Transcriptional and Mutational Analysis of the Uptake Hydrogenase of the Filamentous Cyanobacterium Anabaena variabilis ATCC 29413

doi:10.1128/JB.182.6.1624-1631.2000

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Journal of Bacteriology, March 2000, p. 1624-1631, Vol. 182, No. 6
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Transcriptional and Mutational Analysis of the Uptake Hydrogenase of the Filamentous Cyanobacterium Anabaena variabilis ATCC 29413

Thomas Happe,^* Kathrin Schütz, and Herbert Böhme

Botanisches Institut der Universität Bonn, D-53115 Bonn, Germany

Received 1 September 1999/Accepted 21 December 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

A 10-kb DNA region of the cyanobacterium Anabaena variabilis ATCC 29413 containing the structural genes of the uptake hydrogenase(hupSL) was cloned and sequenced. In contrast to the hupL geneof Anabaena sp. strain PCC 7120, which is interrupted by a 10.5-kbDNA fragment in vegetative cells, there is no programmed rearrangementwithin the hupL gene during the heterocyst differentiation ofA. variabilis. The hupSL genes were transcribed as a 2.7-kb operonand were induced only under nitrogen-fixing conditions, as shownby Northern blot experiments and reverse transcriptase PCR. Primerextension experiments with a fluorescence-labeled oligonucleotideprimer confirmed these results and identified the 5' start ofthe mRNA transcript 103 bp upstream of the ATG initiation codon.A consensus sequence in the promoter that is recognized by thefumarate nitrate reductase regulator (Fnr) could be detected.The hupSL operon in A. variabilis was interrupted by an interposondeletion (mutant strain AVM13). Under N₂-fixing conditions, themutant strain exhibited significantly increased rates in H₂ accumulationand produced three times more hydrogen than the wild type. Theseresults indicate that the uptake hydrogenase is catalyticallyactive in the wild type and that the enzyme reoxidizes the H₂developed by the nitrogenase. The Nif phenotype of the mutantstrain showed a slight decrease of acetylene reduction comparedto that of the wildtype.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The only microorganisms with an O₂-producing photosynthesis that have a hydrogen metabolism are cyanobacteria and green algae(23, 25). In cyanobacteria, up to three enzymes can be involvedin hydrogen metabolism: the nitrogenase which produces H₂ duringnitrogen fixation (24), the membrane-bound hydrogenase whichreoxidizes the H₂ (10), and the bidirectional hydrogenase catalyzingboth oxidation of molecular hydrogen and reduction of protons(38). In cyanobacteria, the genetics of bidirectional hydrogenasesare especially well characterized (3, 7). But, the H₂ productionin filamentous cyanobacteria during the reduction of nitrogento NH₃ is mainly catalyzed by the nitrogenase in the heterocysts.The Anabaena cells can oxidize the hydrogen with the uptake hydrogenasevia the oxyhydrogen (Knallgas) reaction. It was suggested thatthe organism gets additional ATP while the Knallgas reaction canprotect the O₂-sensitive nitrogenase by removing the oxygen inthe heterocysts (30).

Hydrogenases have been described for a large number of microorganisms and studied intensively in diverse phylogenetic groupsof bacteria (22, 34, 54). The uptake hydrogenases are membrane-boundenzymes which consist of two subunits with [Fe-S] clusters asprosthetic groups. The large subunit, HupL, carries additionallya Ni atom in the active center. In most of the bacterial families,the hupSL genes are clustered in an operon in which hupS is locatedupstream of the hupL gene (20, 51, 53). Recently, some hydrogenasesequences from filamentous cyanobacteria were published (10,31, 38). The uptake hydrogenase in the heterocyst-formingorganism Anabaena sp. strain PCC 7120 is interrupted by a 10.5-kbelement. Under nitrogen-fixing conditions, this fragment is excisedby a site-specific recombinase that is encoded inside the rightborder of the hupL element (10). This rearrangement is not foundin the hupSL genes of Nostoc sp. strain PCC 73102 (31).

In the present study, we isolated and characterized the hup gene region in Anabaena variabilis ATCC 29413. In contrast tothe best characterized filamentous cyanobacterium Anabaena sp.strain PCC 7120, the closely related strain A. variabilis hassome interesting features. Heterocyst differentiation in Anabaenasp. strain PCC 7120 is accompanied by developmentally regulatedgenome rearrangements that affect fdxN, nifD, and hupL gene expression(9, 10). A. variabilis does not contain the fdxN element(6), and in this study we show that the hupL gene is also notrearranged in A. variabilis.

In order to analyze the function of the uptake hydrogenase in nitrogen and hydrogen metabolism, we constructed a hupSL deletionmutant by the insertion of an interposon in the hupSL operon.Physiological studies to compare the mutant phenotype with thatof the wild type were carried out. The transcriptional regulationof the hupSL genes was investigated by Northern analysis and reversetranscriptase PCR. Further transcriptional investigations weremade by determining the 5' end of the mRNA by the primer extensiontechnique and analyzing the promoterregion.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains and growth conditions. Bacterial strains and plasmids are listed in Table 1. Cells of the N₂-fixing cyanobacterium A. variabilis ATCC 29413 weregrown either in BG11, BG11₀ (12), or BG11₀ medium supplementedwith 5 mM NH₄Cl and 10 mM TES [N-tris (hydroxymethyl)methyl-2-aminoethanesulfonic acid] under continuous irradiance of 100 µmol m² s¹ and bubbled with air enriched with CO₂ to 1% (vol/vol) at 30°C.To induce heterocyst formation, the cultures were pelleted, washedtwice with BG11₀, and grown in BG11₀ for 24 h.

