Surface Signaling in Ferric Citrate Transport Gene Induction: Interaction of the FecA, FecR, and FecI Regulatory Proteins

doi:10.1128/JB.182.3.637-646.2000

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Journal of Bacteriology, February 2000, p. 637-646, Vol. 182, No. 3
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Surface Signaling in Ferric Citrate Transport Gene Induction: Interaction of the FecA, FecR, and FecI Regulatory Proteins

Sabine Enz, Susanne Mahren, Uwe H. Stroeher, and Volkmar Braun^*

Mikrobiologie/Membranphysiologie, Universität Tübingen, D-72076 Tübingen, Germany

Received 28 July 1999/Accepted 26 October 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

In Escherichia coli, transcription of the ferric citrate transport genes fecABCDE is controlled by a novel signal transductionmechanism that starts at the cell surface. Binding of ferric citrateto the outer membrane protein FecA initiates a signal that istransmitted by FecR across the cytoplasmic membrane into the cytoplasmwhere FecI, the sigma factor, is activated. Interaction betweenthe signaling proteins was demonstrated by utilizing two methods.In in vitro binding assays, FecR that was His tagged at the Nterminus [(His)₁₀-FecR] and bound to a Ni-nitrilotriacetic acidagarose column was able to retain FecA, and FecR that was Histagged at the C terminus [FecR-(His)₆] retained FecI on the column.An N-terminally truncated, induction-negative but transport-activeFecA protein did not bind to (His)₁₀-FecR. The in vivo assay involvedthe determination of the FecA, FecR, and FecI interacting domainswith the bacterial two-hybrid Lex-based system. FecA_1-79interacts with FecR_101-317 and FecR_1-85 interactswith FecI_1-173. These data clearly support a model thatproposes interaction of the periplasmic N terminus of FecA withthe periplasmic C-terminal portion of FecR and interaction ofthe cytoplasmic N terminus of FecR with FecI, which results inFecIactivation.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Escherichia coli takes up ferric citrate through the outer membrane by active transport mediated by the FecA receptor proteinand the TonB-ExbB-ExbD energy-transducing device. The TonB-ExbB-ExbDcomplex (2, 18, 23) transfers the energy required for activetransport across the outer membrane (2). Ferric citrate oriron is subsequently released from FecA and binds to FecB in theperiplasm. Iron is then transported across the cytoplasmic membraneby an ATP-binding cassette transport system consisting of theFecC, -D, and -E proteins (3, 10, 19, 24, 30). Ferriccitrate binding to FecA induces transcription of the fecABCDEtransport genes, but does not affect transcription of the fecIRregulatory genes (15, 16). Induction can be uncoupled fromtransport by point mutations in fecA that lead to constitutiveinduction of transcription and the inability to transport ferriccitrate (9). Furthermore, the deletion of residues 14 to 68of mature FecA removes the induction function; however, transportactivity is fully retained (10). A further vital component forthe response to ferric citrate is FecR. FecR is an integral cytoplasmicmembrane protein of 317 residues; the N terminus has been localizedto the cytoplasm and the C terminus has been localized to theperiplasm. A hydrophobic sequence from residues 85 to 100 probablyforms the single transmembrane segment (28). The location ofFecR in the three subcellular compartments (the periplasm, thecytoplasmic membrane, and the cytoplasm) suggests a structuraland functional role in the signaling cascade of the fec system.C- terminally truncated FecR derivatives display a constitutivephenotype and a FecR N-terminal fragment of only 59 amino acids(aa) is able to induce fec transport gene transcription independentlyof ferric citrate (15). These data led us to propose that theinformation of ferric citrate binding to FecA is transmitted acrossthe outer membrane by FecA and across the cytoplasmic membraneby FecR. FecR subsequently activates FecI, which binds the RNApolymerase core enzyme and directs it to the fecA promoter toinitiate transcription of the fecA, -B, -C, -D, and -E genes.Therefore, signal transduction could involve a series of conformationalchanges; starting with the binding of ferric citrate to FecA,a signal is then transmitted through the N terminus of FecA tothe C terminus of FecR and then across the cytoplasmic membraneto the N terminus of FecR, which interacts with FecI. To supportthe model of such a signal cascade, we searched for a physicalinteraction between the proposed Fec signal-transducing proteins.Using N-terminally and C-terminally His-tagged FecR bound to Ni-nitrilotriaceticacid (NTA) agarose columns, we have shown that there is a specificinteraction between isolated FecR and isolated FecA and FecI proteins.An alternative approach was undertaken using an in vivo systembased on the ability of the Lex repressor to bind to an alteredoperator placed upstream of lacZ (5). Using this system, wedemonstrated heterodimer formation of the N terminus of FecA withthe C terminus of FecR and of the N terminus of FecR with FecI.The in vitro and in vivo data demonstrate an interaction of theFecAIR proteins and their subdomains as predicted by the proposedmodel.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains, plasmids, and media. The E. coli strains and plasmids used in this study are listed in Table 1. All strains are derivatives of E. coli K-12, exceptfor the E. coli B derivative BL21(DE3). Cells were grown in tryptone-yeastextract (TY) medium or nutrient broth (NB) medium as previouslydescribed (14). Growth on ferric citrate as the sole iron sourcewas tested on Fec agar plates containing NB medium, 1.5% nutrientagar, 0.2 mM 2,2'-dipyridyl, and 1 mM citrate. Antibiotics wereused at the following concentrations: ampicillin, 50 µg per ml;tetracycline, 12 µg per ml; and chloramphenicol, 40 µg per ml.

