$ -Km was blunt ligated in the ApaI site of pFAJ861,resulting in plasmid pFAJ862 (Km^r cassette in the same orientation as cytN [plus direction]) andpFAJ863 (Km^r cassette in the orientation opposite that of cytN [minus direction]).The resulting fragment was subsequently cloned as an EcoRI/XbaIfragment into the PstI site of the suicide plasmid pSUP202 afterblunting all sticky ends. These resulting plasmids, named pFAJ857(plus direction) and pFAJ856 (minus direction) were subsequentlymobilized from E. coli S17-1 into A. brasilense Sp7 by conjugation.Km^r A. brasilense exconjugants were screened for the loss of therecombinant plasmid and for double homologous recombination byreplica plating on the appropriate antibiotics as Km^r and tetracycline-sensitive (Tc^s) clones. Recombination at the correct location was verified bySouthern hybridization with DNA fragments from the cytN gene andthe Km^r cassette as probes. The orientation of the cassette was verifiedby Southern hybridization. In FAJ851, transcription of the Km^r cassette is in the same orientation as that of the downstreamgenes cytO and cytP, while in FAJ852, transcription of the Km^r gene is opposite to the transcription orientation of the downstreamgenes.

SDS-PAGE and heme staining. Membrane proteins, isolated as described above, were subsequently dissolved in denaturing equilibration buffer (60 mM Tris-HCl[pH 6.8], 2% [wt/vol] sodium dodecyl sulfate [SDS], 10% [wt/vol]glycerol, 28 µM bromophenol blue, 5% [vol/vol] $beta$ -mercaptoethanol)and separated by polyacrylamide gel electrophoresis (PAGE) inSDS-15% (wt/vol) polyacrylamide gels (20). Protein samples werenot heated before electrophoresis. The resulting gels were stainedfor covalently bound heme with o-dianisidine (12) before beingstained with Coomassie blue.

Nucleotide sequence accession number. The sequence of the cytNOQP operon has been submitted to the GenBank/EMBL database under accession no. AF054871.

	RESULTS

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Spectral analysis of A. brasilense membranes. Membranes were isolated from cells as described in Materials and Methods. In the reduced-minus-oxidized spectra of membranesisolated from aerobically and microaerobically grown cells (Fig.1A and C), the $alpha$ peak at 552 nm and the $beta$ peak at 522 nm are attributableto c-type cytochromes and the 560-nm ( $beta$ -peak) and 527-nm ( $beta$ -peak)shoulders are attributable to cytochromes b. In membranes of microaerobicallygrown cells, the cytochrome c peak at 552 nm was clearly morepronounced than the cytochrome b shoulder at 560 nm (Fig. 1C),suggesting a relatively high cytochrome c/cytochrome b ratio.This high level of cytochrome c was also evident from the $beta$ band(522 nm), which showed asymmetry at shorter wavelengths (Fig.1C). In the CO-binding spectrum reaction of CO with the high-spinheme is responsible for the inverted shoulder at 560 nm (Fig.1B and D). Spectral analysis revealed that the terminal oxidasesexpressed in Azospirillum cells were similar in microaerobic conditions,whether or not combined nitrogen was available in the growth medium(data not shown). In aerobic conditions (Fig. 1C) the reduced-minus-oxidizedspectrum showed a pronounced peak at 560 nm and a decreased peakat 552 nm. The CO-reduced-minus-reduced difference spectrum showeda clear inverted shoulder at 560 nm (Fig. 1D). These observationsindicate a smaller amount of cytochrome c than of cytochrome band suggest the presence of a second cytochrome b-containing oxidasepresent in aerobic conditions.

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FIG. 1. Difference spectroscopy of membrane proteins isolated from microaerobically and aerobically grown A. brasilense Sp7. (A and C) Dithionite-reduced-minus-air-oxidized spectra between 400 and 700 nm (5 mg of protein/ml) (A) and between 500 and 700 nm (3 mg of protein/ml) (C). (B and D) CO plus dithionite-reduced-minus-dithionite-reduced difference spectra between 400 and 700 nm (2 mg of protein/ml) (B) and between 500 and 700 nm (2 mg of protein/ml) (D).

