Interaction of Bacillus subtilis Fur (Ferric Uptake Repressor) with the dhb Operator In Vitro and In Vivo

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Journal of Bacteriology, July 1999, p. 4299-4307, Vol. 181, No. 14
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Interaction of Bacillus subtilis Fur (Ferric Uptake Repressor) with the dhb Operator In Vitro and In Vivo

Nada Bsat and John D. Helmann^*

Section of Microbiology, Cornell University, Ithaca, New York 14853-8101

Received 12 March 1999/Accepted 29 April 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Bacillus subtilis contains three metalloregulatory proteins belonging to the ferric uptake repressor (Fur) family: Fur, Zur,and PerR. We have overproduced and purified Fur protein and analyzedits interaction with the operator region controlling the expressionof the dihydroxybenzoate siderophore biosynthesis (dhb) operon.The purified protein binds with high affinity and selectivityto the dhb regulatory region. DNA binding does not require addediron, nor is binding reduced by dialysis of Fur against EDTA ortreatment with Chelex. Fur selectively inhibits transcriptionfrom the dhb promoter by $sigma$ ^A RNA polymerase, even if Fur is added after RNA polymerase holoenzyme.Since neither DNA binding nor inhibition of transcription requiresthe addition of ferrous ion in vitro, the mechanism by which ironregulates Fur function in vivo is not obvious. Mutagenesis ofthe fur gene reveals that in vivo repression of the dhb operonby iron requires His97, a residue thought to be involved in ironsensing in other Fur homologs. Moreover, we identify His96 asa second likely iron ligand, since a His96Ala mutant mediatesrepression at 50 µM but not at 5 µM iron. Our data lead us tosuggest that Fur is able to bind DNA independently of bound ironand that the in vivo role of iron is to counteract the effectof an inhibitory factor, perhaps another metal ion, that antagonizesthis DNA-bindingactivity.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Iron is an essential and often growth-limiting nutrient for microorganisms. The rapid oxidation of ferrous to ferric iron,which is virtually insoluble at a nearly neutral pH, reduces thelevel of bioavailable iron far below the approximately 1 µM thatmost organisms require for optimal growth (4, 18, 28, 29).Consequently, many bacteria synthesize and excrete high-affinityiron chelators (siderophores) that can solubilize ferric ironand subsequently be imported by a corresponding ferri-siderophoreuptake system (29). The expression of genes for siderophorebiosynthesis and transport is repressed by added iron. In manybacteria, this repression is mediated by a metal-sensing DNA-bindingprotein, the ferric uptake repressor (Fur) protein (22, 23).

Fur has been best characterized from Escherichia coli (designated Fur_EC), but homologs have been identified in numerous otherbacteria (22, 23). In vivo, Fur_EC represses a large regulonof iron uptake functions when iron is present in excess (6).Most other metals are ineffective at eliciting repression in vivo,although Mn(II) leads to the repression of some, but not all,Fur-regulated genes (3, 5, 21, 32). In many gram-negativebacteria, selection for manganese-resistant (Mn^r) mutants leads to mutations in fur, suggesting that the abilityof Mn(II) to activate Fur for DNA binding may be a source of manganesetoxicity, perhaps by inappropriately repressing iron uptake functions(21).

Fur_EC is an ~16-kDa dimeric protein with an amino-terminal DNA recognition domain and a carboxyl-terminal metal-binding domain(12, 37). In vitro studies have demonstrated that Fur_EC bindsto a specific DNA target site, the fur box, and that this bindingrequires a divalent metal ion as a cofactor (3, 14). In thevast majority of studies, Mn(II) is used to activate Fur, sincethis ion, unlike Fe(II), is stable in the presence of oxygen.It is generally assumed that Mn(II)-Fur is functionally analogousto the Fe(II) form thought to mediate repression in vivo. However,the metal-binding sites of Fur are not yet well characterized.Fur binds two divalent ions per monomer, and binding is thoughtto involve a cluster of conserved histidine residues and two pairsof cysteines in the carboxyl-terminal metal-binding domain (12,24). One site is apparently occupied by a tightly associated(structural) zinc ion, while the second site is thought to bindFe(II) reversibly to regulate DNA binding (24).

Bacillus subtilis contains three Fur homologs (8, 17) that regulate a peroxide stress response (PerR), zinc uptake (Zur),and iron uptake (Fur). Fur regulates the expression of severaloperons implicated in iron transport (8, 23), including thedihydroxybenzoate siderophore biosynthesis (dhb) operon. Transcriptionof the dhb operon is initiated from a single $sigma$ ^A-dependent promoter with an overlapping consensus fur box (33).Mutations in this fur box or in fur prevent the iron-mediatedrepression of dhb (8, 33). However, unlike its homologs fromgram-negative organisms, B. subtilis Fur does not recognize Mn(II)as a corepressor in vivo, and selection for Mn^r does not generate fur mutants (8, 9).