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TABLE 1. E. coli strains and plasmids used in this study

Construction of plasmids. Plasmid pFecRHis was constructed by inserting the fecR gene upstream of the codons encoding six histidine residues of thefusion vector pET25b(+) (Novagen, Schwalbach, Germany) cleavedwith NdeI-EcoRI. The fecR gene was amplified by PCR from plasmidpSV66fecIRA' with primers FecRI and His2701 (Table 2).

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TABLE 2. Deoxyoligonucleotides used in this study

Plasmid pHisFecR was obtained as follows. The NdeI-HindIII fragment of fecR from plasmid pAA70 was blunt ended with the Klenowfragment of DNA polymerase I, cloned downstream of the codonsencoding 10 histidine residues in the fusion vector pET19b (Novagen),cleaved with NdeI-BamHI, and blunt ended with the Klenowfragment.

The low-copy-number plasmids pIRHis and pIHisR, in which wild-type fecR was replaced by fecRhis or hisfecR, respectively,were created as follows. The fecRhis-containing NdeI-StyI fragmentfrom plasmid pFecRHis was inserted into the NdeI-HindIII-digestedand Klenow-treated plasmid pIS135 fecIR, yielding pIRHis. PlasmidpIHisR was obtained by cloning the hisfecR-carrying NdeI-PstIfragment into the NcoI-PstI-cleaved and Klenow-treated plasmidpIS135 fecIR.

The following plasmids were all constructed so as to fuse various regions of FecA, FecR, and FecI in frame with either LexA_1-87408or LexA_1-87WT (5). Plasmid pUS10 was constructed by replacingthe BstEII-XhoI fragment containing the Fos zipper on pMS604 withthe N-terminal region of the mature FecA protein with oligonucleotidesLexFecA1 and LexFecA2. Plasmids pUS11 to pUS12 were made by replacingthe XhoI-BlgII fragment of pDP804 containing the Jun zipper motifwith various parts of the FecR periplasmic domain with oligonucleotidesLexFecR1, LexFecR2, LexFecR3, and LexFecR7 (Table 2 and see Fig.4). Plasmid pSM85 encodes the N-terminal region of FecR representingthe region from aa 1 to 85. This region was cloned via XhoI-BglIIinto pDP804. The plasmids pSM19 and pSM9 represent N-terminaldeletions of FecR cloned into pDP804, whereas pSM38 and pSM58are carboxy-terminal deletions of FecR. Plasmid pSM173 is theentire FecI gene cloned into pMS604 via BstEII-PstI.

The regions used for cloning FecA, FecR, and FecI were PCR-amplified products derived from plasmid pSV66. Oligonucleotideprimers and sequences used for the PCR amplification are describedin Table 2. All plasmid constructs were confirmed by DNAsequencing.

PCR techniques. PCR amplification was carried out using Taq polymerase (Qiagen, Hilden, Germany) under standard conditions. DNA was initiallydenatured by heating to 95°C for 5 min. This was followed by 30cycles consisting of denaturing at 95°C for 30 sec, annealingat 55°C for 30 sec, and extension at 72°C for 2min.

Recombinant DNA techniques. Standard techniques (20) or the protocols of the suppliers were used for the isolation of plasmid DNA, PCR, digestion withrestriction endonucleases, ligation, transformation, and agarosegel electrophoresis. DNA was sequenced by the dideoxy chain-terminationmethod (21) using the AutoRead sequencing kit (Pharmacia Biotech,Freiburg, Germany). The reaction products were sequenced on anA.L.F. DNA sequencer (PharmaciaBiotech).

Purification of FecR-(His)₆ and (His)₁₀-FecR. E. coli BL21(DE3) transformed with pFecRHis or pHisFecR was grown at 37°C in TY medium. Transcription of the fusion geneswas induced by adding IPTG (isopropyl- $beta$ -D-thiogalactopyranoside)(1 mM) when the cultures reached an optical density at 578 nmof 0.5 (26). The culture was incubated for 2 h, and the cellswere harvested by centrifugation and suspended in binding buffer(20 mM Tris-HCl, 0.5 M NaCl, 5 mM imidazole [pH 7.9]). Crude cellextracts were obtained by disrupting the cells with a French pressurecell. The inclusion bodies, which contained the overexpressedfusion proteins, were separated by centrifugation (4,000 × g for20 min) and solubilized by incubating for 1 h at 25°C in bindingbuffer supplemented with 6 M urea. Undissolved material was removedby centrifugation (30,000 × g for 30 min), and the supernatantfractions were dialyzed against binding buffer to remove the urea.Precipitated material was removed by centrifugation (30,000 ×g for 30 min), and the supernatants were applied to Ni-NTA agarosecolumns previously equilibrated with binding buffer. After twowash steps with 10 bed volumes of binding buffer and 10 bed volumesof wash buffer (20 mM Tris-HCl, 0.5 M NaCl, 60 mM imidazole [pH7.9]), bound fusion proteins were eluted with 5 bed volumes ofelution buffer (20 mM Tris-HCl, 0.5 M NaCl, 1 M imidazole [pH7.9]). The proteins of each fraction were precipitated with 10%trichloroacetic acid and equal proportions of each fraction wereanalyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis(SDS-PAGE), with 15% acrylamide gels (11).