Analysis of the DNA sequence and the deduced amino acid sequences. Identification of the genes encoding this potential cytochrome cbb₃ oxidase was done by a PCR-based cloning procedure as describedin Materials and Methods. The identified DNA fragment subclonedin pFAJ860 contained all of the genes of A. brasilense correspondingto known fix(cyt,cco)NOQP genes of other bacteria.

Four ORFs (orf1, orf2, orf3, and orf4) of, respectively, 1,494, 765, 159, and 885 bp were detected (Fig. 2). Each of theseORFs was preceded by a putative Shine-Dalgarno sequence upstreamof the ATG start codon. orf1 was preceded by a potential anaerobox(TTGA-N₅-ATCAA) 189 bp upstream of the ATG codon (9). At 60bp downstream of orf4, a sequence with interrupted dyad symmetry( $Delta$ G [25°C] = $-$ 25 kcal), followed by a T-rich region, suggeststhe presence of a Rho-independent transcription terminator (35).The amino acid sequences deduced from these ORFs showed high similaritywith those of known genes, i.e., fixN (cyt,ccoN), -O, -Q, and-P. The identified ORFs were therefore designated cytN (orf1),cytO (orf2), cytQ (orf3), and cytP (orf4).

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FIG. 2. Physical map of the 6-kb KpnI fragment of pFAJ860. The 4-kb part containing the cytNOQP operon was completely sequenced on both strands. The region downstream of this 4-kb fragment was only partially sequenced. Both arrows indicate insertion of the Km^r cassette. Abbreviations: A, ApaI; B, BamHI; Bs, BssHII; K, KpnI; P, PstI; S, SalI.

The cytN gene encodes a protein of 498 amino acids (predicted molecular mass of 56 kDa for the apoprotein). CytN of A. brasilenseshowed identities ranging from 68 to 70% with CytN-like proteinsof Rhodobacter sphaeroides (accession no. U58092), Sinorhizobiummeliloti (18) (accession no. X15079), P. denitrificans (7),A. caulinodans (23), Bradyrhizobium japonicum (32), and R.capsulatus (45).

cytO encodes an apoprotein of 246 amino acids with a predicted molecular mass of 27.7 kDa. An N-terminal transmembrane helixand a highly conserved heme c-binding site (CYNCH) at position71 could be identified. CytO showed 62 to 68% identity with thealigned CytO-like proteins of R. sphaeroides (accession no. U58092),S. meliloti (18) (accession no. X15079), P. denitrificans(7), A. caulinodans (23), B. japonicum (32), and R. capsulatus(45).

cytQ encodes a small protein of 53 amino acids with a predicted molecular mass of 6 kDa. It exhibited identities of only 34%with the FixQ protein of B. japonicum (32), 40% with FixQ ofS. meliloti (18) (accession no. X15079), 38% with CytQ ofA. caulinodans (23), 34% with CcoQ of R. capsulatus (45),30% with CcoQ of R. sphaeroides (accession no. U58092), and20% with CcoQ of P. denitrificans (7). In B. japonicum FixQis not involved in the assembly of the oxidase complex and seemsnot to be an essential subunit of the complex (55).

cytP codes for an apoprotein of 295 amino acids with a predicted molecular mass of 31.8 kDa. A hydrophobic stretch is locatedat positions 34 to 50. The protein exhibited two heme-bindingmotifs (CAACH at position 121 and CAACH at position 220). CytPshowed an identity of 42 to 53% with the CytP-like proteins ofR. sphaeroides (accession no. U58092), S. meliloti (18) (accessionno. X15079), P. denitrificans (7), A. caulinodans (23),B. japonicum (32), and R. capsulatus (45).