We have overproduced and purified B. subtilis Fur and initiated a study of its interactions with both DNA and metal ions.Surprisingly, Fur is purified in an active zinc-containing formthat does not require the addition of Fe(II) to bind DNA or torepress transcription. Nevertheless, genetic studies are consistentwith a model in which iron does interact directly with Fur invivo.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains, plasmids, and oligonucleotide primers. The strains, plasmids, and oligonucleotide primers used in this study are listed in Table 1. E. coli DH5 $alpha$ was used for routinecloning experiments, while RK4353 (RecA⁺) was used to generate multimeric plasmids for efficient Campbellintegration into the B. subtilis genome. To overproduce Fur, thegene was amplified by PCR with primers 75 and 76. These primersintroduce NdeI and KpnI sites on the PCR product ends; these sitesare then used for cloning into NdeI-KpnI-cut pET17b (Novagen),generating pHB6505. The synthetic oligonucleotide primers usedwere obtained from the DNA Services Facility of the Cornell NewYork State Center for Advanced Technology-Biotechnology.

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TABLE 1. Strains, plasmids, and oligonucleotide primers used in this study

Reagents, media, and growth conditions. Chemicals and antibiotics were purchased from Sigma Chemical Co. (St. Louis, Mo.) unless otherwise indicated. CuSO₄ (99.999%),FeSO₄ (99.999%), FeCl₃ (at least 99.99%), MnCl₂ (99.999%), NiSO₄(99.999%), and ZnSO₄ (99.999%) were obtained from Aldrich ChemicalCo. (Milwaukee, Wis.). Radioactive isotopes were purchased fromDuPont, NEN Research Products (Boston, Mass.). Manganese- andiron-limited minimal media (MM) were prepared as previously described(7). Ampicillin (100 µg/ml) was used for the selection of E.coli strains. Erythromycin (1 µg/ml) and lincomycin (25 µg/ml)(for testing macrolide-lincosamide-streptogramin B resistance),kanamycin (10 µg/ml), spectinomycin (100 µg/ml), and chloramphenicol(5 µg/ml) were used for the selection of B. subtilisstrains.

DNA manipulations and sequencing. Routine molecular biology procedures and DNA manipulations were carried out as described previously (34). B. subtilis transformationwas done by standard procedures (13). E. coli plasmid DNA andDNA fragments were isolated with QIAprep Spin Miniprep and PCRpurification and gel extraction kits, respectively (Qiagen Inc.,Chatsworth, Calif.). Restriction endonucleases, DNA ligase, VentDNA polymerase, T4 polynucleotide kinase, and calf intestinalalkaline phosphatase (New England Biolabs, Beverly, Mass.), Sequenase(Amersham Life Science Inc.), Pfu DNA polymerase (Stratagene,La Jolla, Calif.), and RNasin RNase inhibitor (Promega Corporation,Madison, Wis.) were used according to manufacturers' instructions.DNA sequencing was performed on both strands for new constructswith AmpliTaq-FS DNA polymerase and dye terminator chemistry atthe DNA Services Facility of the Cornell New York State Centerfor Advanced Technology-Biotechnology.

Overproduction and purification of Fur. Wild-type Fur was purified with E. coli BL21(DE3)/pLysE (39) containing pHB6505, a pET17b derivative. A 1-liter culturewas grown from a fresh transformant at 37°C in Luria broth containing0.4% glucose to enhance plasmid stability. At an optical densityat 600 nm (OD₆₀₀) of 0.4, isopropyl- $beta$ -D-thiogalactopyranoside(IPTG; Amersham Life Science) was added to 1 mM, and growth wascontinued for 1 h. Rifampin was added to 100 µg/ml, incubationwas continued for 2 h, and the cells were harvested. Cell pelletswere suspended in 20 ml of disruption buffer (50 mM Tris-HCl [pH8], 2 mM EDTA, 0.1 mM dithiothreitol [DTT], 1 mM 2-mercaptoethanol,100 mM NaCl, 10% [vol/vol] glycerol, 1 mM phenylmethylsulfonylfluoride [PMSF], 5% [vol/vol] bacterial protease inhibitor cocktail[Sigma P8465]) containing 130 µg of hen egg white lysozyme/ml,and the suspension was incubated on ice for 10 min. Sodium deoxycholatewas added to 0.05% (wt/vol), and the cell suspension was disruptedby pulsed sonication for 2 min. Lysates were diluted with 20 mlof TEDG buffer (10 mM Tris-HCl [pH 8], 0.1 mM EDTA, 0.1 mM DTT,5% [vol/vol] glycerol, 1 mM PMSF) and clarified twice by centrifugationfor 15 min each time. The resulting supernatant was applied at4°C to a heparin-Sepharose CL-6B column (Pharmacia LKB, Piscataway,N.J.), and Fur was eluted with a linear gradient of 0.05 to 1M NaCl in TEDG buffer (it elutes near 350 mM NaCl). Fractionscontaining Fur were pooled, precipitated with ammonium sulfate(65% saturation), suspended in TEDG buffer, and applied to a Mono-Q(HR5/5) column for Pharmacia fast protein liquid chromatography.Fur was eluted with 350 mM NaCl, concentrated by ammonium sulfateprecipitation, and resuspended in TEDG buffer containing 300 mMNaCl and 1 mM DTT. Fur was further purified by fast protein liquidchromatography on a Superdex-75 column with the same buffer. Asjudged against molecular mass standards, Fur elutes with an apparentmolecular mass of 35 kDa, as predicted for a dimer. Fur was >98%pure, as judged by sodium dodecyl sulfate (SDS)-polyacrylamidegel electrophoresis (PAGE). The glycerol concentration was adjustedto 50% (vol/vol), and Fur was stored in aliquots at $-$ 20°C. TheFur protein concentration was determined with the Bio-Rad Laboratories(Hercules, Calif.) dye-binding (Bradford) assay and refers inall cases to the dimericprotein.