Binding assays. FecI was purified as described previously (1) with the following specifications. E. coli BL21(DE3) transformed with pAA71fecIwas grown at 37°C in TY medium to an optical density at 578 nmof 0.5. fecI transcription was induced by adding IPTG to a finalconcentration of 1 mM, and the culture incubation was continuedfor 2 h. FecI was solubilized from inclusion bodies by incubatingfor 1 h at 25°C in binding buffer supplemented with 2 mg of N-dodecyl-N,N-dimethyl-3-ammonio-1-propanesulfonateper ml. Undissolved cell debris was removed by centrifugation(30,000 × g for 30 min), and the supernatant was applied to Ni-NTAagarose columns loaded with FecR-(His)₆ or (His)₁₀-FecR. Chromatographywas performed as describedabove.

FecA was overproduced in E. coli BL21(DE3) transformed with pIS711fecA or pSP47fecA $Delta$ 47-101 by the addition of IPTG to thecultures (10). The outer membrane fraction was prepared andsolubilized by incubating for 1 h at 25°C in binding buffer supplementedwith 2 mg of octylglucoside per ml. Undissolved material was removedby centrifugation (30,000 × g for 30 min), and the supernatantwas applied to Ni-NTA agarose columns loaded with the FecR fusionproteins. Chromatography was performed as describedabove.

Immunoblot analysis. After electrophoresis, the SDS-PAGE gels were electroblotted onto nitrocellulose (Schleicher and Schuell, Dassel, Germany)in transfer buffer (25 mM Tris-HCl, 192 mM glycine, 20% [vol/vol]methanol [pH 8.3]) at 20 V for 12 to 16 h. Nitrocellulose wasblocked in wash buffer (20 mM Tris-HCl, 0.5 M NaCl, 0.05% Tween20 [pH 7.5]) supplemented with 3% bovine serum albumin (BSA).Antisera were incubated in wash buffer supplemented with 1% BSAand 1:5,000-diluted antibodies. Antibody-conjugated alkaline phosphatasewith 5-bromo-4-chloro-3-indolylphosphate and nitroblue tetrazoliumin the detection buffer (100 mM Tris-HCl, 100 mM NaCl, 5 mM MgCl₂[pH 9.5]) was used for identification of theproteins.

Polyclonal antiserum was obtained by immunizing rabbits with the SDS-PAGE-purified 20-kDa fragment of FecR (Eurogentec, Seraing,Belgium).

Determination of $beta$ -galactosidase activity. $beta$ -Galactosidase activity was determined according to Miller (14) and Giacomini et al. (7).

For determination of the histidine-tagged FecR in vivo activity, the cells were grown in NB medium supplemented as indicatedabove. For the LexA-based repression system, the cells were grownin TY medium. Bacterial strains were grown overnight in TY mediumsupplemented with 1 mM IPTG. The cultures were subcultured (1:50)in TY medium and allowed to grow for an additional 5 h in thepresence of 1 mMIPTG.

LexA-based repression assay. The various constructs of FecA, FecR, and FecI which are fused to the lexA gene were transformed into strain SU202. The lexAgene used for these fusion lacks the domain normally involvedin the formation of dimers. The strain SU202 contains the lacZgene under the control of an altered sulA operator. The alteredoperator binding site allows only LexA to bind when it has formedheterodimers (5). Differing combinations of plasmids were usedto determine which of the Lex-Fec gene products could form heterodimers.The ability to form heterodimers was monitored by measuring the $beta$ -galactosidase activity. The amount of $beta$ -galactosidase was thendetermined. The formation of heterodimers and therefore the interactionof the fused protein domains are seen as a reduction of $beta$ -galactosidaseactivity.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Construction and chromatographic characterization of FecR histidine tagged at either the N-terminal or C-terminal end. If the N-terminal portion of FecA interacts with the C-terminal portion of FecR, and the N-terminal region of FecR contactsFecI, the His tag should thus be located at the noninteractingend of FecR to prevent interference with binding. Therefore, thefecR gene was cloned into the expression vectors pET25b(+) andpET19b to create FecR derivatives containing a C-terminal 6-histidinetag and an N-terminal 10-histidine tag, respectively. FecR-(His)₆contained a linker of 24 amino acids between (His)₆ and FecR,and (His)₁₀-FecR contained an 11-amino-acid linker. E. coli BL21(DE3)was transformed with each of the resulting plasmids, pHisFecRand pFecRHis, and the hybrid proteins were overexpressed by theaddition of IPTG to the cultures. Both hybrid proteins, like unmodifiedFecR, accumulated as inclusion bodies. To solubilize the proteins,the isolated inclusion bodies were treated with the binding bufferwhich was subsequently used for Ni-NTA agarose column chromatography,supplemented with 6 M urea. Removal of urea by dialysis priorto chromatography resulted in a precipitate of presumably incorrectlyfolded FecR which was removed by centrifugation. Only solubleFecR was used in all further chromatographicanalyses.