Construction and phenotypic analysis of a cytN mutant. A Km^r insertion mutant was constructed as described in Materials and Methods. The Km^r cassette was inserted in both orientations (Fig. 2).

Membranes isolated from both cytN mutants and wild-type cells grown in microaerobic conditions were tested for the presenceof covalently bound heme by SDS-PAGE followed by heme staining(Fig. 3). Six heme c-containing proteins, of approximately 6,21, 27, 28, 32, and 40 kDa, were present in the wild type. Inthe cytN mutants FAJ851 and FAJ852, the 28- and 32-kDa heme-containingproteins, with molecular masses similar to the predicted molecularmasses of A. brasilense CytP (31.8 kDa) and CytO (27.7 kDa), wereabsent. The other staining bands in both the wild type and cytNmutants represented other, yet-uncharacterized heme-containingproteins, such as NO reductase or bc₁ complex proteins presentin A. brasilense cells grown under the tested conditions (17).

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FIG. 3. Analysis for covalently bound heme in A. brasilense membrane proteins. Membranes were isolated from microaerobically grown wild-type A. brasilense (Sp7) (lane 1) and cytN mutants (FAJ851 [lane 2] and FAJ852 [lane 3]). Equal amounts of proteins (approximately 200 µg) were loaded. The positions of molecular size markers (Bio-Rad) are indicated by horizontal lines (in kilodaltons).

Reduced-minus-oxidized absorbance spectra of membranes isolated from the wild-type Sp7 and from mutants FAJ851 and FAJ852,grown to the beginning of the stationary phase in microaerobicbatch cultures, are shown in Fig. 4. The relative high cytochromec552/cytochrome b560 ratio, characteristic of the presence ofa cytochrome cbb₃ terminal oxidase, was lowered in the mutants,as shown by the decrease in the cytochrome c peak at 552 nm. Furthermore,these spectra of membranes isolated from A. brasilense cytN mutantsin microaerobic conditions showed a high similarity with spectraof membranes isolated from A. brasilense wild-type cells grownin aerobic conditions (Fig. 1C).

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FIG. 4. Dithionite-reduced-minus-air-oxidized spectra, between 500 and 700 nm, of membrane proteins isolated from microaerobically grown cells of A. brasilense Sp7 (wild type) and FAJ851 and FAJ852 (cytN mutants). Equal amounts of protein (approximately 2.6 mg/ml) were analyzed.

Growth of the cytN mutant and the wild type was compared under different conditions (Fig. 5). Specific growth rates duringexponential phase (µ_e) were calculated as described in Materialsand Methods. The A. brasilense cytN mutant and the wild type showedsimilar growth patterns, illustrated by the increase in OD₅₇₈(Fig. 5A₁) and protein concentrations (Fig. 5A₂), in aerobic conditions,although a higher protein concentration was obtained in wild-typecells. After an EFT of approximately 8 h, when the carbon sourcemalate becomes limiting, cells entered the stationary phase (Fig.5A₁). The specific growth rates of A. brasilense Sp7 and the cytNmutant during exponential phase were similar (µ_e of approximately0.2 h¹ [Fig. 5A₂]).

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FIG. 5. Comparison of fermentation parameters of the wild-type A. brasilense Sp7 and the A. brasilense cytN mutant FAJ851 under aerobic (A), microaerobic and NH₄⁺-supplemented (B), and nitrogen-fixing (C) conditions. (A₁, B₁, and C₁) OD₅₇₈ values and malate concentrations. Panels B₁ and C₁ also show the percentage of O₂ present in the incoming airflow during fermentation in microaerobic conditions. Note that in panel C₁ the lines for percent O₂ during fermentation of the wild-type Sp7 and the cytN mutant FAJ851 coincide. (A₂, B₂, and C₂) Protein concentrations and specific growth rates (µ). Values for protein concentration and L-malate are the averages of at least four different measurements. (A₁, B₁, and C₁)

, OD₅₇₈ for Sp7;

, OD₅₇₈ for FAJ851; $bullet$ , L-malate for Sp7; $open circle$ , L-malate for FAJ851; ---, percent O₂ for Sp7; $---$ , percent O₂ for FAJ851. (A₂, B₂, and C₂) $black-triangle$ , protein for Sp7; $triangle$ , protein for FAJ851; $black-lozenge$ , µ for Sp7; $diamond$ , µ for FAJ851.