The percentage of purified Fur active for DNA binding can be estimated from the transcription repression experiments. In thesestudies, between 16 and 32 nM Fur was required to completely represstranscription from a 4 nM DNA template. Since these experimentsare performed at concentrations of Fur well above the measureddissociation constant, we can estimate the fraction of activeFur as being between 0.12 and 0.25 (assuming that the bindingof a single dimer is sufficient for repression). All Fur concentrationsreported in this study are total protein rather than activemolecules.

To estimate the metal content of Fur, Fur was dialyzed at 4°C three times against TG buffer (5 mM Tris-HCl [pH 8], 10% [vol/vol]glycerol, 1 mM PMSF) and analyzed by flame atomic absorption spectroscopyat the ICP Analytical Laboratory of the Cornell Department ofFruit and Vegetable Science. Iron, zinc, and nickel atomic absorptionstandard solutions were purchased fromSigma.

Treatment of Fur with chelators. Two strategies were used to remove loosely associated metals from Fur. In one protocol, Fur was dialyzed at 4°C against TEDGbuffer containing 25 mM EDTA and 300 mM NaCl and then dialyzedagainst TEDG buffer containing 1 mM DTT and 300 mM NaCl to reducethe concentration of EDTA. The glycerol concentration was adjustedto 50% (vol/vol) and Fur was stored in aliquots at $-$ 20°C. In theother protocol, Fur was preincubated with 5% (wt/vol) Chelex 100(Bio-Rad) in electrophoretic mobility shift assay (EMSA) buffer(see below) on ice for 1 h with frequent mixing. The resin wasallowed to settle, and the Fur-containing supernatant was removedand used inEMSA.

EMSAs with the dhb promoter. A DNA fragment containing the promoter, fur box, and partial coding sequence (to codon 53) of dhbA was generated by PCR withprimers 200 and 201, which incorporate HindIII and BamHI sites,respectively. The 400-bp product was cleaved with AlwNI, generatinga 280-bp fragment (containing the promoter and fur box) and a120-bp downstream fragment. DNA was end labeled with T4 polynucleotidekinase. Fur was equilibrated in EMSA buffer (20 mM Tris-HCl [pH8], 50 mM KCl, 5% [vol/vol] glycerol, 0.5 mM DTT, 0.1 mg of bovineserum albumin per ml) for 10 min at room temperature (RT), 50pM (1 fmol) of end-labeled DNA and 5 µg of competitor salmon testisDNA per ml were added, and incubation was continued for 10 minat RT. The reactions were analyzed next to a dye marker on a 4%nondenaturing gel (40 mM Tris-acetate) that was prerun for 10min in Tris-acetate buffer containing 0.5 mM DTT. After 2 h at150 V, the gel was dried and exposed to a PhosphorImager screenfor analysis (STORM; Molecular Dynamics, Inc.). The data pointswere fit, by use of the DeltaGraph Professional reiterative curve-fittingalgorithm, to an equation of the following form: percent DNA boundequals 100{1/[1 + (K/[Fur])ⁿ]}. In this equation, K represents the apparent dissociation constantfor Fur binding, [Fur] is the concentration of dimeric Fur protein,and n is the cooperativity coefficient. Both K and n were independentlyoptimized. Competition experiments were done with either the samedhb fragment or a PCR product containing the fur coding regionas a nonspecificcontrol.

In vitro transcription of the dhb promoter fragment. The dhb-containing template and the vector control for in vitro transcription assays were generated by linearizing pHB6548and pJPM122, respectively, with BamHI. B. subtilis core RNA polymeraseand $sigma$ ^A preparations were described previously (25, 26). RNA polymeraseholoenzyme (RNAP) was reconstituted by incubating the core with $sigma$ ^A (1:5 molar ratio) on ice for 15 min prior to use. The DNA template(4 nM) was preincubated with RNAP (80 nM, unless otherwise indicated)in transcription buffer (20 mM Tris-HCl [pH 8], 50 mM KCl, 5%[vol/vol] glycerol, 0.5 mM DTT, 0.1 mg of bovine serum albuminper ml, 10 mM MgCl₂, 10 U of RNasin RNase inhibitor per reaction)for 10 min at 37°C. To assay transcriptional repression, Fur orRNAP was preincubated with DNA for 5 min at RT or 37°C, respectively,prior to the addition of the other protein. When appropriate,10 µM freshly dissolved FeSO₄ was added. Transcription was initiatedby the addition of a nucleotide mixture (400 µM each ATP, GTP,and CTP and 60 µM [ $alpha$ -³²P]UTP; ~3,000 cpm/pmol), and reaction mixtures were incubatedfor 8 min at 37°C. The reactions were stopped with 100 µl of stopsolution (2.5 M ammonium acetate, 20 mM EDTA [pH 8], 0.2 mg ofglycogen per ml), and nucleic acids were recovered by phenol extractionand ethanol precipitation prior to resuspension in 10 µl of formamidegel loading buffer (80% formamide, 10 mM EDTA [pH 8], 1 mg ofxylene cyanol FF per ml, 1 mg of bromphenol blue per ml). Thesamples were denatured for 4 min at 90°C and loaded on a 6% denaturingpolyacrylamide gel. The gel was dried and exposed to a STORM PhosphorImagerscreen foranalysis.