The inclusion bodies contained either FecR-(His)₆ or (His)₁₀-FecR and two degradation products, as revealed by SDS-PAGE (datanot shown). FecR is proteolytically cleaved after residue 181into fragments of 20 and 15 kDa (29). Even though full-lengthFecR can be isolated, it always breaks down into the two proteolyticdomains. Figure 1 shows the results of representative chromatographicanalyses of the solubilized portions of FecR-(His)₆ and (His)₁₀-FecRon a Ni-NTA agarose column. Fractions of each chromatographicstep, as indicated in Fig. 1, were analyzed by SDS-PAGE. The uncleavedproteins FecR-(His)₆ and (His)₁₀-FecR, containing linkers of 24and 11 residues, respectively, exhibited the expected molecularmasses of 40.5 and 38 kDa. As Fig. 1A shows, the 20.5-kDa fragmentresulted from the C-terminal 15-kDa portion of FecR plus the 5.5-kDahistidine tag. In (His)₁₀-FecR, the N-terminal FecR 20-kDa fragmentwas increased to 23 kDa. The (His)₁₀-FecR contained an additionaldegradation product of 17 kDa. Immunoblotting with polyclonalFecR antibodies raised to the purified N-terminal 20-kDa FecRdegradation product confirmed that all the fragments arose fromFecR (Fig. 1C). The immunoblot shows the 40.5-kDa uncleaved FecR-(His)₆and its untagged 20-kDa degradation fragment, as well as the 38-kDa(His)₁₀-FecR and its corresponding degradation product of 23 kDa(Fig. 1C). Western blotting with histidine antibodies revealedessentially the same result as with FecR antibodies, with theexception that the anti-histidine serum could detect the 20.5-kDaFecR-(His)₆ fragment instead of the untagged 20-kDa degradationproduct and the 23-kDa fragment of (His)₁₀-FecR (data not shown).As expected, the 20-kDa fragment of FecR-(His)₆ and the 15- and17-kDa fragments of (His)₁₀-FecR did not contain the His label.The protein band of approximately 38 kDa seen in Fig. 1B (flowthrough)does not represent (His)₁₀-FecR as determined by Western blotting.No histidine-tagged FecR was found in any of the wash steps (Fig.1). Why the nonhistidine-labeled fragments were retained on thenickel column is unknown, but it is likely that the proteolyticproducts of FecR stay associated with each other and are thuseluted from the column in conjunction with the histidine-taggedfragment.

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FIG. 1. Affinity chromatography of FecR-(His)₆ (A) and (His)₁₀-FecR (B) on a Ni-NTA agarose column. The eluted fractions were subjected to SDS-PAGE (with 15% acrylamide gels) and stained with Coomassie brilliant blue. (C) Western blotting of Ni-NTA agarose column eluant fractions with anti-FecR serum. FecR-(His)₆, (His)₁₀-FecR, and their proteolytic cleavage products are indicated by arrows. Numbers indicate molecular masses in kilodaltons.

Binding of FecI to FecR-(His)₆ fixed to a Ni-NTA agarose column. Ni-NTA agarose was used as an affinity matrix for FecR-(His)₆ and (His)₁₀-FecR to determine the physical interaction of FecRwith FecI and FecA. FecI was solubilized from inclusion bodieswith binding buffer supplemented with N-dodecyl-N,N-dimethyl-3-ammonio-1-propanesulfonate,which results in active FecI as shown by fecA promoter DNA bandshiftcaused by FecI in the presence of RNA polymerase (1). Thismaterial was then applied to a Ni-NTA agarose column loaded withFecR-(His)₆ (Fig. 2A) or (His)₁₀-FecR (Fig. 2B). In this and thefollowing experiments, a surplus of the proteins was used forloading the column and was removed by the two wash steps untilno protein was eluted. FecI was retained on the column and wascoeluted with FecR-(His)₆, which demonstrates binding of FecIto FecR-(His)₆. In contrast, FecI was completely eluted in theflowthrough and in the first wash from the column loaded with(His)₁₀-FecR. The (His)₁₀ tag at the N terminus of (His)₁₀-FecRpresumably inhibited binding to FecI. This experiment also showsthat FecI itself does not bind to the Ni-NTA agarose column.

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FIG. 2. Binding of FecI to FecR-(His)₆ (A) and (His)₁₀-FecR (B) on a Ni-NTA agarose column. The eluted fractions were subjected to SDS-PAGE (with 15% acrylamide gels) and stained with Coomassie brilliant blue. FecI, FecR-(His)₆, (His)₁₀-FecR, and their proteolytic cleavage products are indicated by arrows. Numbers indicate molecular masses in kilodaltons.

Binding of FecA to (His)₁₀-FecR fixed to a Ni-NTA agarose column. FecA was solubilized from isolated outer membranes with binding buffer supplemented with octylglucoside and then applied toa Ni-NTA agarose column loaded with (His)₁₀-FecR (Fig. 3A) orFecR-(His)₆ (Fig. 3B). The majority of FecA coeluted with (His)₁₀-FecRand only low amounts of FecA were detected in the flowthroughof the (His)₁₀-FecR column and in the first wash. In contrast,FecA was hardly retained on the FecR-(His)₆ column. Retentionof FecA by (His)₁₀-FecR and failure of retention by FecR-(His)₆support the conclusion that FecA is bound to FecR and that theC-terminal portion of FecR recognizes FecA.

