Isolation and Characterization of a Soluble NADPH-Dependent Fe(III) Reductase from Geobacter sulfurreducens

doi:10.1128/JB.183.15.4468-4476.2001

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Journal of Bacteriology, August 2001, p. 4468-4476, Vol. 183, No. 15
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.15.4468-4476.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Isolation and Characterization of a Soluble NADPH-Dependent Fe(III) Reductase from Geobacter sulfurreducens

Franz Kaufmann and Derek R. Lovley^*

Department of Microbiology, Morrill Science Center, University of Massachusetts, Amherst, Massachusetts 01003

Received 1 February 2001/Accepted 2 May 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

NADPH is an intermediate in the oxidation of organic compounds coupled to Fe(III) reduction in Geobacter species, but Fe(III)reduction with NADPH as the electron donor has not been studiedin these organisms. Crude extracts of Geobacter sulfurreducenscatalyzed the NADPH-dependent reduction of Fe(III)-nitrilotriaceticacid (NTA). The responsible enzyme, which was recovered in thesoluble protein fraction, was purified to apparent homogeneityin a four-step procedure. Its specific activity for Fe(III) reductionwas 65 µmol · min¹ · mg¹. The soluble Fe(III) reductase was specific for NADPH and didnot utilize NADH as an electron donor. Although the enzyme reducedseveral forms of Fe(III), Fe(III)-NTA was the preferred electronacceptor. The protein possessed methyl viologen:NADP⁺ oxidoreductase activity and catalyzed the reduction of NADP⁺ with reduced methyl viologen as electron donor at a rate of 385U/mg. The enzyme consisted of two subunits with molecular massesof 87 and 78 kDa and had a native molecular mass of 320 kDa, asdetermined by gel filtration. The purified enzyme contained 28.9mol of Fe, 17.4 mol of acid-labile sulfur, and 0.7 mol of flavinadenine dinucleotide per mol of protein. The genes encoding thetwo subunits were identified in the complete sequence of the G.sulfurreducens genome from the N-terminal amino acid sequencesderived from the subunits of the purified protein. The sequencesof the two subunits had about 30% amino acid identity to the respectivesubunits of the formate dehydrogenase from Moorella thermoacetica,but the soluble Fe(III) reductase did not possess formate dehydrogenaseactivity. This soluble Fe(III) reductase differs significantlyfrom previously characterized dissimilatory and assimilatory Fe(III)reductases in its molecular composition and cofactorcontent.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Dissimilatory Fe(III) reduction plays an important role in the degradation of natural and contaminant organic matter underanaerobic conditions (29). The ability to couple growth withthe reduction of Fe(III) has been found in phylogenetically diversemembers of the Bacteria and Archaea (25, 27), and geologicaland microbiological evidence suggests that Fe(III) reduction wasone of the earliest forms of microbial respiration (26, 50).Studies on the physiology and biochemistry of dissimilatory Fe(III)reduction have focused largely on members of the genera Shewanellaand Geobacter. Shewanella species are gram-negative facultativeanaerobes that can use a variety of electron acceptors includingFe(III) (36, 37). Geobacter species are strictly anaerobic,gram-negative organisms that can couple the complete oxidationof organic matter to the reduction of Fe(III) (27). Membersof the genus Geobacter are found in a variety of freshwater andsedimentary environments in which Fe(III) reduction is a dominantelectron-accepting process (9, 47).

The mechanisms for electron transfer to Fe(III) in dissimilatory Fe(III)-reducing microorganisms have yet to be determined.In most environments, much of the Fe(III) is present as insolubleFe(III) oxide, and it has generally been considered that Fe(III)-reducingorganisms must be in close contact with this insoluble Fe(III)in order to reduce it (28). A number of studies have identifiedmembrane-associated c-type cytochromes in Shewanella (12, 18,36) and Geobacter (16, 24, 33) species which can reduceFe(III) in vitro, and it has been suggested that these cytochromesare involved in electron transport to extracellular Fe(III). However,it has yet to be proven that the Fe(III) derived from Fe(III)oxide is reduced extracellularly. Furthermore, soluble Fe(III)is present in a variety of sedimentary environments in which microbialFe(III) reduction is important (32, 38, 43), and the presenceof chelators that solubilize Fe(III) can greatly stimulate Fe(III)reduction (31). This suggests that soluble Fe(III) could alsoserve as an electronacceptor.

Recent studies on acetate oxidation in Geobacter species demonstrated that NADPH is an intermediate of the tricarboxcylicacid cycle (7, 15). In this study we describe the purificationand characterization of an enzyme from G. sulfurreducens thatcatalyzes the reduction of soluble Fe(III) with NADPH as the electrondonor.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell growth. G. sulfurreducens strain PCA (ATCC 51573) was obtained from our laboratory culture collection and cultivated in an anaerobicfreshwater medium, containing 20 mM sodium acetate as the electrondonor and either 50 mM ferric citrate or 40 mM fumarate as theelectron acceptor, under an atmosphere of N₂-CO₂ (80:20) (6).Cells were grown in 1-liter Pyrex bottles filled with 0.9 literof medium or, for mass cultivation, in 10-liter carboys. The cellswere harvested at the end of the exponential growth phase by centrifugationand washed in anaerobic 50 mM HEPES (pH 7.0) containing 5 mM dithiothreitoland 1 mM MgCl₂. The washed cells were suspended in 1 ml of anaerobic50 mM HEPES (pH 7.0) per g of wet cells and stored at $-$ 80°C.