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TABLE 1. Bacterial strains and plasmids used in this study^a

For deletion mutagenesis, a wild-type strain of A. variabilis with a spontaneous mutation (FD strain) which also grows at40°C was used. The mutant AVM13 was grown in BG11 medium supplementedwith 50 µg of neomycin per ml. The growth conditions, media, andantibiotic concentrations for Escherichia coli strains were describedelsewhere (47).

Nucleic acid isolation. Genomic DNA of the A. variabilis wild type and the mutant was isolated according to the method of Smoker and Barnum (42).Plasmid DNA was obtained by standard techniques (36). Totalcellular RNA was isolated from 200-ml cultures grown in differentmedia (BG11, BG11₀, and NH₄⁺). The cells were disrupted with glass beads (450 microns), followedby organic extraction and ethanol precipitation. To remove contaminatingDNA and proteins, a cesium-chloride gradient ultracentrifugationpurification step (4) was done. The concentration of RNA wasdetermined by measuring the absorbance at 260nm.

Hybridization. For Southern blot hybridization analysis, chromosomal DNA of A. variabilis and the exconjugants, as well as the plasmid DNAfrom the clones of the partial libraries, was isolated and cutwith appropriate restriction enzymes. Following separation byelectrophoresis in 1% agarose gels, the DNA was transferred toHybond N nylon membranes (Amersham Pharmacia Biotech) by the capillarymethod described by Sambrook et al. (36). Prehybridization,overnight hybridization, and washing steps were carried out at58 to 62°C. Labeling of probes and detection of hybridizationsignals were performed with the DIG Labeling and Detection kit(Roche Diagnostics, BoehringerMannheim).

Northern blot experiments were carried out by separating total RNA of the different cultures in 1% denaturing formaldehydeagarose gels and transferring to Hybond N nylon. pKS14 was labeledwith digoxigenin-UTP by in vitro transcription with the T7-RNA-polymerase(Roche Diagnostics, Boehringer Mannheim). RNA-RNA hybridizationwas performed overnight at 65°C in DIG Easy Hybsolution.

Screening of partial gene banks and sequencing. Genomic DNA of A. variabilis was digested by different restriction endonucleases. After separation on a 1% agarose gel, HindIIIand XbaI fragments between 4.5 and 5.0 kb were eluted out of thegel pieces. The extracted gel fragments were ligated to HindIII-and XbaI-linearized and -dephosphorylated pBluescript SK( $-$ ) vectorsand transformed into competent E. coli MC1061 cells by the CaCl₂method (13; modified by reference 36). A 0.8-kb HindIII-Asp700fragment (pIF1) and a 0.6-kb Asp700-HindIII fragment (pTS1), obtainedfrom the plasmid pAM1311 (10), were digoxigenin-labeled andused for Southern blot experiments with the clones of the partiallibraries.

The plasmids pKS1 and pKS18 were treated with exonuclease III and S1 nuclease of an Erase-a-Base kit (Promega). Followingligation and transformation, the deletion clones were analyzedby restriction. Sequencing was then performed by the dideoxy chaintermination method (37).

PCR and primer extension analysis. The 5' end of the uptake hydrogenase mRNA was determined by a primer extension protocol (29) with fluorescence-labeled oligonucleotidesand an automated DNA sequencer (2). The synthetic cy5-labeledoligonucleotide HupS7 (5'-Cy5-CGCATACTGTCGGTTCTTCGGC-3') was a22-mer complementary to the bases 85 to 64 downstream of the translationstart codon ATG of the hupSgene.

Primer extension mixtures included 10 to 20 µg of RNA of the different preparations, 10 pmol of the HupS7 oligonucleotide,50 U of RNasin Ribonuclease Inhibitor, 1 mM concentrations ofdeoxynucleoside triphosphates, and 5 U of avian myeloblastosisvirus reverse transcriptase. The mixtures were incubated at 42°Cfor 1 h. The dideoxy sequencing reaction using a clone containingthe 5' region of the hupS gene (pKS15) and the same HupS7 primerwas performed according to the instructions of the cy5-Auto ReadSequencing kit (Amersham Pharmacia Biotech). The primer extensionproduct and the sequence ladder were loaded together onto a gelof the A.L.F. Express DNA Sequencer, and the transcription startpoint was determined by comparing their retentiontimes.

Inverse PCR as described by Pang and Knecht (32) was used to determine the flanking sequences of the 3' end of the hupLgene. Two primers which were complementary to bases 1230 to 1310(HupL2 [5'-CGCTTGGCGATATAACTTGA-3']) and identical to bases 1337to 1362 (HupL3 [5'-GTCACTGGATAGATATCGAAGGTGGC-3']) of the hupLgene were selected. These primers, facing outwards from the knownDNA sequence, were used to carry out PCR with genomic DNA fromA. variabilis.