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FIG. 3. Binding of FecA to (His)₁₀-FecR (A) and FecR-(His)₆ (B) on a Ni-NTA agarose column and of FecA $Delta$ 47 to His₁₀-FecR (C) on a Ni-NTA agarose column. The eluted fractions were subjected to SDS-PAGE (with 15% acrylamide gels) and stained with Coomassie brilliant blue. FecA, FecA $Delta$ 47 (designated FecA47), FecR-(His)₆, (His)₁₀-FecR, and their proteolytic cleavage products are indicated by arrows. Numbers indicate molecular masses in kilodaltons.

The reliability of FecA binding to (His)₁₀-FecR was tested with FecA47. Previous studies have shown that FecA47, which lacksresidues 14 to 68 of mature FecA, displays no induction activitybut full transport activity (10). FecA47 was not retained by(His)₁₀-FecR and was eluted in the flowthrough and the first wash(Fig. 3C). The results of this control experiment support a directand specific role of the periplasmic N terminus of FecA and theC-terminal portion of FecR in FecA-FecR interaction. Control experimentswith FecA alone show no binding to the Ni-NTA agarose column (datanotshown).

In vivo activity of FecR-(His)₆ and (His)₁₀-FecR. Induction of fec transport gene expression was studied in E. coli AA93 $Delta$ fec transformed with plasmid pIS1034, which encodesfecA and a fecA-lacZ promoter fusion. $beta$ -Galactosidase activitywas determined 2 h after the addition of 1 mM citrate to cellscultivated in NB medium. Plasmids pIRHis and pIHisR were constructedby replacing wild-type fecR by fecRhis or hisfecR on the low-copy-numberplasmid pIS135 fecIR. Under these conditions, no inclusion bodieswere observed. FecR-(His)₆ and (His)₁₀-FecR responded to citrateand displayed approximately 60% wild-type FecR activity (Table3). No $beta$ -galactosidase activity above background level was detectedwithout the addition of citrate; no activity was detected in E.coli AA93 without FecR (pIS136 fecI). These results demonstratethat the addition of histidines to the C terminus or the N terminushad only a minor effect on FecR activity and that the histidine-taggedFecR derivatives were properly inserted into the cytoplasmic membrane.

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TABLE 3. Induction of fecA-lacZ expression in E. coli AA93 $Delta$ fec pIS1034 fecA fecA-lacZ synthesizing wild-type FecR, FecR-(His)₆, (His)₁₀-FecR, or no FecR

In vivo interaction of the N terminus of FecA with the C terminus of FecR. In vivo interaction of the N terminus of FecA with the C terminus of FecR was examined with a bacterial two-hybrid system(5). The two-hybrid system is based on the ability of the LexAprotein to form dimers, which then bind to the sulA operator anddownregulate transcription. The LexA protein consists of two distinctdomains: one domain is required for the dimerization and the otheris required for binding to the operator sequence. In this system,the dimerization domain is deleted from LexA and replaced withother domains that are thought to dimerize. The control plasmidpMS604 contains the first 87 aa of LexA-408 and the control plasmidpDP804 contains the first 87 aa of the wild-type LexA (the regioninvolved in operator binding), fused to the Fos and Jun zippermotifs, respectively. In the bacterial strain SU202, an alteredsulA hybrid operator containing a site with a wild-type half anda mutated half is placed in front of lacZ, which acts as the reportergene for LexA binding. This altered operator is only bound iftwo heterodimeric LexA molecules are formed. The DNA encodingthe first 79 aa of the mature FecA protein and aa 101 to 317 ofFecR were PCR amplified. These regions were chosen as the mostlikely interacting domains between FecA and FecR, since the Nterminus of FecA reaches into the periplasm as does the C terminusof FecR (10, 28). The FecA region was cloned via the restrictionendonuclease sites BstEII-XhoI into pMS604, giving rise to pUS10(FecA_1-79),whereas the FecR region was cloned with XhoI-BglII restrictionsites into pDP804, giving rise to pUS11(FecR_101-317) (Fig.4). These cloning strategies remove the Fos and Jun zipper motifspresent on pMS604 and pDP804. Since the cloned regions were derivedfrom PCR amplification, several independent clones were examined.Plasmids pUS12 and pUS13, also obtained by PCR amplification,represent amino- and carboxy-terminal deletions of FecR. Thiswas done in an attempt to define a minimal region of FecR thatinteracts with FecA. The plasmid pUS12 encodes aa 151 to 317 ofFecR fused to LexA_1-87408 and represents the PCR amplificationproduct with oligonucleotides LexFecR2 and LexFecR3, whereas pUS13encodes aa 101 to 275 of FecR and is derived from oligonucleotidesLexFecR1 and LexFecR7 (Fig. 4).

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FIG. 4. Diagrammatic representation of the cloning of FecA, FecR, and FecI regions into the plasmids pDP804 and pMS604. Domains of FecA and FecI were fused in frame to LexA_1-87WT, by which the Fos zipper domain originally present in pMS604 was deleted. Domains of FecR were all cloned into the XhoI-BglII restriction endonuclease sites present in pDP804. All fecR regions cloned are fused in frame to Lex_1-87408, which deleted the Jun zipper motif in pDP804.