Siderophore assays. B. subtilis cultures were grown overnight at 37°C in MM with or without added FeCl₃ (5 µM). Siderophore levels were determinedwith the Arnow assay as previously described (2, 9). Siderophoreyields were normalized to the cell mass by dividing the measuredsiderophore level (OD₅₁₀) by the culture density (OD₆₀₀). Allassays were performed with duplicate samples, and the values wereaveraged.

PCR. The PCR mixture contained HB1000 chromosomal DNA, 50 µM each deoxynucleoside triphosphate, 100 pmol each of the forward andreverse primers, and 2 U of Vent DNA polymerase (or 1.25 U ofPfu DNA polymerase) in a total volume of 100 µl. The reactionmixtures were denatured for 2 min at 94°C, followed by 30 cyclesof 10 s at 95°C, 30 s at 50°C (or 55°C, depending on the primersused), and 30 s at 72°C and a final extension of 5 min at 72°C.

Megaprimer site-directed mutagenesis and complementation analysis. The fur-containing 810-bp DNA fragment (100 bp upstream of the fur transcription start site to 220 bp downstream of the furtranslation stop codon) was amplified from HB1000 chromosomalDNA with primers 140 and 139 by PCR as described above with thefollowing modifications: cloned Pfu polymerase and Pfu bufferwere used instead of Vent polymerase, the annealing temperaturewas 47°C, and the extension time was 1 min. The resulting productwas cloned into pGEM-cat as a HindIII-BamHI fragment (pHB6524),sequenced, and then subcloned from pHB6524 into pDG1662 to generatepHB6525. For fur complementation analysis, pHB6525 was transformedinto HB6637, and double-crossover recombinants were selected withchloramphenicol and screened for Spc^s and macrolide-lincosamide-streptogramin B sensitivity, ensuringintegration at amyE. The resulting strain (HB6640) was testedby siderophore assays for complementation of fur::kan. With pHB6524as a template, the various histidine and cysteine mutants weregenerated by megaprimer PCR mutagenesis as described previously(35) with a few modifications. Briefly, pHB6524 was cut withHindIII and PCR amplified with the appropriate mutagenic primer(147 to 155) and primer 139 at an annealing temperature of 50°C.To enrich for the megaprimer DNA strand, the first PCR productwas used as a template in a subsequent asymmetric PCR with 10-foldless of the mutagenic primer than of primer 139. The asymmetricPCR product was used with primer 140 and BamHI-cut pHB6524 asa template in a third PCR at an annealing temperature of 48°C.The final product was purified, cloned into pGEM-cat as an 810-bpHindIII-BamHI fragment (pHB6527 to pHB6534 and pHB6537), sequenced,and then subcloned into pDG1662 (pHB6538 to pHB6545 and pHB6547).The pDG1662-derived plasmids were then integrated into HB6637(fur null mutant) and HB6634 (fur wild type) (HB6650 to HB6663,HB6668, HB6670, HB6672, and HB6673) to study complementation andrecessiveness to wild-type Fur,respectively.

Immunoprecipitation of Fur from ³⁵S-Met-labeled cells. Cells were grown to the late logarithmic phase in MM without iron supplementation. Aliquots (1.6 ml) were labeled with L-[³⁵S]methionine (20 µCi; 1,175 Ci/mmol) for 45 min, chased with nonradioactivemethionine (2.5 mM), cooled on ice, and centrifuged. Cell pelletswere washed with 0.8 ml of glucose buffer (50 mM glucose, 25 mMTris-HCl [pH 8]), resuspended in 100 µl of lysis buffer (glucosebuffer with 0.1 mg of lysozyme per ml), and incubated on ice for10 min. One hundred microliters of detergent solution (2% NonidetP-40, 1% sodium deoxycholate) was added, and the samples werevortexed and incubated for 10 min at 37°C. After centrifugation,the supernatant was preadsorbed to 50 µl of protein G-agarosesuspension (Boehringer Mannheim Biochemicals, Indianapolis, Ind.)for 3 h. After centrifugation for 20 s, the supernatant was incubatedwith polyclonal rabbit anti-Fur_EC antibodies for 1 h, 50 µl ofprotein G-agarose was added, and incubation was continued overnight.The pellets were washed in the buffers recommended by the manufacturer(Boehringer). All of the previous incubations were performed at4°C on a rocking platform, unless otherwise indicated. The pelletswere resuspended in 50 µl of gel loading buffer, boiled for 5min, and centrifuged, and the immunoprecipitated proteins in thesupernatant were separated by SDS-12% PAGE. The gel was driedand exposed to a PhosphorImager screen foranalysis.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Overproduction, purification, and physical characterization of Fur. The fur gene was cloned into pET17b, and Fur was overproduced in E. coli BL21(DE3)/pLysE (39). Since the fur gene was toxicfor E. coli, it was necessary to use pLysE to stabilize the pETtransformants (38). The overproduced Fur was almost equallydistributed between inclusion bodies and the extract supernatantand was purified to homogeneity from the supernatant. Purificationwas achieved by chromatography on heparin-Sepharose, Mono-Q, andSuperdex-75. Fur elutes from the Superdex-75 column with an apparentmolecular mass of 35 kDa, in agreement with its calculated dimericmass, and with the dimeric state of Fur_EC in solution (4, 12).From promoter titration experiments (see Materials and Methodsand below), we estimate that between 12 and 25% of the isolatedFur is active for DNAbinding.