Constructions of plasmids and conjugative plasmid transfer. Different cargoplasmids were constructed and then transferred from E. coli HB101 to A. variabilis. A 2.15-kb XbaI fragmentcontaining the hupS gene and part of the hupL gene was removedfrom the plasmid pKS1 by replacing it with a 1.1-kb neomycin resistancecassette from C.K3, yielding pKS4. C.K3 contains the npt genefrom Tn5 with a promoter from the psbA gene of Amaranthus hybridus(18). pAVM13 was constructed by inserting the resulting 3.77-kbHindIII fragment from pKS4 in pSUP202 (41).

The resulting cargoplasmid pAVM13 was introduced from E. coli cells into the A. variabilis FD strain via triparental mating(using the conjugal plasmid pRL443 and the helper plasmid pRL623for mobilization). The conjugative plasmid transfer was performedaccording to the method of Elhai et al. (19). Instead of thenormal wild-type strain, a spontaneous mutant (FD strain) whichgrows at 40°C was used for triparental mating. Exconjugants wereselected by plating on BG11 plates containing 50 µg of neomycinper ml. Nm^r exconjugants were picked and grown in liquid medium, one addedwith neomycin and one added with ampicillin, to select the Amp^s exconjugants which have made the marker rescue via double crossover.One ampicillin-sensitive mutant chosen for further studies wasdesignated AVM13. Insertion of the neomycin resistance cassetteand complete segregation in AVM13 was shown by Southernhybridization.

Determination of nitrogenase and hydrogenase activity. In vivo nitrogenase activity was measured by acetylene reduction assay (17) using a Hewlett-Packard gas chromatograph Model5890 Series II with a 6-ft Porapak N80/100 column for acetylene-ethyleneseparation and a flame ionization detector. The specific nitrogenaseactivity was expressed as follows: nanomoles of ethylene (C₂H₄)/microgramsof chlorophyll $alpha$ × h. The developed H₂ was quantified in a gaschromatograph (Hewlett-Packard Model 5890 Series II) equippedwith a thermal conductivity detector and a molecular sieve columnand expressed as follows: nanomoles of H₂/nanograms of chlorophyll $alpha$ × h. The hydrogen uptake was measured during incubation at 25°Cby the decrease of a known amount of H₂ (2 ml of 0.3% H₂-99.7%argon) added to theprobe.

Nucleotide sequence accession number. The nucleotide sequence data reported in this study is available from the EMBL, GenBank, and DDBJ nucleotide sequence databasesunder accession no. Y13216.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Isolation, characterization, and sequence comparison of the hupSL region in A. variabilis ATCC 29413. To identify the hup gene region in A. variabilis ATCC 29413, the hupSL genes were cloned by partial genomic library screeningusing different fragments within the hupL gene of Anabaena sp.strain PCC 7120 as probes in Southern hybridization experiments(see Materials and Methods). First, a HindIII (pKS1) clone witha 4,824-bp insert was isolated. This nucleotide sequence has twoopen reading frames (ORFs) that show over 90% homology to thehupSL genes of Anabaena sp. strain PCC 7120. As a result, no stopcodon was found at the 3' end of the hupL gene, indicating thathupL was only partially encompassed by the insert ofpKS1.

A second partial gene bank was constructed to obtain the remaining part of hupL. After screening with a DNA probe (pTS1) containingthe downstream region of the Anabaena sp. strain PCC 7120 hupLgene, one positive clone (pKS18) which contained the 120 bp ofthe 3' end of the A. variabilis hupL gene was obtained. The missing30 bp of the hupL gene were then identified by inverse PCR (32)using two inverted oligonucleotide primers which were designedfrom within the hupL sequence of the HindIII fragment. Both strandsof the inserts, which contain the complete sequence of the hupSLgene region, were determined (data not shown). Together, the nucleotidesequence revealed 10 complete ORFs and one partial ORF (Fig. 1).Comparisons of their deduced amino acid and DNA sequences withknown sequences in databases were performed (1, 21).

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FIG. 1. Physical and genetical maps of the 10-kb hupSL gene region of A. variabilis. The physical maps are for the enzymes HindIII and XbaI. The region is divided into three subclones, marked with horizontal lines. The organization of the genes is indicated by arrows under the restriction map; ORF8 has been only partially sequenced. hupSL code for the two subunits of the uptake hydrogenase; rkpK probably encodes the UDP-glucose dehydrogenase. The gene arrangement of the cargoplasmid pAVM13 with the integrated neomycin resistance cassette (Nm^r) is shown. Note that pAVM13 is drawn on a different scale.