We examined the ability of pUS10(LexA_1-87WT-FecA_1-79) and pUS11(LexA_1-87408-FecR_101-317) to interactwith the sulA operator and repress the production of $beta$ -galactosidase.Initially, we determined if the various proteins alone could repressthe lac gene in the absence of an appropriate partner. The plasmidspDP804(LexA_1-87408-Jun zipper), pMS604(LexA_1-87WT-Foszipper), pUS10(LexA_1-87WT-FecA_1-79) and pUS11(LexA_1-87408-FecR_101-317)alone showed no repression of the lac system. This nonrepressedlevel was then set as the 100% level. All subsequent $beta$ -galactosidaseactivity is given as a percentage of this level. The combinationof the proteins LexA_1-87WT-FecA_1-79 with LexA_1-87408-FecR_101-317gave a residual activity of 9%. $beta$ -Galactosidase activity of thecontrol plasmid pMS604(LexA_1-87WT-Fos zipper) with pDP804(LexA_1-87408-Junzipper) was on the order of 4 to 7%. The combination of LexA_1-87WT-FecA_1-79with LexA_1-87408-FecR_101-317 showed repression tothe same level as the active control. The amino- and carboxy-terminalFecR fragments encoded by pUS12(LexA_1-87408-FecR_151-317)and pUS13(LexA_1-87408-FecR_101-275) and combined withpUS10(LexA_1-87 WT-FecA_1-79) gave $beta$ -galactosidase activitieson the order of 100% (Table 4). This would indicate that bothFecR regions (residues 101 to 150 and 275 to 317) contribute tothe interaction with FecA. This does not, however, rule out othersites of interaction with FecA within residues 151 to 274 of FecR.Next, we determined if there is any nonspecific interaction betweenproteins LexA_1-87WT-FecA_1-79 and LexA_1-87408-Junzipper and between LexA_1-87408-FecR_101-317 and LexA_1-87WT-Fos zipper. These protein combinations showed no repressionof lacZ (Table 4). It is therefore clear that the repressionof lacZ taking place with the protein combinations LexA_1-87WT-FecA_1-79 and LexA_1-87408-FecR_101-317 is dependenton the interaction of the FecA and FecR domains fused to LexA.

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TABLE 4. $beta$ -Galactosidase activity by the bacterial two-hybrid Lex-based system in E. coli SU202 sulA::lacZ^a

In vivo interaction of the N terminus of FecR with FecI. In vivo interaction of the C terminus of FecR with FecI was examined by the same bacterial two-hybrid system used for theFecA-FecR interaction. Prior to cloning the FecI gene fragmentinto pMS604, the residual Fos zipper was removed via PvuII-AsnIrestriction. Since FecI contains a XhoI restriction endonucleasesite, it was not possible to clone it in the same manner as FecA,and it was thus cloned via BstEII-PstI into pMS604, giving riseto pSM173. The plasmid pSM173 contains the complete fecI geneof 519 bp (173 aa) (Fig. 4). To define a minimal interacting regionon FecI, amino- and carboxy-terminal deletions were constructed.Plasmid pSM133 contains aa 1 to 133 of FecI and was made by PCRamplification with oligonucleotides FecIBstEII and FecI4.2 (Table2). The N-terminal deletion plasmid designated pSM4 containsaa 82 to 173 of FecI and was constructed by PCR amplificationwith oligonucleotides FecI2 and FecIPstI. For the constructionof LexA_1-87408-FecR_1-85, the region encoding aa 1through 85 of FecR was PCR amplified and cloned via XhoI-BglIIinto pDP804. The resultant plasmid was designated pSM85. Thisregion represents the cytoplasmic domain of FecR, which is mostlikely where FecR interacts with FecI. In addition, various deletionswere constructed in an attempt to define a minimal region of FecRthat interacts with FecI. The resultant plasmids, designated pSM9and pSM19, have the first 9 or 19 aa of FecR deleted, respectively.Plasmids pSM38 and pSM58 encode FecR fragments from aa 1 to 38and 1 to 58, respectively. All four constructs were cloned intopDP804 via XhoI-BglII (Fig. 4). All FecR constructs are fusedin frame with LexA_1-87408, whereas the FecI constructs arefused to LexA_1-87WT.