In microaerobic conditions in a medium supplemented with NH₄⁺, the low DO concentration had no influence on the growth behaviorof the A. brasilense wild type compared to that in aerobic conditions(Fig. 5A and B). Within a few hours, the OD₅₇₈ increased drastically(Fig. 5B₁) (µ_e of approximately 0.2 h¹ [Fig. 5B₂]), and the stationary phase was reached after an EFTsimilar to that for aerobically grown cells. In contrast, thespecific growth rate of the A. brasilense cytN mutant during exponentialphase was considerably affected (µ_e of approximately 0.02 h¹ [Fig. 5B₂]). Only after an EFT of 40 h did the cells reach anOD₅₇₈ similar to the OD₅₇₈ obtained for the wild type at the beginningof the stationary phase (Fig. 5B₁). The carbon source malate wasstill not entirely consumed. Respiratory behavior can be judgedby the changes in the percentage of O₂ present in the incominggas flow during fermentation. An increase in the percentage ofO₂ is due to an increase in the airflow rate. The higher O₂ concentrationin the incoming gas flow together with the simultaneously increasedtotal gas flow through the fermentor causes a higher O₂ transferrate, reflecting the higher O₂ consumption by the growing cells.Figure 5B₁ shows that when the wild-type cells were grown in microaerobicNH₄⁺-supplemented conditions, the percentage of O₂ in the gas flow,automatically adjusted to maintain a constant DO concentrationof 2.5 µM, was increased at regular time intervals in order tocope with the high O₂ demand of the fast-growing cells. For theA. brasilense cytN mutant grown in similar conditions, a low constantpercentage of O₂ in the gas flow was sufficient to maintain theDO concentration at 2.5 µM.

The specific growth rate of the wild type during exponential phase under nitrogen-fixing conditions (µ_e of approximately 0.03h¹ [Fig. 5C₂]) was decreased compared to specific growth rates obtainedunder the same conditions but in the presence of an NH₄⁺ source (µ_e of approximately 0.2 h¹ [Fig. 5B₂]). The cells needed approximately 30 h to reach stationaryphase, and the final cell protein concentration was significantlylower than during NH₄⁺-supplemented growth (Fig. 5C₁ and C₂). The percentage of O₂ inthe gas flow during fermentation remained relatively constant,indicating a low O₂ demand (Fig. 5C₁). In these nitrogen-fixingconditions, the growth and respiratory behaviors of the A. brasilensecytN mutant did not differ drastically from those of the wildtype (Fig. 5C₁ and C₂). A lower rate of consumption of the carbonsource malate, a slightly lower specific growth rate during exponentialphase (µ_e of approximately 0.02 h¹), and a reduction of the specific nitrogenase activity of theA. brasilense cytN mutant (13.5 ± 0.99 nmol of ethylene/mg ofprotein/h) to approximately 80% of the wild-type activity (16.52± 1.25 nmol of ethylene/mg of protein/h) were observed for theA. brasilense cytN mutant compared to the wild-type strain. Thehigh specific growth rate observed for both the A. brasilensecytN mutant and the wild type at the start of nitrogen-fixinggrowth is probably due to the presence of internal NH₄⁺ in the inoculated cells (Fig. 5C₂).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The similarity between spectra shown in this work and those reported for the purified cbb₃-type cytochrome c oxidase complexesfrom B. japonicum (33), R. capsulatus (15), and M. magnetoacticum(43) suggests that an analogous cytochrome cbb₃ oxidase is presentin microaerobically grown Azospirillum cells. Accordingly, andconsistent with previous results, a relative increase in the levelof cytochrome c versus cytochrome b was observed during a shiftfrom aerobic to microaerobic conditions (6, 21).