Two ORFs encode the small and large subunits of the uptake hydrogenase (hupSL). The proteins consist of 321 and 531 aminoacid residues with calculated molecular masses of 35.1 and 61.9kDa, respectively. Comparisons of the deduced amino acid sequencesof hupS and hupL gene products with the HupS and HupL proteinsof the filamentous cyanobacteria Anabaena sp. strain PCC 7120and Nostoc sp. strain 73102 revealed very high similarities. Bothsubunits in A. variabilis showed more than 95% identity with thehomologous region from Anabaena sp. strain PCC 7120. This is notsurprising for these closely related organisms since 90% and highersimilarities are also known for the nifHDK cluster (95% nucleotideidentity) (6) and the ndh genes (93% nucleotide identity; T.Happe, personal communication). The intergenic region betweenhupS and hupL in A. variabilis consists of 76 bp and is only 60%homologous to the intergenic DNA sequence (54 bp) of Anabaenasp. strain PCC 7120. Unlike the hupL gene of Anabaena sp. strainPCC 7120, the hupSL operon in vegetative cells of A. variabilisis not interrupted by a 10.5-kb element. In Anabaena sp. strainPCC 7120, this DNA fragment is excised during heterocyst differentiation.Southern hybridizations with different DNA probes support thesequence data of a contiguous hupSL operon in A. variabilis.

The three ORFs upstream of the hupSL genes (Fig. 1) encode products that showed no similarity to any known protein. They probablydo not belong to the hupSL operon because they are transcribedin the opposite direction. Also, no homologies were found forORF4, ORF5, and ORF6. Interestingly, one (ORF7, 159 amino acidsencoded) showed about 44% amino acid identity to a regulator proteinof Enterococcus faecalis. One ORF (453 amino acids) 2 kb downstreamof the hupL gene, showed homology to a UDP-glucose dehydrogenaseof Synechocystis sp. strain PCC 6803 (46% identity) and Sinorhizobiummeliloti (43% identity). In S. meliloti, the dehydrogenase catalyzesthe reaction from UDP-glucose to UDP-glucuronic acid and is involvedin the synthesis of capsular polysaccharides. The partial ORFat the 3' end of the XbaI clone demonstrated homology to the C-terminalend of a UDP-glucose dehydratase from Synechocystis sp. strain6803 (48%identity).

Transcriptional analysis. Northern blot analysis was performed to examine the expression of the hupSL operon in N₂-fixing and non-N₂-fixing cultures.The Northern blot was hybridized with a digoxigenin-labeled probe(pKS14) from within the hupS gene. The transcript was only detectedin RNA isolated from N₂-fixing cultures (Fig. 2). Using an RNAmarker, the size of the hupSL operon was determined to be 2.7kb. Transcripts were completely missing in cells grown in mediumsupplemented with either ammonia or nitrate. The results of theNorthern analysis were in good agreement with the results madeby RT-PCR using total RNA from BG11 and BG11₀ cultures (data notshown). These results indicate that the A. variabilis hupSL operonis either nitrogen regulated or induced by hydrogen. In the cyanobacteriumNostoc sp. strain PCC 73102, the hupL transcript is also inducedduring heterocyst differentiation (5).

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FIG. 2. RNA gel blot analysis of the hupSL transcript. Hybridization of the hupS gene containing a 950-bp HincII fragment to total RNA (10 µg each) isolated from cells grown with NO₃ (1), NH₄⁺ (3) in the medium and under nitrogen-fixing conditions (2). The locations of the RNA size markers are shown.

The 5' end of the hupSL mRNA was determined by means of the primer extension technique with a fluorescence-labeled oligonucleotideprimer and an automated DNA sequencer. Performing the extensionreaction with RNA isolated under N₂-limiting conditions, a majorextension product was detected. By comparing the retention timeof this product with the signal in the sequence chromatogram (Fig.3), the first transcribed nucleotide, a thymidine, was located103 nucleotides upstream of the translational start codon ATGof the hupS gene (Fig. 4). No primer extension product was foundwith RNA isolated from BG11 cultures (Fig. 3). This provides furtherevidence that the hupSL operon is expressed only under N₂-fixingconditions. Fifteen base pairs upstream of the transcription initiation,a sequence that resembles a $-$ 10 consensus region (TAAACT) of thehup operon in E. coli (26) was found. Half of a sequence motifidentical to the consensus Fnr-binding sequence 144 bp upstreamof the transcription start site (Fig. 4) was also found. In addition,a fivefold direct repeat of the sequence TA/GACAAC upstream ofthe ATG start codon was obvious to identify.

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FIG. 3. Localization of the transcription start point of the hupSL genes. (A) Nucleotide sequence of the pKS1 clone containing the promoter region of the hupSL operon. Arrow indicates the start codon in the genome sequence. (B) Primer extension products obtained with RNA isolated from BG11 and BG11₀ cultures as the template and the oligonucleotide HupS7 as the primer. The retention times of the start codon and of the major extension product are shown. All signals result from the BG11₀ RNA except for the smaller peak at retention time 198.

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FIG. 4. Nucleotide sequence of the hupSL promoter region. The start codon of hupS is in bold; the N-terminal end of the amino acid sequence is written under the nucleotide sequence. Shine-Dalgarno homologies are underlined. The transcription start point is given by +1. The repetitive elements in the promoter sequence are boxed. The primer HupS7, used for primer extension, is also shown. The putative $-$ 10 consensus sequence and the Fnr-binding site are underlined and in bold.