As purified, Fur migrates on SDS-polyacrylamide gels as a doublet, with the predominant and larger product (A) correspondingto the expected molecular mass of 17.4 kDa (Fig. 1). The identitiesof the purified proteins (A and B, separately) were confirmedby amino-terminal sequencing of the first 10 amino acid residues,which matched the predicted Fur sequence (8). Unlike Fur_EC(40), B. subtilis Fur retains its N-terminal methionine. Thefaster-migrating band (B) could be either an isoform of Fur withaltered mobility or a degradation product. This band was observedconsistently despite the addition of a cocktail of protease inhibitorsduring cell lysis. Since the two isoforms persist even after reductionwith freshly prepared $beta$ -mercaptoethanol or DTT, it is unlikelythat there is an intramolecular disulfide bond. Therefore, wetentatively conclude that the smaller band is truncated at itsC terminus. A protease-sensitive region has also been observedin the C-terminal region of Fur_EC mutants altered in either oftwo conserved cysteines (11). Preliminary atomic absorptionspectroscopy indicates that zinc but neither iron nor manganesecopurifies with Fur (calculated molar ratio of Zn to Fur of between2 and 3).

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FIG. 1. Purification of Fur and SDS-12% PAGE analysis of fractions from the purification of Fur. Lanes: M, molecular mass standards; 1 and 2, total proteins from uninduced and IPTG-induced BL21(DE3)/pLysE/pHB6505, respectively; 3, pooled fractions from heparin-Sepharose; 4, pooled fractions from Mono-Q; 5, fraction from Superdex-75. Fur runs just below the 21.5-kDa marker, and the Fur doublet is indicated by A and B on the right.

Fur binds specifically to the dhb promoter region. Purified Fur was assayed for DNA binding in EMSAs with a 400-bp fur box-containing dhb promoter fragment cleaved with AlwNIto generate a 280-bp fur box-containing fragment and a 120-bpcontrol fragment (Fig. 2). When incubated with the dhb promoterfragment, 10 nM Fur caused an electrophoretic mobility shift ofthe larger, fur box-containing fragment but not the fragment lackinga fur box (Fig. 3A, lane 2). The specificity of the interactionof Fur with the dhb promoter fragment was tested in competitionassays with either the same dhb DNA fragment or an unrelated DNAfragment generated by PCR. Fur at 10 nM was first incubated with50 pM end-labeled dhb fragment before the addition of 10 or 100nM cold competitor DNA, and incubation was continued for another10 min at RT (Fig. 3B). While the dhb promoter region efficientlycompeted for binding, the nonspecific DNA did not compete, evenwhen present in a 10-fold molar excess (100 nM) over Fur. Thisresult demonstrates that Fur specifically interacts with the dhbfur box-containing promoter element. The inability of 10 nM Furto efficiently shift labeled DNA in the presence of 10 nM dhbcompetitor is consistent with our estimation of the fraction ofactive Fur as being between 12 and 25%.

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FIG. 2. dhb promoter-operator region. The $-$ 35 and $-$ 10 regions of the dhb $sigma$ ^A-dependent promoter (33) are indicated by underlining. The fur box required for iron-mediated repression of dhb transcription (33) is indicated by double underlining, and the start codon (ATG) for dhbA is shown in uppercase letters. The fragment used in the EMSA experiments extends from ~90 bp upstream of the $-$ 35 element (as indicated) to the right bracket. The AlwNI site used to bisect the dhb fragment for EMSA experiments is indicated.

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FIG. 3. Specific binding of Fur to the dhb regulatory region. (A) The dhb promoter fragment (50 pM) was cut with AlwNI, end labeled, and incubated with native or EDTA-treated Fur. Lanes: 1, no Fur; 2, 10 nM Fur; 3, 10 nM EDTA-treated Fur. The positions of the unbound fur box and the shifted complex are indicated by unbound and bound, respectively. (B) The dhb promoter fragment (50 pM) was incubated with Fur for 10 min prior to the addition of cold competitor DNA. Lanes: 1, no Fur; 2, 10 nM Fur; 3, 10 nM Fur and 10 nM dhb competitor DNA; 4, 10 nM Fur and 100 nM dhb competitor DNA; 5, 10 nM Fur and 10 nM nonspecific competitor DNA; 6, 10 nM Fur and 100 nM nonspecific competitor DNA. The shifted complex is displaced only by the addition of the specific dhb competitor DNA.

Effects of Fe(II) on the binding of Fur to the dhb promoter region. DNA binding by Fur is thought to require an activating metal ion. We attempted to remove loosely associated metal ions fromFur by dialysis against buffer containing 25 mM EDTA followedby dialysis against buffer lacking EDTA. Surprisingly, the EDTA-treatedFur was just as active as the native Fur in EMSAs (Fig. 3A, lane3). Similarly, treatment of Fur with Chelex did not inhibit DNAbinding (data not shown). Thus, purified Fur binds to the dhbpromoter fragment in the absence of any added metal ions, andany copurifying metal ions required for binding (e.g., zinc) appearto be tightly associated and not easily removed by chelatingagents.