Genetic evidence of a cytNOQP operon in A. brasilense supports this biochemical analysis. The A. brasilense cytNOQP operonis preceded by a putative anaerobox. So far, no direct evidencefor the existence of an FNR-like protein in Azospirillum is available(47).

cytN of A. brasilense encodes subunit I of the cbb₃-type terminal oxidase. The highly conserved histidine residues shown tobe involved in the binding of the high-spin b/Cu_B reaction center(5, 26) are conserved at positions 362, 274, 275, and 224in the A. brasilense CytN. The histidine residues assumed to bethe axial ligands for the low-spin heme b (22, 56) are locatedat positions 74 and 364. The histidine residue implicated in Mg²⁺ and Mn²⁺ binding in B. japonicum FixN (54) is present at position 354.The histidine residue suggested to bind and release protons inB. japonicum FixN (54) is at position 260. Based on a structuralcomparison between subunit I of conventional cytochrome c oxidases,containing 12 transmembrane helices, and the cytochrome cbb₃ oxidases,usually characterized by 14 potential transmembrane helices, Zuffereyet al. (56) hypothesized that the first 2 of these 14 transmembranehelices of CytN-like proteins should be cytoplasmic. This hypothesiswas supported by studies with fusion proteins (56). Interestinglythe A. brasilense CytN protein seems to be truncated and lacksthese two first transmembrane helices encountered in other sequencedCytN-like proteins.

To investigate the role of the cytochrome cbb₃ oxidase, a Km^r insertion mutant of A. brasilense cytN was constructed. Resultsfrom heme-stained SDS-PAGE gels and spectral analysis of membranesfrom both A. brasilense wild-type and A. brasilense cytN mutantcells led us to conclude that the A. brasilense cytN mutant lacksa functional cytochrome cbb₃ terminal oxidase.

Subsequently, growth analysis was performed. In microaerobic conditions a high respiration rate potentially supporting efficientenergy production allows the A. brasilense wild-type cells togrow at rates similar to those obtained in highly aerated cultures,despite the low DO concentration. As the A. brasilense cytN mutantwas not able to sustain such growth, the cytochrome cbb₃ oxidaseseems to be responsible for the high respiration rates observedat low DO concentrations. During nitrogen fixation, the specificgrowth rate of the wild type was considerably lower than in NH₄⁺-supplemented conditions. As nitrogen fixation is a very energy-consumingprocess, a shortage of ATP seems a plausible cause for growthlimitation. This seems to be the case in symbiotic microorganismssuch as Rhizobium or Bradyrhizobium species, where nitrogen fixationtakes place in nodules. These nodules create the optimal low O₂concentration to prevent O₂ damage to the nitrogenase and functionsimultaneously as an O₂ delivery system (40) to a high-affinitycytochrome cbb₃ terminal oxidase. This oxidase allows high respirationrates and generation of a proton motive force at nanomolar concentrationsof O₂ (33). Cytochrome cbb₃ mutants are completely (32) orat least partially (19, 23) unable to fix N₂, indicating theimportance of energy as a limiting factor. Assuming that energylimitation explains the lower specific growth rates of the wild-typeA. brasilense during nitrogen fixation, the A. brasilense cytNmutant affected in its cytochrome cbb₃ terminal oxidase wouldbe expected to show an even more pronounced energy-limited growth.However, only minor differences were observed between the specificgrowth rates of the A. brasilense cytN mutant and the wild typein these conditions, and the nitrogenase of the A. brasilensecytN mutant still retained approximately 80% of its activity.Therefore, a more likely explanation of growth limitation in nitrogen-fixingconditions seems to be the shortage of NH₄⁺. Possibly the nitrogenase cannot produce sufficient NH₄⁺ to cope with the high NH₄⁺ consumption by fast-growing cells. Alternatively, the strictregulation of the nitrogen-fixing process cannot be excluded asa growth-limiting factor. If cells fix nitrogen at high rates,the internal NH₄⁺ accumulating in the cells could switch off the system (52).Nitrogen fixation and thus the NH₄⁺ concentration consequently decrease, which in turn allows thesystem to resume nitrogen fixation. Conceivably, there can neverbe an accumulation of sufficient NH₄⁺ to allow fast growth and subsequent energy limitation.