Construction of a hupSL mutant and physiological characterization. To investigate the biological properties of the hupSL genes, a mutant strain (AVM13) in which the complete hupS gene and the5' end of the hupL gene were deleted was constructed. A 2.15-kbXbaI fragment from within the plasmid pKS1 (4.8-kb HindIII fragment)was replaced by the selectable marker gene npt (Fig. 1).

Total DNA from two homocygote recombinant clones (13₁ and 13₂) was prepared, and marker rescue and complete segregation wasconfirmed by Southern hybridization using a 715-bp fragment fromwithin the hupL gene as a probe (pKS13) (Fig. 1 and 5). The probehybridized with wild-type DNA at approximately 4.8 kb, correspondingto the original HindIII fragment. On the other hand, there isonly one signal at 3.8 kb in the lane containing genomic DNA ofthe mutant 13₁. This result indicates that the genome of thisclone is completely segregated while the genome of 13₂ is notbecause two signals at 4.8 and 3.8 kb occurred on the blot. Themutant 13₁ was designated AVM13 and was chosen for further investigations.

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FIG. 5. Southern analysis of the hupSL operon. (A) Total DNA (5 µg) from A. variabilis and the two mutant strains 13₁ and 13₂ was restricted with HindIII. (B) pKS13 containing part of the hupL gene was used as a probe. The arrows indicate the hybridization signals of the wild type (4.8 kb) and the mutants (3.8 kb).

The physiological effects of the mutation in strain AVM13 were investigated by comparing the diazotrophic growth under aerobicconditions and the hydrogen metabolism (the in vivo nitrogenaseand hydrogenase activity) of the mutant and the wild-type strains.Because the uptake hydrogenase is only active in heterocysts duringnitrogen fixation, the deletion of the hup genes should have effectson a culture grown in medium without combined nitrogen. The A.variabilis wild type and mutant strain AVM13 were grown in mediawith combined nitrogen (BG11) or without combined N₂ (BG11₀).Following the growth, the chlorophyll $alpha$ content of the cultureswas measured. In BG11, AVM13 cells have growth rates similar tothat of the wild type (data not shown). During the first 80 h,the diazotrophic growth of both strains was nearly the same; however,after 80 h and until the end of the measurements, the mutant straingrew worse than did the wild type (Fig. 6A). Since the deletionof the hupSL genes in mutant AVM13 cells affected the growth underN₂-fixing conditions, the effect of the mutation on the nitrogenase,the key enzyme of nitrogen fixation which is also involved inhydrogen metabolism, was examined. The maximum of the nitrogenaseactivity could be determined about 24 h after induction of thecells. Both cultures had nearly the same nitrogenase activityafter 24 h, but in the following days, much higher values of acetylenereduction for the wild type were measured (Fig. 6B).

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FIG. 6. Bacterial growth (A), nitrogenase activity (B), and hydrogen production (C) of the A. variabilis wild type and AVM13 mutant strain under nitrogen-fixing conditions. After growing in BG11 medium containing combined nitrogen, the cells of the wild type and the mutant were washed with N-free medium BG11₀ and adjusted to the same cell density (measured by the chlorophyll $alpha$ content). Open circles, A. variabilis wild type; closed circles, AVM13 (A. variabilis hupSL interposon mutant).

Concerning the H₂ evolution, this paper demonstrates that the mutant AVM13 and the wild type produced equal rates of hydrogenin the first 16 h after induction with BG11₀ medium. At this time,the hupSL genes encoding the uptake hydrogenase were not expressed(data not shown). Contrastingly, after the expression of the hupSLoperon, the H₂ evolution of the mutant strain AVM13 increaseddramatically in the next 20 h, while for the wild type no changein the rates of H₂ evolution could be seen (Fig. 6C). Similarresults were obtained for another mutant, in which the neomycinresistance cassette was cloned in the opposite direction to thehupSL operon. Under nitrogen-fixing conditions, the mutant developedvery high rates of H₂ (68 nmol H₂/µg Chl $alpha$ × h) because the producedhydrogen could not be oxidized. The wild-type cells, however,consumed even more hydrogen than the nitrogenase produced ( $-$ 36nanomoles of H₂/micrograms of chlorophyll $alpha$ × h). The activityof the bidirectional NAD⁺-hydrogenase assayed under non-N₂-fixing conditions was very lowfor both the wild type and themutant.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The similarity of the uptake hydrogenase from Anabaena sp. strain PCC 7120 and A. variabilis allowed for the isolation ofa 4.8-kb HindIII fragment and of a 4.8-kb XbaI fragment of A.variabilis via hybridization of partial genomic libraries usingthe Anabaena sp. strain PCC 7120 hupL gene as a probe. The highdegree of similarity between the hupSL operon of A. variabilisand other filamentous cyanobacteria (Anabaena sp. strain PCC 7120,95%; Nostoc sp. strain PCC 73102, 90%) may reflect more stringentrequirements for the conservation of amino acids in the uptakehydrogenase. The noncoding region between hupS and hupL, however,shows only slight similarities between A. variabilis and Anabaenasp. strain PCC 7120 and no similarities between A. variabilisand Nostoc sp. strain PCC 73102. This may hint not only at thephysiological importance of the uptake hydrogenase but also atthe phylogenetic divergence during evolution in filamentouscyanobacteria.