B. subtilis Fur represses dhb expression in vivo in response to iron (8, 33). However, as purified, Fur is able to bindto DNA specifically in the absence of added iron. To clarify thediscrepancy between the in vitro and in vivo data, we wished todetermine if Fe(II) increases the affinity of Fur for the dhbpromoter fragment. EMSAs were conducted over a range of Fur concentrations(0.06 to 128 nM) in the presence and absence of added ferrousion (Fig. 4). In the absence of added iron, the best-fit bindingcurve corresponded to a K_d (apparent) of 4.6 nM (correspondingto a K_d of ~0.8 nM when corrected for active protein) and a cooperativitycoefficient of 2, perhaps indicating oligomerization of Fur concomitantwith DNA binding. In the presence of added iron, the calculatedaffinity of Fur for DNA was enhanced twofold (apparent K_d, 2.3nM) and cooperativity was slightly increased (cooperativity coefficient,~3). These results suggest that Fe(II) does increase, albeit onlymodestly, the interaction of Fur with the fur box-containing fragment.

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FIG. 4. Effect of added Fe(II) on the affinity of Fur for the dhb promoter region. A curve for the binding of Fur to the dhb promoter fragment in the presence and absence of Fe(II) is shown. Fur (0.5, 1, 2, 4, 8, 16, and 32 nM) in the presence of Fe(II) (

) and Fur (0.06, 0.125, 0.25, 0.5, 1, 2, 4, 8, 16, 32, 64, and 128 nM) in the absence of Fe(II) (

) were incubated with 50 pM end-labeled template and separated by nondenaturing PAGE, and the percentages of bound and unbound DNA were determined by PhosphorImager analysis with the program ImageQuant (Molecular Dynamics, Inc.).

Repression of dhb transcription by Fur in vitro. Despite the lack of a dramatic effect on DNA-binding affinity, we hypothesized that Fe(II) might nevertheless stabilize aconformation of Fur necessary for efficient transcriptional repression.To test this idea, purified B. subtilis $sigma$ ^A holoenzyme was used to transcribe a linearized plasmid DNA templateto produce a 268-bp runoff dhb transcript together with a smaller,vector-derived transcript that serves as a control for nonspecificeffects of Fur (Fig. 5A, lane 2). As expected, when the vectoralone was used as a template, the larger, dhb transcript was notobserved (Fig. 5A, lane 1). Fur (4 to 80 nM) was preincubatedwith the dhb template (4 nM) prior to the addition of 80 nM RNAP.Repression of the dhb transcript was evident at 16 nM Fur andwas complete at 32 nM Fur. Fur did not repress the vector-derivedtranscript at any of the concentrations tested. Thus, Fur specificallyrepresses dhb transcription.

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FIG. 5. Fur specifically represses dhb transcription. (A) Addition of Fur before RNAP. The linearized vector (lanes 1 and 3) or the dhb-containing template DNA (lanes 2, 4, 5, 6, 7, 8, and 9) (4 nM) was incubated with 80 nM RNAP for 10 min at 37°C (lanes 1 and 2) or with Fur for 5 min at RT prior to the addition of 80 nM RNAP and incubation for another 5 min at 37°C (lanes 3 to 9). Lanes: 1 and 2, no Fur; 3 and 4, 80 nM Fur; 5, 64 nM Fur; 6, 32 nM Fur; 7, 16 nM Fur; 8, 8 nM Fur; 9, 4 nM Fur. The positions of the dhb transcript and the vector transcript are indicated on the right. (B) Addition of Fur after RNAP. The linearized vector (lane 1) or the dhb-containing template DNA (lanes 2 to 10) (4 nM) was incubated with 80 nM RNAP for 10 min at 37°C (lanes 1 and 2) or preincubated with 80 nM RNAP for 5 min at 37°C prior to the addition of Fur alone (lanes 3, 5, 7, and 9) or Fur and Fe(II) (lanes 4, 6, 8, and 10) and incubation for another 5 min at RT. Lanes: 1 and 2, no Fur; 3, 4 nM Fur; 4, 4 nM Fur and 10 µM Fe(II); 5, 16 nM Fur; 6, 16 nM Fur and 10 µM Fe(II); 7, 64 nM Fur; 8, 64 nM Fur and 10 µM Fe(II); 9, 256 nM Fur; 10, 256 nM Fur and 10 µM Fe(II). The positions of the dhb transcript and the vector transcript are indicated on the right.

To determine if Fe(II) affects the ability of Fur to repress transcription, we measured transcriptional repression in thepresence and absence of freshly prepared 10 µM Fe(II). In thesestudies, we altered the order of addition such that the DNA templatewas preincubated first with RNAP and then with Fur for 5 min priorto initiation of the transcription reactions. Once again, 16 nMFur led to significant repression, which was complete at 32 nMFur (Fig. 5B). The addition of Fe(II) did not affect the abilityof Fur to repress the transcription of dhb. However, there wassome repression of the vector-derived transcript at the highestFur concentration tested (256 nM), and this effect did requireiron.

Repression of dhb transcription by Fur in vivo: role of conserved histidine and cysteine residues in repression. While iron is required for the in vivo repression of siderophore biosynthesis, our in vitro studies indicate that Fe(II) additionis not required for the specific binding and repression of dhbtranscription. In contrast, in other studies of Fur_EC, the additionof divalent cations is typically required to observe DNA binding(3, 14, 22). Unfortunately, little is known about the actualmechanism of iron sensing by Fur proteins, although it is thoughtthat binding involves a subset of the conserved histidine andcysteine residues in the carboxyl-terminaldomain.