Enzyme assays. All enzyme assays were performed at 30°C in a UV2401-PC dual-beam spectrophotometer (Shimadzu, Baltimore, Md.) equipped witha temperature-controlled cuvette holder. Fe(III) reductase activitywas routinely measured aerobically by monitoring the reductionof Fe(III) to Fe(II) using the colorimetric Fe(II) capture agentferrozine [3-(2-pyridyl)-5,6-(4-phenylsulfonic acid)-1,2,4-triazine].Reaction mixtures (1.0 ml) contained 50 mM MES (pH 5.5), 1.0 mMferrozine, 2 mM Fe(III)-nitrilotriacetic acid [Fe(III)-NTA], and200 µM NADPH. The reactions were started by the addition of eitherNADPH or protein (1 to 200 µg), and the formation of the Fe(II)-ferrozinecomplex was monitored at 562 nm ( $varepsilon$ = 28 mM¹ · cm¹). One unit is the amount of enzyme catalyzing the reduction of1 µmol of Fe(III) per min. In the absence of NADPH, the additionof crude extract to the assay mixture resulted in the reductionof 5 to 10 µM Fe(III) over 2 to 3 min. Therefore, enzymatic assayson crude extracts were initiated by the addition of NADPH afterthis nonspecific reduction of Fe(III) ceased. Reduction of otherforms of Fe(III) was determined similarly by replacing Fe(III)-NTAwith 1 mM Fe(III)-EDTA, 1 mM Fe(III)-citrate, or 0.5 mmol of Fe(III)-oxyhydroxideper liter. The pH optimum of the enzyme was determined using thefollowing buffers: 100 mM acetate at pH 4.0, 4.5 and 5.0; 50 mM2-[N-morpholino]ethanesulfonic acid-NaOH (MES) at pH 5.0, 5.5,6.0, and 6.5; 50 mM 3-(N-morpholino]propanesulfonic acid)-NaOH(MOPS) at pH 6.5 and 7.0; and 50 mM Tris-HCl at pH 7.0, 7.5, and8.0.

The reduction of menadione (2-methyl-1,4-naphthoquinone) was assayed by monitoring the oxidation of NADPH at 366 nm ( $varepsilon$ = 3.3mM¹ · cm¹). The reaction mixtures (1 ml) contained 50 mM MES (pH 5.5),0.3 mM NADPH, and 0.5 mM menadione. The reactions were startedby the addition of enzyme (5 to 20 µg) ormenadione.

Methyl viologen:NADP⁺ oxidoreductase activity was measured under anaerobic conditions in an assay mixture (1 ml) containing50 mM Tris-HCl (pH 7.5), 10 mM methyl viologen, and 0.3 mM NADP⁺. Before the reaction was initiated by adding either enzyme (1to 5 µg) or NADP⁺, the reaction mixture was reduced chemically to an absorptionat 578 nm of 1.5 by adding 0.1 M Ti(III) citrate. Oxidation ofmethyl viologen was monitored at 578 nm ( $varepsilon$ = 9.7 mM¹ · cm¹). Malate dehydrogenase activity was measured by monitoring theoxidation of NADH at 340 nm ( $varepsilon$ = 6.22 mM¹ · cm¹) in the presence of oxaloacetate (44). Reaction mixtures (1ml) contained 50 mM HEPES-NaOH (pH 7.0), 0.2 mM NADH, and 0.4mM oxaloacetate. Reactions were started by the addition of crudeextract (10 to 30 µg) or oxaloacetate. Formate dehydrogenase wasassayed under anaerobic conditions in a reaction mixture (1 ml)containing 50 mM Tris-HCl (pH 7.5), 3 mM dithiothreitol, 10 mMformate, and 10 mM methyl viologen. The reaction mixture was reducedto give a slight blue color by adding 0.1 M Ti(III)-citrate. Reactionswere started by adding enzyme (5 to 20 µg) or formate, and thereduction of methyl viologen was monitored at 578 nm ( $varepsilon$ = 9.7mM¹ · cm¹).

Preparation of subcellular fractions. All manipulations were carried out under anaerobic conditions in a glove bag under an atmosphere of 7% CO₂-5% H₂ balancedwith N₂. Solutions were made anaerobic by repeatedly evacuatingand flushing them with oxygen-free N₂ passed over a heated coppercolumn. Subcellular fractions were prepared using a modificationof the method of Gaspard et al. (16). Freshly harvested cells(about 1 g [wet weight]) were washed in 100 ml of anaerobic 50mM HEPES buffer (pH 7.0) and resuspended in 20 ml of 100 mM Tris-HCl(pH 8.0) containing 25% (wt/vol) sucrose. Lysozyme (20 mg) wasadded, and the suspension was stirred for 20 min. Following theaddition of Na₂-EDTA (pH 8.0) to a final concentration of 5 mMand stirring for 15 min, MgCl₂ was added to a final concentrationof 13 mM and the suspension was stirred for another 15 min. Microscopicexamination of the suspension revealed that almost all the cellshad been converted to spheroplasts by this treatment. After centrifugationfor 30 min at 20,000 × g at 4°C to pellet the spheroplasts, thesupernatant was reserved as the periplasmic fraction. The pelletwas resuspended in 20 ml of 10 mM HEPES (pH 7.0). To lyse thespheroplasts, a few crystals of DNase I were added and the suspensionwas frozen and thawed twice. The resulting crude extract was centrifugedfor 30 min at 20,000 × g to remove unlysed cells and cell debris.The supernatant was subsequently centrifuged for 1 h at 100,000× g to pellet the membranes. The final supernatant, the cytoplasmicfraction, was reserved for further analysis, and the membranepellet was suspended in 5 ml of 50 mM HEPES (pH 7.0).