Similar to the observations made for A. caulinodans (19, 23), an unknown alternative oxidase can partially overcome theabsence of the cytochrome cbb₃ terminal oxidase in microaerobicconditions, either in presence or absence of NH₄⁺, since A. brasilense cytN mutants could still grow. Similar toprevious results for A. brasilense Sp7 (6), but in contrastto those for A. brasilense Cd (34), no terminal oxidase containingcytochrome d seems to be present. No indications could be foundfor the presence of heme a, not even in membranes of aerobicallygrown cells. Although the concentrations of heme a discoveredbefore in A. brasilense Sp7 were barely detectable (21), itcannot be ruled out that under certain conditions this cytochromec oxidase is expressed. Comparison of the reduced-minus-oxidizedspectra of membranes from the A. brasilense cytN mutant and thewild type points in the direction of an additional heme b-containingterminal oxidase such as, e.g., a bo-quinol oxidase during microaerobicgrowth. This oxidase also seems to be present in fully aeratedmembranes of the wild type. A conclusive interpretation of theCO-reduced-minus-reduced spectra (data not shown) was hamperedby interference of the absorption maxima of this potential bo-quinolcomplex by the absorption maxima of other proteins putativelypresent in the membranes, such as the bc₁ complex, denitrifyingcomplexes, or even other alternative oxidases (11). However,the presence of a bo-quinol oxidase seems to be consistent withearlier reports on A. brasilense Sp7, which indicate the presenceof particulate cytochrome b (6, 21) and a CO-binding cytochromeo (6, 21) in aerobic conditions. Likewise, spectral analysissuggested the presence of a cytochrome o-containing terminal oxidasein A. brasilense Cd, expressed in aerobic but also in microaerobicconditions (34). This terminal oxidase, however, seemed to functionafter the antimycin A inhibition site (after the cytochrome creductase complex). In addition it was shown that an alternativeoxidase, other than cytochrome caa₃-type cytochrome c oxidaseand less sensitive to KCN, could accept electrons from TMPD (N,N,N'-tetramethyl-p-phenylenediamine)plus ascorbate, indicating the presence of another cytochromec-type terminal oxidase (34). We suggest that, given the spectralsimilarities between cytochrome o-containing and cbb₃-type terminaloxidases, the cytochrome o-like cytochrome c oxidase identifiedpreviously is identical to the cytochrome cbb₃ cytochrome c terminaloxidase of A. brasilense Sp7 characterized in this study. Thepresence of such a cbb₃-type cytochrome c oxidase might have accountedfor the residual reduction of ascorbate in the presence of a lowconcentration KCN, which is known to inhibit the cytochrome caa₃-typecytochrome c oxidase.

	ACKNOWLEDGMENTS

K.M. is a recipient of the Fonds voor Wetenschappelijk Onderzoek-Vlaanderen. This work was supported by grants (to J.V.) fromthe Flemish Government (GOA) and the Fonds voor WetenschappelijkOnderzoek-Vlaanderen.

We thank the Laboratory of Industrial Microbiology, KULeuven, Heverlee, Belgium, for kindly providing the fermentation equipment.