Protein sequence alignment of the HupS and HupL subunits was done with several Ni-Fe hydrogenases from different bacterialgroups by using the ClustalW program (48; data not shown). Thelarge subunit of Ni-Fe hydrogenases contains the Ni atom in theactive site. As in the other organisms, one putative Ni-bindingsite (R-X-C-G-X-C) is located at the N-terminal site of the HupLprotein in A. variabilis. The second conserved Ni-binding site(D-P-C-X-X-C) is found at the C-terminal end. The small subunitof A. variabilis contains 11 Cys residues. Nine of them correspondwell to nine Cys residues of the known X-ray structure of thehydrogenase from Desulfovibrio gigas (52). HupS of D. gigashas two [4Fe-4S] clusters and one [3Fe-3S] cluster as prostheticgroups. The typical features of the small subunit of the dimericNi-Fe hydrogenase are the presence of a signal peptide at theN terminus and a motif located at the C terminus for anchoringthe uptake hydrogenase to the membrane (51). Both features couldnot be found for the HupS protein of A. variabilis and of Nostocsp. strain PCC 73102 (31). As Oxelfelt et al. pointed out, therole of the motifs is not yet clear and some examples of uptakehydrogenases which lack these featuresexist.

The cloning and sequencing of hydrogenase genes cluster led to the discovery of a number of accessory genes just up- and downstreamof the two structural genes (51). In Alcaligenes eutrophus,up to 20 ORFs encoding proteins that are essential for the formationof the active hydrogenase have been characterized (20). Therefore,we sequenced 3 kb upstream and 4 kb downstream of the hupSL operon.Eight ORFs were discovered, but none of them showed similaritiesto other known accessory genes. Two kilobases downstream of thehupL gene, two ORFs which might encode for proteins of glucosemetabolism could be detected. This means that the accessory genesof the uptake hydrogenase must be located elsewhere in the bacterialgenome.

During late stages of heterocyst differentiation, three DNA rearrangements were found in Anabaena sp. strain PCC 7120 (10,24). In vegetative cells, the genes nifD, fdxN, and hupL areinterrupted by insertions of DNA elements. After excision by site-specificrecombinases, the intact transcripts can be expressed in heterocysts.The nif1 region of A. variabilis, however, possesses only the11-kb element in the nifD gene and no interruption in the fdxNgene. The data in this study revealed the presence of a contiguoushupSL operon in A. variabilis. These results are supported bythe fact that the specific recombinase xisC of the hupL rearrangementof Anabaena sp. strain PCC 7120 could not be detected in Southernblot analysis with genomic DNA of A. variabilis (5). Besidethe nif1 region, A. variabilis has an alternative Mo-dependentnitrogenase gene cluster (nif2) which is transcribed only underanaerobic conditions (46). Low-stringency Southern hybridizationindicated that the hupL gene is a single-copy gene and that nosimilar ORFs for hupSL genes exist. Since the hupSL transcriptis induced only under nitrogen-fixing conditions, A. variabilishas to regulate the uptake hydrogenase in a different way. InNorthern analysis, we could show that the hupSL genes are probablytranscribed as a dicistronic operon of a 2.7-kb size. In lithoautotrophicbacteria, most of the known genes for the uptake hydrogenase areclustered in a polycistronic operon, often with a third gene encodingHupC (51). The hupSL transcript could only be detected in cellsgrown 24 h on an N-free medium. The nifDHK genes of A. variabilisare induced earlier (12 h) during heterocyst differentiation (datanot shown). This observation suggests that the hupSL genes aretranscribed during the late stages of heterocyst differentiationwhen the nitrogenase is already active. It has been reported thatthe levels of uptake hydrogenase activity in Anabaena sp. strainPCC 7120 are up to five times higher in cultures grown under H₂-N₂-CO₂conditions (25), so the endogenous H₂ produced by the nitrogenasemay act as an inducer of the hydrogenasesynthesis.

In cyanobacteria, promoter DNA elements that displayed a conserved element at $-$ 10 from the transcription initiation site couldbe found (15), which conforms to the E. coli $-$ 10 promoter consensussequence (TATAAT). The controlling promoters of genes encodingchimeric hydrogenases of hydrogen-oxidizing bacteria have alsobeen characterized (8, 35, 50). In most of the cases, sequenceelements resembling a $-$ 24/ $-$ 12 consensus sequence of $sigma$ ⁵⁴-dependent promoters are located just upstream of the transcriptionstart (39). Neither a TATAAT motif nor a $-$ 24/ $-$ 12 consensus sequencecould be detected upstream of the hupSL operon of A. variabilis.Interestingly, the location of a fumarate nitrate reductase regulator(Fnr)-binding motif and a $-$ 10 consensus motif, which was foundduring the regulation of the hyp operon in E. coli (26), wasconfirmed. Comparing the putative Fnr-binding site of the upstreamregion of the hupSL operon with the promoter of the hypBCDE transcript,the same succession of bases could be demonstrated; only the distanceof the motifs to the transcription site isdifferent.