For the determination of the interaction between FecR and FecI, the same approach was taken for FecA as for FecR. The combinationsof LexA_1-87408-FecR_1-85(pSM85) and LexA_1-87WT-FecI_1-173(pSM173)proteins showed clear repression of $beta$ -galactosidase activity (residualactivity 14%) (Table 4). The deletions of FecR represented bythe proteins LexA_1-87408-FecR_9-85(pSM9) and LexA_1-87408-FecR_1-58(pSM58)in combination with LexA_1-87WT-FecI_1-173 also repressed $beta$ -galactosidase synthesis to 12 and 14%, respectively (Table 4).The protein LexA_1-87408-FecR_9-85(pSM9) contains adeletion of 9 aa from the N terminus of FecR, whereas LexA_1-87408-FecR_1-58(pSM27) is a 27-aa deletion from the periplasmicC terminus. Other FecR deletions represented by LexA_1-87408-FecR_19-85(pSM19)and LexA_1-87408-FecR_1-38(pSM38) showed no repression.Furthermore, all deletions affecting FecI represented by LexA_1-87WT-FecI_1-133(pSM133)and LexA_1-87WT-FecI_82-173(pSM4) showed no repression.As controls, the proteins LexA_1-87WT-FecI_1-173(pSM173)and LexA_1-87408-FecR_1-85(pSM85) alone or in combinationwith LexA_1-87408-Jun zipper(pDP804) and LexA_1-87WT-Foszipper(pMS604), respectively, showed no repression of $beta$ -galactosidaseactivity (Table 4). The data indicate that a region encompassingaa 9 to 58 of FecR is required for the interaction with FecI.Furthermore, it would appear that a large region of FecI is requiredfor the interaction withFecR.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The chromosomally encoded FecR regulatory protein is contained in cells in such low amounts that it cannot be detected afterradiolabeling and SDS-PAGE or by Western blotting. It has to beoverexpressed, and then it precipitates as inclusion bodies (15,29). Although FecR-(His)₆ and (His)₁₀-FecR were more hydrophilicthan FecR, they also formed inclusion bodies which were barelycontaminated with other proteins, as revealed by SDS-PAGE. Theinclusion bodies were not soluble in buffers and buffers supplementedwith detergents that usually do not denature proteins, such asoctylglucoside, Triton X-100, Tween 20, CHAPS {3-[(3-cholamidopropyl)-dimethylammonio]-1-propanesulfonate},and Nonidet P-40; for this reason these detergents are frequentlyused to solubilize cytoplasmic membrane proteins. Very likely,the small portion of active FecR-(His)₆ and (His)₁₀-FecR thatwas inserted in the cytoplasmic membrane was solubilized, butthe amounts were not sufficient for detection by staining afterSDS-PAGE and for performing in vitro binding studies. Urea (6M) had to be used to solubilize the inclusion bodies. This procedurealmost certainly denatured FecR-(His)₆ and (His)₁₀-FecR, and itis not known to what extent FecR-(His)₆ and (His)₁₀-FecR renaturedduring the dialysis to remove urea. However, retention of FecAand lack of retention of FecA $Delta$ 47-101 on the Ni-NTA agarose columnand retention of FecI by FecR-(His)₆ but not by (His)₁₀-FecR demonstratebinding specificity which suggests correctly folded FecR derivativesare present. In addition, since not only the His-tagged completeproteins and the His-tagged proteolytic fragments but also theuntagged fragments were retained by the Ni-NTA column, the untaggedfragments were probably bound to the His-tagged fragments. A well-knownexample of the preservation and restoration of an active proteinafter the cleavage of a peptide bond is $alpha$ -complementation of $beta$ -galactosidase.FecR is also cleaved by an unknown protease to the same two majorproducts as are the His-tagged FecR derivatives. The requirementfor cleavage of FecR for induction of the fec system was studiedwith a number of FecR mutants (29). Of eight FecR mutants whichwere inactive or which transcribed fecA-lacZ constitutively, sevenwere no longer cleaved. This clearly showed that there is no correlationbetween cleavage and phenotype, and since the mutations were scatteredover the entire polypeptide, specific proteolytic processing canbe ruled out for FecR activity (29).

The interaction and binding of the FecA N-terminal, but not the C-terminal, region to (His)₁₀-FecR was shown by control experimentswhich demonstrated that FecA47, lacking residues 14 to 68, didnot bind to (His)₁₀-FecR, which clearly shows the specificityfor the N terminus of FecA. Furthermore, the specificity of bindingto the N terminus of FecR was demonstrated by experiments in whichFecA did not bind to FecR-(His)₆. The histidine residues at theC terminus of FecR-(His)₆ apparently prevented binding of FecA.This lack of binding could be due to steric reasons such thatthe His tag masks the binding site on FecR or that fixation ofFecR-(His)₆ on Ni-NTA agarose hinders access to the C-terminalportion of FecR or the partially charged His residues repulseFecA. Since FecR-(His)₆ displayed 60% in vivo activity in ferriccitrate-dependent regulation of fecA-lacZ transcription, and sincethis activity should be much lower if binding of FecA to FecR-(His)₆is impaired, it is more likely that fixation of FecR-(His)₆ toNi-NTA agarose is the cause for the lack of FecA-FecR-(His)₆ interaction.For the in vivo relevance of the demonstrated interaction betweenFecA and FecR-(His)₆, one has to take into account that the invitro interactions were not influenced by the addition of ferriccitrate (data not shown). This was not unexpected, since transcriptioninitiation in vivo requires not only binding of ferric citrateto FecA but also the electrochemical potential of the cytoplasmicmembrane mediated by the Ton system (10). Since the in vitroconditions do not reflect the in vivo situation, these experimentsdo not reveal whether FecA binds permanently to FecR in vivo.However, the in vitro data clearly demonstrate that the N terminusof FecA and the C terminus of FecR are required for FecA-FecRinteraction, which supports the previous in vivo data (10).