We used site-directed mutagenesis of the fur gene to individually alter nine cysteine and histidine residues to alanine. Weinserted the wild-type and mutant fur genes in single copies atamyE and tested for complementation of a fur null mutant (Fig.6). As an indirect measure of the transcriptional activity ofthe dhb locus, we monitored the levels of siderophores (dihydroxybenzoicacid and dihydroxybenzoyl serine) present in cell supernatantsafter growth in the presence of various concentrations of iron.In this assay, the H93A-, H95A-, and H132A-expressing strainsall displayed a pattern of iron-mediated repression not significantlydifferent from that of the wild type. In contrast, the strainsexpressing mutant Fur proteins altered in any of the four Cysresidues were completely derepressed for dhb expression, similarto the fur null mutant. The H96A and H97A Fur mutants appearedto have altered function. While the H97A mutant protein displayedvery little iron responsiveness, it did not yield a completelyderepressed null phenotype. The H96A mutant protein had the mostinteresting phenotype: it displayed a level of basal activitysimilar to that of the wild type and mediated full repressionof dhb at 50 µM but not 5 µM added iron.

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FIG. 6. Complementation of fur::kan by the various histidine-to-alanine and cysteine-to-alanine fur mutations. The mutations were inserted at amyE in HB6637 (fur::kan) by a double recombination event, the strains were grown in MM in the absence (dark gray bar) or presence of 5 µM Fe(III) (hatched bar) or 50 µM Fe(III) (light gray bar), and catechol siderophore yields were expressed as OD₅₁₀/OD₆₀₀ ± standard deviations. WT, wild type.

To determine whether the null phenotypes observed for some of the mutants (Fig. 6) were due to instability of the mutant proteins,we labeled the various B. subtilis mutant strains with L-[³⁵S]methionine, immunoprecipitated Fur from whole-cell extractsby using polyclonal antibodies against Fur_EC, and analyzed theprecipitates by SDS-PAGE (Fig. 7). These antibodies cross-reactwith purified B. subtilis Fur in dot blot assays (data not shown)and allow visualization of a protein with the expected size forFur (17.4 kDa) in the wild-type strain but not in a fur mutantstrain. In addition to full-length Fur, a smaller protein is alsodetected. This is likely to be a degradation product of Fur, sinceit is missing from the fur mutant strain.

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FIG. 7. Fur is destabilized by all four cysteine mutations and two of the histidine mutations. Pulse-labeled fur mutants were lysed, and Fur was immunoprecipitated from the extracts with polyclonal antibodies against E. coli Fur and protein-G agarose beads. The immunoprecipitated proteins in the supernatant were separated by SDS-12% PAGE, and the gel was analyzed by PhosphorImager analysis. Arrows show full-length Fur (upper band) and a Fur degradation product (lower band). WT, wild type.

The immunoprecipitation experiment revealed nearly wild-type levels of Fur in the strains expressing the H95A, H96A, and H97Aproteins. The presence of essentially wild-type levels of H96AFur and H97A Fur is significant, since these proteins had alteredresponses to iron in vivo. The H93A and H132A proteins were presentat very low levels in this assay, despite their nearly normalbiological activity. We do not know whether the reduced levelsof these proteins resulted from instability in vivo or duringthe immunoprecipitation procedure. The lack of signal for thefour Cys mutant proteins suggests that these proteins may failto accumulate in vivo, consistent with their null phenotypes,with the stability defects of two Fur_EC Cys mutant proteins (11),and with the finding that these mutant proteins are unstable whenoverproduced in E. coli (data not shown). Although it seems unlikely,we cannot yet rule out the possibility that one or more of thesemutations may affect the ability of these antisera to recognizeFur.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We report the purification and initial characterization of the DNA- and metal-binding properties of B. subtilis Fur, the firstmember of the Fur family to be biochemically characterized froma gram-positiveorganism.

In vitro repression of the dhb promoter. B. subtilis Fur acts as an iron-dependent repressor of the dhb operon in vivo (8, 33). However, in vitro Fe(II) failedto significantly affect either the affinity of Fur for the dhboperator (Fig. 4) or the ability of Fur to repress transcription(Fig. 5). We conclude that in vitro Fur is an iron-independentrepressor of dhb transcription. Interestingly, Fur efficientlyrepresses transcription even if RNAP is incubated with the dhbpromoter region prior to the addition of Fur. This finding suggestseither that Fur can bind to the promoter region downstream ofprebound RNAP or that Fur can displace RNAP. Further studies areneeded to distinguish between these possibilities. For comparison,in vitro studies have demonstrated that neither Fur_EC nor E. coliRNAP can displace the other (15, 16).

Interactions of Fur with metal ions. Fur_EC is the prototype for a large family of metal-dependent repressors (22), including three functionally distinct B. subtilishomologs (8, 17). It is generally accepted that Fur bindsto Fe(II) in vivo and is thereby activated to bind DNA, leadingto the repression of iron uptake functions. However, the interactionof Fur with metal ions is not wellunderstood.