	FOOTNOTES

^* Corresponding author. Mailing address: F.A. Janssens Laboratory of Genetics, KULeuven, Kardinaal Mercierlaan 92, 3001 Heverlee,The Netherlands. Phone: 32 16 329679. Fax: 32 16 321966. E-mail:jozef.vanderleyden{at}agr.kuleuven.ac.be.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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	ALL ASM JOURNALS

1.	Altschul, S. F., W. Gish, W. Milles, E. W. Myersand, and D. J. Lipman. 1990. Basic local alignment tool. J. Mol. Biol. 215:403-410[Medline].
2.	Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.). 1991. Current protocols in molecular biology, p. 4.8.1-4.8.5. Wiley Interscience, New York, N.Y.
3.	Barak, R., I. Nur, Y. Okon, and Y. Henis. 1982. Aerotactic response of Azospirillum brasilense. J. Bacteriol. 152:643-649[Abstract/Free Full Text].
4.	Bergersen, F. J., and G. L. Turner. 1980. Properties of terminal oxidase systems of bacteroids from root nodules of soybean and cowpea and of N₂-fixing bacteria grown in continuous culture. J. Gen. Microbiol. 118:235-252.
5.	Calhoun, M. W., J. W. Thomas, J. J. Hill, J. P. Hosler, J. P. Shapleigh, M. M. J. Tecklenburg, S. Ferguson-Miller, G. T. Babcock, J. O. Alben, and R. B. Gennis. 1993. Identity of the axial ligand of the high-spin heme in cytochrome oxidase: spectroscopic characterization of mutants in the bo-type oxidase of Escherichia coli and the aa₃-type oxidase of Rhodobacter sphaeroides. Biochemistry 32:10905-10911[Medline].
6.	Chakrabarti, S. K., A. K. Mishra, and P. K. Chakrabartty. 1984. Cytochromes in Azospirillum brasilense. Curr. Microbiol. 11:343-348.
7.	de Gier, J.-W. L., M. Schepper, W. N. M. Reijnders, S. J. van Dyck, D. J. Slotboom, A. Warne, M. Saraste, K. Krab, M. Finel, A. H. Stouthamer, R. J. M. van Spanning, and J. van der Oost. 1996. Structural and functional analysis of aa₃-type and cbb₃-type cytochrome c oxidases of Paracoccus denitrificans reveals significant differences in proton-pump design. Mol. Microbiol. 20:1247-1260[Medline].
8.	Dente, L., G. Cesareni, and R. Cortese. 1983. pEMBL: a new family of single stranded plasmids. Nucleic Acids Res. 11:1645-1655[Abstract/Free Full Text].
9.	Eiglmeier, K., N. Honoré, S. Iuchi, E. C. C. Lin, and S. T. Cole. 1989. Molecular genetic analysis of FNR-dependent promoters. Mol. Microbiol. 3:869-878[Medline].
10.	Fellay, R., J. Frey, and H. Krisch. 1987. Interposon mutagenesis of soil and water bacteria: a family of DNA fragments designed for in vitro insertional mutagenesis of gram-negative bacteria. Gene 52:147-154[Medline].
11.	Ferguson, S. J. 1994. Denitrification and its control. Antonie Leeuwenhoek 66:89-110[Medline].
12.	Francis, R. T., and R. R. Becker. 1984. Specific indication of hemoproteins in polyacrylamide gels using a double-staining process. Anal. Biochem. 136:509-514[Medline].
13.	Friedman, A. M., S. R. Long, S. E. Brown, S. E. Buikema, and F. M. Ausubel. 1982. Construction of a broad host range cloning vector and its use in the genetic analysis of Rhizobium mutants. Gene 18:289-296[Medline].
14.	Garcia-Horsman, J. A., B. Barquera, J. Rumbley, J. Ma, and R. B. Gennis. 1994. The superfamily of heme-copper respiratory oxidases. J. Bacteriol. 176:5587-5600[Free Full Text].
15.	Gray, K. A., M. Grooms, H. Myllykallio, C. Moomaw, C. Slaughter, and F. Daldal. 1994. Rhodobacter capsulatus contains a novel cb-type cytochrome c oxidase without a Cu_A center. Biochemistry 33:3120-3127[Medline].
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