Purification of soluble Fe(III) reductase. Wet cells (10 to 20 g) were suspended in 10 to 20 ml of 50 mM HEPES (pH 7.0), amended with a few crystals of DNase I, anddisrupted by passage through a French pressure cell at 40,000kPa. The crude extract was centrifuged for 1 h at 100,000 × gat 4°C to pellet cell debris and membranes. Soluble Fe(III) reductasewas purified in an anaerobic glove bag at 20°C. All buffers weremade anaerobic as described above. The ultracentrifuged crudeextract (ca. 30 ml) was filtered (0.2-µm-pore-size filters), dilutedto 90 ml with 25 mM MOPS (pH 6.5), and applied to a Q-SepharoseHP column (1.6 by 10 cm; Amersham Pharmacia Biotech, Piscataway,N.J.) equilibrated with 25 mM MOPS (pH 6.5). Protein was elutedwith a linear gradient of 0 to 0.4 M NaCl (240 ml). Fractionscontaining Fe(III) reductase activity eluted at about 0.22 M NaCl.The pooled fractions were amended with 50 mM Tris-HCl (pH 7.5)containing 3.2 M ammonium sulfate to give a final concentrationof 0.7 M ammonium sulfate and applied to a butyl-Sepharose HiPrepcolumn (1.6 by 10 cm; Amersham Pharmacia Biotech) equilibratedwith 50 mM Tris-HCl (pH 7.5) containing 0.7 M ammonium sulfate.Bound protein was eluted in a linear gradient of 0.7 to 0 M ammoniumsulfate (200 ml). Fractions containing Fe(III) reductase activity,which eluted at 0.5 M ammonium sulfate, were pooled and concentratedto ca. 1.5 ml using Ultrafree-15 (30-kDa cutoff) centrifugal filterdevices (Millipore, Bedford, Mass.). The concentrated pool wasfiltered (0.2-µm-pore-size filters) and applied to a Superdex200 prep grade column (1.6 by 60 cm; Amersham Pharmacia Biotech)equilibrated with 50 mM Tris-HCl (pH 7.5), and the protein waseluted with the same buffer. Fe(III) reductase-containing fractionswere pooled and applied to a MonoQ column (0.5 by 5 cm; AmershamPharmacia Biotech) equilibrated with 50 mM Tris-HCl (pH 7.5) containing20% (vol/vol) ethylene glycol. Protein was eluted with a gradientof 0.1 to 0.3 M NaCl, and the soluble Fe(III) reductase elutedat 0.2 MNaCl.

Molecular weight determination. The native M_r of the soluble Fe(III) reductase was determined by gel filtration on a Superdex 200 column (1.6 by 60 cm; AmershamPharmacia Biotech) with 50 mM Tris-HCl (pH 7.5) containing 0.15M NaCl as the elution buffer. Thyroglobulin (M_r 669,000), apoferritin(M_r 443,000), $beta$ -amylase (M_r 200,000), alcohol dehydrogenase (M_r150,000), and bovine serum albumin (M_r 66,000) were used as molecularweightstandards.

Gel electrophoresis. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) was carried out by the method of Laemmli (23). Phosphorylaseb (M_r 97,000), bovine serum albumin (M_r 66,000), ovalbumin (M_r45,000), carbonic anhydrase (M_r 30,000), trypsin inhibitor (M_r20, 000), and $alpha$ -lactalbumin (M_r 14,400) were used as molecularweight standards. Proteins were separated on 10% polyacrylamidegels and stained with Coomasssie brilliantblue.

Determination of flavin, iron, and sulfur contents. To determine the flavin cofactor content, purified Fe(III) reductase (0.5 to 1 µM) was air oxidized and extracted with 5%(wt/vol) trichloroacetic acid. Denatured protein was removed bycentrifugation, and the pH of the supernatant was adjusted to6.0 with 2 M K₂HPO₄. Then 20 µl of supernatant was analyzed byhigh-pressure liquid chromatography using a Supelcosil-LCPAH column(Supelco, Bellefonte, Pa.). The mobile phase was 20 mM ammoniumacetate buffer (pH 6.0) containing 21% acetonitrile and was usedat a flow rate of 0.5 ml/min (retention times: flavin adeninedinucleotide [FAD], 3.2 min; flavin mononucleotide [FMN], 4.2min). Flavins were detected with a HP1312A fluorescence detector(Hewlett-Packard, Wilmington, Del.) by their emission at 525 nmfollowing excitation at 260 nm (2).

Iron content was determined as described by Fish (13), using an iron volumetric standard (Aldrich, Milwaukee, Wis.). Acid-labilesulfur was estimated by the method of Rabinowitz (42) with ferredoxinfrom Clostridium pasteurianum as a reference. The presence ofiron, molybdenum, tungsten, and selenium was tested by inductivelycoupled plasma mass spectrometry (ICP-MS) analysis by A. Siripinyfrom the Department of Chemistry at the University of Massachusetts,Amherst, Mass., using a Sciex Elan 6000 instrument (Perkin-Elmer,Norwalk, Conn.). Total protein was determined by the bicinchoninicacid method (46) with bovine serum albumin as standard. Thecofactor content was calculated based on protein determinationand a native molecular mass of 320kDa.