DNase footprinting experiments and in vitro transcription confirm the unusual localization of the Fnr-binding site in thenapF control region in E. coli (16). As shown in Fig. 7, fourbases of the napF promoter sequence are modified from the Fnrconsensus sequence, but only one base is exchanged in the promoterregion of hupSL as compared with the napF promoter. During anaerobicgrowth, the Fnr protein induces the expression of several operonsin E. coli (43). In A. variabilis, the induction of the hupSLoperon occurs within the heterocysts. Heterocysts are terminallydifferentiated cells whose interiors become anaerobic. This suggestsa similar regulation of the hupSL operon compared with that ofE. coli.

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FIG. 7. Nucleotide sequences of the consensus Fnr-binding site, the Fnr-binding site within the napF promoter of E. coli, and the promoter of the hupSL operon of A. variabilis. Three nucleotides out of 10 are different between the consensus sequence of the Fnr-binding site in E. coli, the napF (periplasmic nitrate reductase) promoter, and the hupSL promoter of A. variabilis.

The fivefold repeats (TA/GACAAC) downstream of the transcription site are another interesting structure which represent anew type of short tandemly repeated heptamers. Cyanobacterialgenomes have a variety of such tandemly repeated sequences withunknown function, but most of them are specific to the heterocystousstrains (24). It has been reported that these sequences mightbe a target of specific DNA-binding proteins for chromosome condensation(27). Further promoter analyses are needed to understand thetranscription of the hupSLoperon.

We also studied the induction of in vivo hydrogen uptake and nitrogenase activities under N-limiting conditions in the wildtype and the hupSL mutant of A. variabilis. There are two hintsthat, in the light, the measured hydrogen originates from thenitrogenase activity. Firstly, hydrogen photoproduction of A.variabilis cultures did not occur under NO₃-saturated conditions in which the nitrogenase genes are not expressed.In BG11 medium, a slight H₂ production was measured only in thedark, which indicates a low catalytic activity of the bidirectionalhydrogenase. Secondly, the curve diagram of the H₂ evolution correspondswell with the one of acetylene reduction. After 24 h of growthunder nitrogen-fixing conditions, the maximal H₂ production andnitrogenase activity could be observed. Similar effects have beendescribed earlier (28, 49). Though a lot of biochemical andgenetical studies have been done, the in vivo function of theuptake hydrogenase is poorly understood at present. In this study,the physiological data clearly show that the uptake hydrogenasereoxidizes the produced hydrogen at high rates in the wild type.Three to five times more hydrogen is produced by the hupSL mutant,dependent on the growth situations. It was shown that the electronsof the oxidized H₂ are fed into the respiratory chain, proceedingto an oxyhydrogen reaction coupled to oxidative phosphorylation(33). The electron transport from H₂ to O₂ supports ATP synthesisand thereby supplies part of the energy required by the nitrogenaseand also protects the nitrogenase by lowering intracellular O₂levels. The hupSL mutant fixed nitrogen after 35 h at lower ratesthan the wild type. However, the growth curves were almost thesame, suggesting that the uptake hydrogenase is not absolutelyessential under diazotrophic culture conditions. Obviously, thereduced rates of fixed nitrogen have only a slight effect on thegrowth of the mutantstrain.

	ACKNOWLEDGMENTS

We thank James W. Golden for the plasmids containing the hupL gene of Anabaena sp. strain PCC 7120 and C. Peter Wolk for thepRL plasmids. We also thank H. Geithmann for photographicwork.

This work was supported by the Deutsche Forschungsgemeinschaft (Ha 2555/1-1).

	FOOTNOTES

^* Corresponding author. Mailing address: Botanisches Institut der Universität Bonn, Karlrobert-Kreiten-Str. 13, D-53115 Bonn,Germany. Phone: 49-228-73-5516. Fax: 49-228-73-1697. E-mail: t.happe{at}uni-bonn.de.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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	ALL ASM JOURNALS