The most unexpected finding from this work is the lack of a requirement for added iron for either DNA binding or transcriptionalrepression in vitro. As purified, B. subtilis Fur contains zinc,as reported for Fur_EC (24), but little or no iron. Moreover,DNA binding is insensitive to treatment of Fur with chelatingagents, including dialysis against EDTA or incubation with Chelex,and is not appreciably enhanced by the addition of Fe(II). Thus,if metal ions are required to activate Fur for DNA binding, theyappear to be tightly bound under our purificationconditions.

Fur_EC binds at least two metal ions per monomer in a carboxyl-terminal metal-binding domain that contains several conservedhistidine and cysteine residues (11, 12, 24). Fur_EC hasrecently been found to be a zinc metalloprotein (24) with atightly associated zinc ion thought to play a structural role.This ion is coordinated with two sulfur ligands, perhaps Cys92and Cys95 (equivalent to Cys100 and Cys103 in B. subtilis Fur),and two nitrogen or oxygen ligands. Further analyses have revealedthat Fur purified in the presence of chelators retains a singlezinc ion (Zn₁Fur), while in the absence of chelators each monomerbinds two zinc ions (Zn₂Fur) (1). Remarkably, both forms bindDNA with similar affinities (1), consistent with our findingsthat Fur from B. subtilis contains associated zinc and binds DNAeven in the absence of addediron.

The second, lower-affinity metal-binding site is presumed to be the regulatory site. In vivo, Fur_EC maintains a level of free(chelatable) iron near 10 µM (27). Thus, the in vivo dissociationconstant for the functional interaction of Fe with Fur is probablynear 10 µM. In vitro studies have suggested that Fur_EC can beactivated for DNA binding by several divalent ions, includingCo(II), Cu(II), Cd(II), Fe(II), and Mn(II) (14). Similar resultshave been obtained with Pseudomonas aeruginosa Fur (30). Theorigins of the in vivo metal selectivity of Fur-mediated repression,in view of the promiscuous metal-binding properties of the purifiedprotein, are not yet clear. Presumably, levels of free metal ionsin the cell are tightly regulated, and only iron (and under someconditions, manganese) (5, 21, 32) achieves a sufficientlevel to effectrepression.

A model for interactions of B. subtilis Fur with metal ions. We currently favor a model for Fur that includes roles for both a structural zinc-binding site and a regulatory site thatsenses the presence of iron. Our in vivo studies of Fur-mediatedrepression indicate that two histidines (H96 and H97, correspondingto D89 and H90 in both Fur_EC and Salmonella typhimurium Fur) arelikely candidates for Fe(II) ligands. A role for these residuesin binding iron is consistent with the finding that S. typhimuriumH90 mutants are iron blind (20). Curiously, mutation of theseresidues in Fur_EC failed to affect iron-dependent regulation (11).

How can we reconcile the apparent lack of a requirement for an activating metal ion in vitro with the well-documented effectsof iron on in vivo activity? We suggest that in vivo Fur is boundto an inhibitor of DNA binding that is antagonized by iron. Inprinciple, this inhibitor might be another protein, a low-molecular-weightligand, or another metal ion. The last possibility is particularlyattractive, as it is easy to imagine how another metal ion mightcompete for the Fe(II)-binding site. A corollary of this hypothesisis that this alternate form of Fur might be active for DNA bindingat some sites, albeit not those associated with the regulationof iron uptakefunctions.

This model is consistent with several observations. First, the ability of S. typhimurium H90A Fur to function in the acidtolerance response, despite an inability to repress siderophorebiosynthesis genes, suggests that Fur lacking bound Fe(II) maystill have DNA-binding activity (20). Second, Fur proteins containingdifferent metal ions have distinct DNA-binding specificities.For example, while most PerR-regulated genes can be repressedby either iron or manganese, the fur gene is repressed only bymanganese (7-10 and unpublished data). Similarly, repression ofthe sodA gene by Fur_EC is effected only by iron, while eitheriron or manganese can lead to repression of the aerobactin genes(32). By extension, it is easy to imagine that in vivo a divalentmetal ion binds Fur and stabilizes a conformation inactive forbinding to iron-regulated target sites (although not, perhaps,to other target sites) and that only upon displacement by Fe(II)is the ability to bind to iron-regulated promoter regions recovered.Indeed, previous studies indicated that the supplementation ofgrowth medium with some divalent cations can derepress siderophorebiosynthesis and the expression of Fur-regulated genes (9).

In summary, our work confirms the notion that iron regulation in B. subtilis is mediated by a Fur homolog that binds directlyto a fur box, as inferred from previous genetic analyses. However,we have not yet been able to demonstrate iron-responsive DNA bindingin vitro because the protein binds tightly to DNA in the absenceof added iron. We suggest that in vivo there is an inhibitoryfactor, perhaps a metal ion, absent from our in vitro system.We are presently exploring this possibility by using crudeextracts.

	ACKNOWLEDGMENTS

We thank M. Vasil for providing the anti-E. coli Furantibodies.

This work was supported by NSF grantMCB9630411.

	FOOTNOTES

^* Corresponding author. Mailing address: Section of Microbiology, Wing Hall, Cornell University, Ithaca, NY 14853-8101. Phone:(607) 255-6570. Fax: (607) 255-3904. E-mail: jdh9{at}cornell.edu.

Present address: Section of Genetics and Development, Cornell University, Ithaca, NY14853.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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