Determination of N-terminal amino acid sequences. For N-terminal amino acid sequencing, the purified protein was separated by SDS-PAGE and transferred to a polyvinylidene difluoridemembrane. The amino acid sequences were determined by automatedEdman degradation (J. Leszyk, University of Massachusetts MedicalSchool, Worcester, Mass.). The N-terminal amino acid sequenceswere used to search the preliminary sequence data of the G. sulfurreducensgenome available at The Institute for Genomic Research (http://www.tigr.org).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Localization of NADPH-dependent Fe(III) reductase. Crude extracts of G. sulfurreducens catalyzed the reduction of Fe(III)-NTA with NADPH as the electron donor at a rate of 0.24µmol · min¹ · mg¹. More than 90% of the NADPH-dependent Fe(III) reductase activitywas localized in the cytoplasmic fraction (Table 1). A similardistribution was found for malate dehydrogenase, an enzyme knownto reside in the cytoplasm (53). These results suggest thatthe NADPH-dependent Fe(III) reductase is a soluble enzyme presenteither in the cytoplasm or only loosely associated with the innermembrane.

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TABLE 1. Localization of Fe(III) reductase

Purification and properties of soluble Fe(III) reductase. Crude extracts prepared from cells grown with fumarate as the electron acceptor exhibited the same level of soluble Fe(III)reductase activity as did those prepared from cells grown on Fe(III)citrate (data not shown). This suggests that G. sulfurreducensconstitutively produces this enzyme. Therefore, the enzyme waspurified from cells grown on fumarate because it was technicallysimpler to mass culture the organism onfumarate.

Incubation of the crude extract under air for 2 h resulted in the loss of about 75% of the Fe(III) reductase activity. Dueto this apparent oxygen sensitivity, the enzyme was purified understrictly anaerobic conditions. Using a four-step procedure, theenzyme was purified to apparent homogeneity with a yield of about20% (Table 2). The specific activities of the final preparationvaried from 40 to 70 U/mg.

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TABLE 2. Purification of soluble Fe(III) reductase

Physical characterization. The native molecular mass of the soluble Fe(III) reductase was determined by gel filtration to be 320 kDa. In SDS-PAGE, twosubunits with relative molecular masses of 87 ( $alpha$ ) and 78 ( $beta$ ) kDawere detected in equal amounts (Fig. 1). This suggests an $alpha$ ₂ $beta$ ₂configuration for the native protein.

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FIG. 1. SDS-PAGE of purified soluble Fe(III) reductase. Lanes: 1, molecular mass markers (in kilodaltons); 2, 0.7 µg of soluble Fe(III) reductase. Proteins were resolved on a 10% polyacrylamide gel and stained with Coomassie brilliant blue.

The purified protein was yellowish brown, and the UV-visible spectrum had a broad absorption ranging from 360 to 500 nm witha peak at 390 nm and a slight shoulder at 450 nm. The absorptionpeak at 390 nm indicated the possible presence of iron-sulfurclusters (40).

Using ICP-MS, 28.9 ± 0.4 (mean ± standard deviation; n = 2) mol of iron per mol of protein was detected in two different preparationsof the enzyme. The same value was obtained with a third enzymepreparation using ferrozine to determine the iron content colorimetrically(13). Since the sequence of soluble Fe(III) reductase showedthe highest similarity to formate dehydrogenases (see below),which can contain W, Mo, and Se, the presence of these metalsin the protein was also investigated. However, no W, Mo, or Secould be detected by ICP-MS. Determination of acid-labile sulfurgave a value of 17.4 ± 2.5 (n = 2) mol per mol ofprotein.

A trichloroacetic acid extract of the protein had a UV-visible spectrum typical for flavins (data not shown). High-pressureliquid chromatography analysis combined with fluorescence detectionrevealed the presence of 0.7 mol of FAD per mol of protein. Smallamounts of FMN (<0.2 mol/mol) were alsodetected.

Enzymatic properties. The Fe(III) reductase had a pH optimum of 5.5, and the highest activity was found at 45°C. The enzyme had a strict specificityfor NADPH and did not utilize NADH as an electron donor. In contrastto previously described soluble Fe(III) reductases (14, 48),the addition of FAD or FMN to the enzyme assay mixture did notstimulate its activity. The apparent K_m values for NADPH and Fe(III)-NTAwere estimated to be 25 µM and 1 mM,respectively.

The enzyme preferentially reduced Fe(III)-NTA over the other forms of Fe(III) that were evaluated. Fe(III) complexed withEDTA or citrate was reduced at rates less than 5% of that observedwith Fe(III)-NTA. Synthetic Fe(III)-oxyhydroxide was reduced bythe enzyme at a rate of 2.5% compared to Fe(III)-NTA.

The enzyme did not reduce menadione with NADPH as the electron donor, suggesting that it cannot transfer electrons to quinones.The protein catalyzed the reduction of NADP⁺ with reduced methyl viologen as the electron donor at a rateof 385 U/mg.

Because of the sequence similarity of soluble Fe(III) reductase to a formate dehydrogenase (see below), the formate dehydrogenaseactivity of the protein was examined. However, there was no formatedehydrogenase activity with formate as the electron donor andmethyl viologen as the electron acceptor. Furthermore, formatewas not an electron donor for the reduction of Fe(III)-NTA.