1.	Altschul, S. F., W. Miller, E. W. Myers, and D. J. Lipman. 1997. Basic local alignment search tool. J. Mol. Biol. 215:403-410.
2.	Ansorge, W., B. Sproat, J. Stegemann, C. Schwager, and M. Zenke. 1987. Automated DNA sequencing: ultrasensitive detection of fluorescent bands during electrophoresis. Nucleic Acids Res. 15:4593-4602[Abstract/Free Full Text].
3.	Appel, J., and R. Schulz. 1996. Sequence analysis of an operon of a nickel hydrogenase from the cyanobacterium Synechocystis sp. PCC 6803. Biochim. Biophys. Acta 1298:141-147[CrossRef][Medline].
4.	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. Greene Publishing Associates and Wiley-Interscience, New York, N.Y.
5.	Axelsson, R., F. Oxelfelt, and P. Lindblad. 1999. Transcriptional regulation of Nostoc uptake hydrogenase. FEMS Microbiol. Lett. 170:77-81[CrossRef][Medline].
6.	Böhme, H. 1998. Regulation of nitrogen fixation in heterocyst-forming cyanobacteria. Trends Plant Sci. 9:346-351[CrossRef].
7.	Boison, G., O. Schmitz, L. Mikheeva, S. Shestakov, and H. Bothe. 1996. Cloning, molecular analysis and insertional mutagenesis of the bidirectional hydrogenase genes from the cyanobacterium Anacystis nidulans. FEBS Lett. 394:153-158[CrossRef][Medline].
8.	Brito, B., M. Martinez, D. Fernandez, L. Rey, E. Cabrera, J. M. Palacios, J. Imperial, and T. Ruiz-Argueso. 1997. Hydrogenase genes from Rhizobium leguminosarum bv. viciae are controlled by the nitrogen fixation regulatory protein nifA. Proc. Natl. Acad. Sci. USA 94:6019-6024[Abstract/Free Full Text].
9.	Buikema, W. J., and R. Haselkorn. 1993. Molecular genetics of cyanobacterial development. Annu. Rev. Plant Physiol. Plant Mol. Biol. 44:333-352[CrossRef].
10.	Carrasco, C. D., J. A. Buettner, and J. W. Golden. 1995. Programmed DNA rearrangement of the cyanobacterial hupL gene in heterocysts. Proc. Natl. Acad. Sci. USA 92:791-795[Abstract/Free Full Text].
11.	Casadaban, M., and S. N. Cohen. 1980. Analysis of gene control signals by DNA fusion and cloning in Escherichia coli. J. Mol. Biol. 138:179-207[CrossRef][Medline].
12.	Castenholz, R. W. 1988. Culturing methods for cyanobacteria. Methods Enzymol. 167:68-93.
13.	Cohen, S. N., A. C. Chang, and L. Hsu. 1972. Nonchromosomal antibiotic resistance in bacteria: genetic transformation of Escherichia coli by R-factor DNA. Proc. Natl. Acad. Sci. USA 69:2110-2114[Abstract/Free Full Text].
14.	Currier, T. C., and C. P. Wolk. 1979. Characteristics of Anabaena variabilis influencing plaque formation by cyanophage N-1. J. Bacteriol. 171:4138-4145.
15.	Curtis, S. E., and J. A. Martin. 1994. The transcription apparatus and the regulation of transcription initiation, p. 769-823. In D. A. Bryant (ed.), The molecular biology of cyanobacteria. Kluwer Academic Publishers, Dordrecht, The Netherlands.
16.	Darwin, A. J., E. C. Ziegelhoffer, P. J. Kiley, and V. Stewart. 1998. Fnr, NarP, and NarL regulation of Escherichia coli K-12 napF (periplasmic nitrate reductase) operon transcription in vitro. J. Bacteriol. 180:4192-4198[Abstract/Free Full Text].
17.	Dilworth, M. J. 1966. Acetylene reduction by nitrogen fixing preparations from Clostridium pasteurianum. Biochim. Biophys. Acta 127:285-294[Medline].
18.	Elhai, J., and C. P. Wolk. 1988. Conjugal transfer of DNA to cyanobacteria. Methods Enzymol. 167:747-754[Medline].
19.	Elhai, J., A. Vepritskiy, A. M. Muro-Pastor, E. Flores, and C. P. Wolk. 1997. Reduction of conjugal transfer efficiency by three restriction activities of Anabaena sp. strain PCC 7120. J. Bacteriol. 179:1998-2005[Abstract/Free Full Text].
20.	Friedrich, B., and E. Schwartz. 1993. Molecular biology of hydrogen utilization in aerobic chemolithotrophs. Annu. Rev. Microbiol. 47:351-383[CrossRef][Medline].
21.	Gish, W., and D. J. States. 1993. Identification of protein coding regions by database similarity search. Nat. Genet. 3:166-172.
22.	Hahn, D., and U. Kueck. 1994. Biochemical and molecular genetic basis of hydrogenases. Process Biochem. 29:633-641[CrossRef].
23.	Happe, T., and J. D. Naber. 1993. Isolation, characterization and N-terminal amino acid sequence of hydrogenase from the green alga Chlamydomonas reinhardtii. Eur. J. Biochem. 214:475-481[Medline].
24.	Haselkorn, R., and W. J. Buikema. 1992. Nitrogen fixation in cyanobacteria, p. 166-190. In G. Stacey, H. J. Evans, and R. H. Burris (ed.), Biological nitrogen fixation. Chapman and Hall, New York, N.Y.
25.	Houchins, J. P. 1984. The physiology and biochemistry of hydrogen metabolism in cyanobacteria. Biochim. Biophys. Acta 768:227-255.
26.	Lutz, S., A. Jacobi, V. Schlensog, R. Bohm, G. Sawers, and A. Bock. 1991. Molecular characterization of an operon (hyp) necessary for the activity of the three hydrogenase isoenzymes in Escherichia coli. Mol. Microbiol. 5:123-135[Medline].
27.	Mazel, D., J. Houmard, A. M. Castets, and N. Tandeau de Marsac. 1990. Highly repetitive DNA sequences in cyanobacterial genomes. J. Bacteriol. 172:2755-2761[Abstract/Free Full Text].
28.	Mikheeva, L. E., O. Schmitz, S. V. Shestakov, and H. Bothe. 1995. Mutants of the cyanobacterium Anabaena variabilis altered in hydrogenase activities. Z. Naturforsch. 50c:505-510.
29.	Myöhänen, S., and J. Wahlfors. 1993. Automated fluorescent primer extension. BioTechniques 14:16-17[Medline].
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