Amino acid sequence analysis of soluble Fe(III) reductase. The N-terminal sequence of the $alpha$ subunit as determined by automated Edman degradation was Met-Val-Ser-Leu-Thr-Ile-Asp-Gly-Lys-Asp-Ile-Thr-Val-Ala-Lys-Glu-Thr-Thr-Ile-Leu.The N-terminal sequence of the $beta$ subunit was Ala-Gln-Val-Val-Phe-Ser-Ser-Trp-Gly-Arg-Thr-Ile-Val-Asp-Asn-Arg-Lys-Gly-Gly-Glu.These sequences were used to search the preliminary G. sulfurreducensgenome sequence database of The Institute of Genomic Research,and 100% matches were found. The open reading frame containingthe N-terminal sequence of the $alpha$ subunit encoded a polypeptideof 844 amino acids with a predicted molecular weight of 89,386.This molecular weight was consistent with the molecular weightof the $alpha$ subunit determined by SDS-PAGE (Fig. 1). Thus, the geneencoding this protein was designated sfrA (for "soluble Fe(III)reductase alpha subunit"). An open reading frame containing theN-terminal sequence of the beta subunit of the soluble Fe(III)reductase was located upstream of sfrA. The encoded protein consistedof 671 amino acids and had a predicted molecular weight of 74,142,which was consistent with the molecular weight determined forthe $beta$ subunit of the purified enzyme. This gene was thereforedesignated sfrB. The two genes were separated by 126 bp and translatedin the same reading frame. Hypothetical proteins encoded by openreading frames identified in the flanking regions of SfrA andSfrB did not show significant sequence similarities to proteinsof known function (data notshown).

Databases were searched for similar proteins by using the BLAST algorithm (1). SfrA had the highest overall sequence similarity(32% identical and 49% similar amino acids) to the large subunitof the tungsten- and selenium-containing NADP⁺-dependent formate dehydrogenase (FdhA) from Moorella thermoacetica(52). Other similar proteins included chain G2 of NADH dehydrogenaseI (NuoG) from Sinorhizobium meliloti (GenBank accession numberP56914) (31% identical and 50% similar amino acids) and thelarge subunit of molybdenum-containing formate dehydrogenase (FdsA)from Ralstonia eutropha (39) (29% identical and 45% similaramino acids). The N-terminal part (residues 1 to 240) of SfrA,FhaA, NuoG, and FdsA contains five clusters of Cys residues (Fig.2) that are thought to be involved in the binding of two [2Fe-2S]and three [4Fe-4S] clusters (39). The arrangement of the iron-sulfurcluster binding motifs in SfrA is similar to that in chain G ofNADH dehydrogenase from various organisms and is not conservedin formate dehydrogenase sequences except for FdhA from M. thermoaceticaand FdsA from R. eutropha (39). Structural information fromformate dehydrogenase H from Escherichia coli (4) and sequencecomparison of formate dehydrogenases (39) demonstrated thattwo conserved regions within the large subunit (F1 and F2 in Fig.2) form the active site for formate oxidation. While some conservationis seen in these regions between SfrA and the formate dehydrogenasesof M. thermoacetica and R. eutropha, SfrA lacks the residues thatare catalytically important for formate oxidation. These residues(boxed in Fig. 2) include a Cys (or SeCys) residue in region F1which is a ligand to the heavy-metal atom (Mo or W) of the molybdopterincofactor, a neighboring His residue, and an Arg residue in regionF2 (4).

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FIG. 2. Alignment of SfrA with related proteins. Identical and conservatively substituted residues are highlighted by black and gray backgrounds, respectively. Putative binding regions for iron-sulfur clusters are indicated, and the potential cluster-ligating residues are highlighted by asterisks. F1 and F2 indicate regions that are conserved in formate dehydrogenase sequences, with the active-site residues in boxes (see the text). Abbreviations: SfrA G.s., soluble Fe(III) reductase $alpha$ subunit from G. sulfurreducens; FdhA M.t., formate dehydrogenase $alpha$ subunit from M. thermoacetica (GenBank accession number U73807); NuoG S.m., NADH dehydrogenase I chain G 2 from S. meliloti (GenBank accession number P56914); FdsA R.e., soluble formate dehydrogenase $alpha$ subunit from R. eutropha (39).

SfrB is most similar to the beta subunit of formate dehydrogenase (FdhB) from M. thermoacetica (38% identity and 50% similarity)and to the small subunit of glutamate synthase (GltD) (about 35%identity and 48% similarity) from different organisms (Pyrococcusabyssi, Thermotoga maritima, Aquifex aeolicus, and E. coli). Analignment of SfrB with FdhB from M. thermoacetica and GltD fromP. abyssi and E. coli is provided in Fig. 3. Residues 386 to 420resemble a consensus sequence proposed to be responsible for NAD(P)Hbinding in glutamate synthase (41). Residues 254 to 282 resemblea consensus sequence for the formation of an ADP binding foldin NAD(P)H-dependent and FAD-containing oxidoreductases (34,51) that is thought to be involved in FAD binding. In the C-terminalpart of SfrB, another conserved region is present (residues 550to 560) that is indicative of FAD binding (11). The N-terminalpart of SfrB (residues 1 to 220, 12 Cys) is similar to the correspondingregion of GltD which is thought to provide Cys ligands for two[4Fe-4S] clusters (49). Residues 202 to 214 of SfrB resembleone of the proposed binding motives for a [4Fe-4S] cluster inGltD (21). In addition, the N-terminal region of SfrA showedsimilarity to iron-sulfur cluster binding domains found in hydrogenases(e.g., the HoxF subunit from the cyanobacteria Anabaena variabilisand Synechococcus strain PCC6301 [45]) and chain F of NADH dehydrogenaseI. Although these similarities and the large number of Cys residuessuggest that SfrB might bind more than one [Fe-S] cluster, sequencecomparison did not indicate potential binding sites for theseclusters.

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FIG. 3. Alignment of SfrB with related proteins. Identical and conservatively substituted residues are highlighted by black and gray backgrounds, respectively. Putative binding regions for an iron-sulfur cluster are indicated, and the potential cluster-ligating residues are highlighted by asterisks. Potential binding sites for FAD and NADPH are indicated (see the text). Abbreviations: SfrB G.s., soluble Fe(III) reductase $beta$ subunit from G. sulfurreducens; FdhB M.t., formate dehydrogenase $beta$ subunit from M. thermoacetica (GenBank accession number U73807); GltD P.a., glutamate synthase $beta$ subunit from P. abyssi (GenBank accession number E75069); GltD E.c., glutamate synthase $beta$ subunit from E. coli (19).

There was some discrepancy between the amounts of iron (29 mol) and acid-labile sulfur (17 mol) that were determined analyticallyand the amounts of iron and sulfur (40 mol each) that would bepredicted for the $alpha$ ₂ $beta$ ₂ holoenzyme based on the potential bindingsites for two [2Fe-2S] and three [4Fe-4S] clusters in the sequenceof the $alpha$ subunit and a potential binding site for at least one[4Fe-4S] cluster in the sequence of the $beta$ subunit (Fig. 2 and3). It is possible that not all of the potential binding sitesare actually ligating [Fe-S] centers or that iron and especiallysulfur were not released quantitatively during chemicalanalysis.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The data presented above expand the known diversity of enzymes that may be involved in Fe(III) reduction in dissimilatoryFe(III)-reducing microorganisms. The Fe(III) reductase describedhere represents the first description of a purified soluble Fe(III)reductase from an organism that conserves energy to support growthfrom Fe(III) reduction. As discussed in detail below, the discoveryof significant soluble NADPH-dependent Fe(III) reductase activityin G. sulfurreducens, coupled with the recent report of a similaractivity in the dissimilatory Fe(III)-reducing archaeon Pyrobaculumislandicum (8), suggests that significant soluble Fe(III) reductaseactivity may be found in a wide phylogenetic diversity of dissimilatoryFe(III)-reducingmicroorganisms.

Comparison with other Fe(III) reductases in dissimilatory Fe(III)-reducing microorganisms. The soluble Fe(III) reductase described here is significantly different from the membrane-bound Fe(III) reductases previouslydescribed in dissimilatory Fe(III)-reducing bacteria. Previousstudies on Fe(III) reduction in G. sulfurreducens (16, 33)and the closely related G. metallireducens (17) focused on theNADH-dependent Fe(III) reductase activity, which was localizedprimarily in the membrane fraction (16, 17, 33). A similarmembrane localization of Fe(III) reductase activity has also beennoted in Shewanella species (10, 35). In general, cytochromeshave been considered to be important electron carriers associatedwith these membrane-bound Fe(III) reductase activities (3,12, 16-18, 30, 33, 36). The Fe(III) reductase describedhere not only was recovered in the soluble protein fraction butalso differed from the membrane-bound Fe(III) reductases in theuse of NADPH as the electron donor and the lack of a c-type cytochromein the Fe(III) reductasecomplex.

The soluble NADPH-dependent Fe(III) reductase in G. sulfurreducens has similarities to the Fe(III) reductase activity foundin P. islandicum (8). Although P. islandicum does not containc-type cytochromes (8), it can conserve energy via dissimilatoryFe(III) oxide reduction (22). NADPH was the preferred electrondonor for the reduction of Fe(III) in crude extracts of P. islandicum,and the Fe(III) reductase activity was found in the soluble fraction(8). No membrane-bound Fe(III) reductase activity could bedetected in P. islandicum. Detailed comparisons between the solubleFe(III) reductase in G. sulfurreducens and the one in P. islandicumare not yet possible because the enzyme from P. islandicum hasyet to be purified andcharacterized.

Comparison with known soluble assimilatory Fe(III) reductases. Most previously described soluble Fe(III) reductases have been recovered from aerobic or facultative microorganisms in whichthe Fe(III) reductase is considered to play a role in iron assimilation(5, 20). These enzymes require the addition of exogenousflavins to reduce Fe(III). Since reduced flavins can nonenzymaticallyreduce Fe(III), it has been suggested that these enzymes shouldbe referred to as flavin reductases rather than Fe(III) reductases(14). A recent example of such an enzyme is the soluble Fe(III)reductase from Archaeoglobus fulgidus, which requires exogenousFAD or FMN for activity (48).

The soluble Fe(III) reductase described here did not require the addition of flavin for Fe(III) reductase activity, and theaddition of flavins did not stimulate Fe(III) reduction. The Fe(III)reductase does contain about 1 mol of FAD per mol of enzyme, andanalysis of the gene sequence for the Fe(III) reductase revealedthe presence of two conserved regions that could form a flavinbinding site in the $beta$ subunit of the soluble Fe(III) reductase.This bound flavin is likely to play a role in the transfer ofelectrons toFe(III).

Potential physiological role. The available evidence suggests that the enzyme described here is a redox-active protein with the potential to reduce solubleforms of Fe(III). However, on the basis of the current evidence,it cannot be determined whether this represents the physiologicalfunction of the protein. The specific activity of NADPH-dependentFe(III) reduction in crude extracts is orders of magnitude higherthan that of the NADH-dependent activity described previouslyfor G. sulfurreducens (33). The same also holds true when thespecific activity of the purified soluble Fe(III) reductase iscompared to the enriched NADH-dependent membrane complex (33).This suggests that NADPH-dependent reduction of soluble Fe(III)might be important during dissimilatory reduction of Fe(III).On the other hand, the cytoplasmic location of soluble Fe(III)reductase and the fact that the protein in expressed at the samelevel during growth on fumarate compared to growth on Fe(III)as the electron acceptor may argue against a role of the proteinin dissimilatory Fe(III) reduction. However, a similar situationis found in the dissimilatory Fe(III)-reducing archaeon P. islandicum.This organism readily grows via Fe(III) reduction (22), whileFe(III) reductase activity in cell-free preparations is foundpredominantly in the cytoplasmic fraction (8).

A role of soluble Fe(III) reductase in assimilatory Fe(III) reduction seems doubtful, since G. sulfurreducens grows only underenvironmental conditions in which dissolved Fe(II) is likely tobe abundantly available. Furthermore, it might be expected thatthe synthesis of an assimilatory Fe(III) reductase would be regulatedby the availability of solubleiron.

Sequence analysis did not clarify the physiological function of soluble Fe(III) reductase. Although both subunits of the solubleFe(III) reductase have the highest sequence similarity to thecorresponding subunits of the tungsten- and selenium-containingNADPH-dependent formate dehydrogenase of M. thermoacetica, itis not a formate dehydrogenase. The enzyme did not have formatedehydrogenase activity, formate was not utilized as an electrondonor for the reduction of Fe(III), and the enzyme did not containtungsten or selenium. Furthermore, sequence alignments indicatedthat it lacked the active-site residues conserved in formate dehydrogenases.The amino acid sequence of the $beta$ subunit of soluble Fe(III) reductasewas similar to the $beta$ subunit of glutamate synthase from differentsources. Bacterial glutamate synthase consists of two subunitsand contains FAD, FMN, and three iron-sulfur clusters (49).The $alpha$ subunit is the site of glutamate synthesis, whereas the $beta$ subunit catalyzes the oxidation of NADPH (49). The $alpha$ subunitof soluble Fe(III) reductase had no similarity to the $alpha$ subunitof glutamate synthase, which makes it unlikely that soluble Fe(III)reductase has a function in glutamate synthesis. The similarityof the $beta$ subunit of soluble Fe(III) reductase to the $beta$ subunitof glutamate synthase indicates that this subunit might containthe site for NADPHoxidation.

Another possibility is that the protein is involved in redox reactions not related to the reduction of Fe(III). Studies onthe citric acid cycle in G. metallireducens (7) and G. sulfurreducens(15) demonstrated that the oxidation of 2-oxoglutarate can bemeasured with viologen as the electron acceptor rather than NAD(P)⁺. This suggests that in vivo, a ferredoxin is the electron acceptorfor 2-oxoglutarate dehydrogenase. Ferredoxin is probably reoxidizedby a ferredoxin:NADP⁺ oxidoreductase, and the presence of such an enzyme was postulated(15). The purified soluble Fe(III) reductase possessed highmethyl viologen:NADP⁺ oxidoreductase activity, and it could be hypothesized that theenzyme is involved in transferring electrons from reduced ferredoxinto NADP⁺.

In summary, the NADPH-dependent soluble Fe(III) reductase from G. sulfurreducens is unlike any previously described enzymewith the capacity for Fe(III) reduction. Genetic studies are underway to further evaluate the physiological role of thisenzyme.

	ACKNOWLEDGMENTS

We thank G. R. Voight for technical assistance. We thank A. Siripiny and R. M. Barnes from the Department of Chemistry atthe University of Massachusetts, Amherst, Mass., for performingICP-MS analyses, and we thank M. Coppi for critical reading ofthemanuscript.

Sequencing of the complete genome of G. sulfurreducens was accomplished with support from the Department of Energy. This researchwas funded by the National Science Foundation grant MCB-9727840and the Department of Energy NABIR program grant DE-FG02-97ER62475.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, Morrill Science Center, University of Massachusetts, Amherst,MA 01003. Phone: (413) 545-9651. Fax: (413) 545-1578. E-mail:dlovley{at}microbio.umass.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Altschul, S. F., W. Gish, W. Miller, E. W. Myers, and D. J. Lipman. 1990. Basic local alignment search tool. J. Mol. Biol. 215:403-410[CrossRef][Medline].
2.	Andres-Lacueva, C., F. Mattivi, and D. Tonon. 1998. Determination of riboflavin, flavin mononucleotide and flavin-adenine dinucleotide in wine and other beverages by high-performance liquid chromatography with fluorescence detection. J. Chromatogr. 823:355-363[CrossRef].
3.	Beliaev, A. S., and D. A. Saffarini. 1998. Shewanella putrefaciens mtrB encodes an outer membrane protein required for Fe(III) and Mn(IV) reduction. J. Bacteriol. 180:6292-6297[Abstract/Free Full Text].
4.	Boyington, J. C., V. N. Gladyshev, S. V. Khangulov, T. C. Stadtman, and P. D. Sun. 1997. Crystal structure of formate dehydrogenase H: catalysis involving Mo, molybdopterin, selenocysteine, and an Fe₄S₄ cluster. Science 275:1305-1308[Abstract/Free Full Text].
5.	Braun, V., and H. Killmann. 1999. Bacterial solutions to the iron-supply problem. Trends Biochem. Sci. 24:104-109[CrossRef][Medline].
6.	Caccavo, F., D. J. Lonergan, D. R. Lovley, M. Davis, J. F. Stolz, and M. J. Mclnerney. 1993. Geobacter sulfurreducens sp. nov., a hydrogen- and acetate-oxidizing dissimilatory metal-reducing microorganism. Appl. Environ. Microbiol. 60:3752-3759[Abstract/Free Full Text].
7.	Champine, J. E., B. Underhill, J. M. Johnston, W. W. Lilly, and S. Goodwin. 2000. Electron transfer in the dissimilatory iron-reducing bacterium Geobacter metallireducens. Anaerobe 6:187-196[CrossRef].
8.	Childers, S. E., and D. R. Lovley. 2001. Differences in Fe(III) reduction in the hyperthermophilic archaeon, Pyrobaculum islandicum, versus mesophilic Fe(III)-reducing bacteria. FEMS Microbiol. Lett. 195:253-258[CrossRef][Medline].
9.	Coates, J. D., E. J. Phillips, D. J. Lonergan, H. Jenter, and D. R. Lovley. 1996. Isolation of Geobacter species from diverse sedimentary environments. Appl. Environ. Microbiol. 62:1531-1536[Abstract].
10.	Dobbin, P. S., A. K. Powell, A. G. McEwan, and D. J. Richardson. 1995. The influence of chelating-agents upon the dissimilatory reduction of Fe(III) by Shewanella putrefaciens. Biometals 8:163-173.
11.	Eggink, G., H. Engel, G. Vriend, P. Terpstra, and B. Witholt. 1990. Rubredoxin reductase of Pseudomonas oleovorans. Structural relationship to other flavoprotein oxidoreductases based on one NAD and two FAD fingerprints. J. Mol. Biol. 212:135-142[CrossRef][Medline].
12.	Field, S. J., P. S. Dobbin, M. R. Cheesman, N. J. Watmough, A. J. Thomson, and D. J. Richardson. 2000. Purification and magneto-optical spectroscopic characterization of cytoplasmic membrane and outer membrane c-type cytochromes from Shewanella frigidimarina NCIMB400. J. Biol. Chem. 275:8518-8522.
13.	Fish, W. W. 1988. Rapid colorimetric micromethod for the quantitation of complexed iron in biological samples. Methods Enzymol. 158:357-364[Medline].
14.	Fontecave, M., J. Covès, and J.-L. Pierre. 1994. Ferric reductases or flavin reductases? BioMetals 7:3-8[Medline].
15.	Galushko, A. S., and B. Schink. 2000. Oxidation of acetate through reactions of the citric acid cycle by Geobacter sulfurreducens in pure culture and in syntrophic coculture. Arch. Microbiol. 174:314-321[CrossRef][Medline].
16.	Gaspard, S., F. Vazquez, and C. Holliger. 1998. Localization and solubilization of the iron(III) reductase of Geobacter sulfurreducens. Appl. Environ. Microbiol. 64:3188-3194[Abstract/Free Full Text].
17.	Gorby, Y. A., and D. R. Lovley. 1991. Electron transport in the dissimilatory iron reducer, GS-15. Appl. Environ. Microbiol. 57:867-870[Abstract/Free Full Text].
18.	Gordon, E. H., A. D. Pike, A. E. Hill, P. M. Cuthbertson, S. K. Chapman, and G. A. Reid. 2000. Identification and characterization of a novel cytochrome c₃ from Shewanella frigidimarina that is involved in Fe(III) respiration. Biochem. J. 349:153-158[CrossRef][Medline].
19.	Gosset, G., E. Merino, F. Recillas, G. Oliver, B. Becerril, and F. Bolivar. 1989. Amino acid sequence analysis of the glutamate synthase enzyme from Escherichia coli K-12. Protein Sequences Data Anal. 2:9-16[Medline].
20.	Guerinot, M. L. 1994. Microbial iron transport. Annu. Rev. Microbiol. 48:743-772[CrossRef][Medline].
21.	Hagen, W. R., M. A. Vanoni, K. Rosenbaum, and K. D. Schnackerz. 2000. On the iron-sulfur clusters in the complex redox enzyme dihydropyrimidine dehydrogenase. Eur. J. Biochem. 267:3640-3646[Medline].
22.	Kashefi, K., and D. R. Lovley. 2000. Reduction of Fe(III), Mn(IV), and toxic metals at 100°C by Pyrobaculum islandicum. Appl. Environ. Microbiol. 66:1050-1056[Abstract/Free Full Text].
23.	Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 227:680-685[CrossRef][Medline].
24.	Lloyd, J. R., E. L. Blunt-Harris, and D. R. Lovley. 1999. The periplasmic 9.6-kilodalton c-type cytochrome of Geobacter sulfurreducens is not an electron shuttle to Fe(III). J. Bacteriol. 181:7647-7649[Abstract/Free Full Text].
25.	Lonergan, D. J., H. L. Jenter, J. D. Coates, E. J. Phillips, T. M. Schmidt, and D. R. Lovley. 1996. Phylogenetic analysis of dissimilatory Fe(III)-reducing bacteria. J. Bacteriol. 178:2402-2408[Abstract/Free Full Text].
26.	Lovley, D. R. 2000. Fe(III) and Mn(IV) reduction, p. 3-30. In D. R. Lovley (ed.), Environmental microbe-metal interactions. ASM Press, Washington, D.C.
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