Active FecI was solubilized from inclusion bodies with a detergent, as was demonstrated previously (1). Solubilized FecIwas shown to direct the RNA polymerase core enzyme to the promoterupstream of the fecA gene, as revealed by bandshift experimentsand by in vitro runoff transcription assays (1). Here, FecR-(His)₆but not (His)₁₀-FecR retained FecI on Ni-NTA-agarose; this resultsupports our previous data, which localized the N terminus ofFecR in the cytoplasm and which demonstrated constitutive transcriptionof the fec transport genes by cytoplasmic N-terminal fragmentsof FecR (15, 28). The reasons for the failure of (His)₁₀-FecRto bind FecI may be the same as those proposed for the failureof FecA to bind to FecR-(His)₆. The relative levels of bindingof FecA to (His)₁₀-FecR compared to that seen for FecI bindingto FecR-(His)₆ may be explained by possible differences in theaffinity of FecA compared to FecI for FecR. Alternatively, thebinding sites on FecR-(His)₆ for FecI are more accessible thanthose for FecA for binding to (His)₁₀-FecR.

The approximately 60% activity of FecR-(His)₆ and (His)₁₀-FecR in ferric citrate-dependent induction of fecA transcriptionindicates that a fraction of the His-tagged FecR derivatives isproperly inserted in the cytoplasmic membrane, receives the signalfrom FecA, transmits the signal across the cytoplasmic membrane,and activates FecI. Using SDS-PAGE and immunoblotting (see Fig.1C) of the His-tagged FecR proteins cloned into high-copy-numberplasmids and overexpressed, we found no indication that a fractionof the proteins lost the His tags and for this reason were active.The assays carried out to determine if the His-tagged FecR proteinsare active were done using low-copy-number plasmids, which shouldsignificantly reduce the possibility that there is active FecRwithout a His tag. We cannot, however, rule out the possibilitythat very small amounts (below our levels of detection) of theHis-tagged FecR proteins have lost their tag. Attempts to maintainFecR in solution by creating a hybrid protein with thioredoxin,which has been shown to work in a number of cases (12), didnot prevent the formation of inclusion bodies for FecR (data notshown). The hybrid protein containing thioredoxin fused to theN-terminus of FecR displayed regulatory activities, similar to(His)₁₀-FecR. Upon the addition of ferric citrate to the growthmedium, $beta$ -galactosidase activity of a fecA-lacZ promoter fusionincreased from 9 to 250 U, which amounts to 77% of the $beta$ -galactosidaseactivity obtained by induction with wild-type fecR (data not shown).This high level of activity is not surprising, since we know fromour in vivo experiments with the bacterial two-hybrid Lex-basedsystem that the first 9 aa of FecR are dispensable for activityand may serve as a linker between FecR and thioredoxin, thus leavingthe cytoplasmic activity domain unaffected to interact withFecI.

The regions of FecA and FecR chosen to examine the interaction with the two-hybrid system were localized to the periplasmaccording to our previous studies. Moreover, the FecA N-proximalregion constitutes a domain whose sole function appears to beimportant for the induction of fec transport gene transcriptionbut not for transport itself. This has been shown by deletionstudies in which residues 14 to 68 of the mature FecA proteinwere removed; this resulted in an induction-inactive but transport-competentFecA derivative. The structure of the N-terminal region of FecAis quite distinct from those of other TonB-dependent transporters.The TonB box required for transport and induction is located atresidues 81 to 84 in FecA, since the FecA N terminus representsan extension when compared to the other TonB-dependent transportersin the outer membrane of E. coli K-12 in which the TonB box isclose to the N terminus (10). The extension of FecA is not partof the globular domain that closes the channel of the $beta$ barrelin the crystal structure of FhuA (6, 13) and FepA (4),if one assumes an overall structure of FecA that is similar toFhuA and FepA. Rather, the long N terminus of FecA would be containedin the periplasm like the N terminus of FhuA and FepA which arenot seen in the crystal structure, probably because they are flexibleand assume no fixed structure. The strong allosteric changes inthe periplasmically exposed region of the globular domain of FhuAupon ferrichrome binding may occur similarly in FecA upon ferriccitrate binding. However, FecA in contrast to FhuA employs thestructural transition to initiate a signaling cascade that finallyinitiates transcription of the fec transport genes. The C-proximalregion of FecR and the N-proximal region of FecR used for studyinginteractions with FecA and FecI also form domains that are separatedby the FecR transmembrane region (residues 85 to 100). We thereforeemployed three domains in the two-hybrid system which displaysome structural independence but receive signals from the surface-exposedferric citrate binding site of FecA and transmit signals throughthe C-proximal region of FecR to the N-terminus of FecR and fromthere toFecI.

The use of the in vivo LexA-based repression system to look at the interaction of FecA with FecR and FecR with FecI clearlyshows that these interactions do take place in vivo and supportsthe data obtained from the in vitro column binding assays. TheLexA system has been successfully used to define very small regionsof protein interaction, for example between the Jun and Fos zippermotifs (5). We have been able to show that the first 79 aaof the mature FecA polypeptide interact with the proposed periplasmicdomain of FecR, consisting of aa 101 to 317. It has not been possibleto reduce this region in FecR and still maintain FecR activity.FecA may interact with FecR over a large region, or FecA may interactwith the N and C termini of the 101- to 317-aa region of FecR.It is also feasible that the active conformation of the periplasmicsegment of FecR is impaired by thedeletions.

Interaction of the cytoplasmic region of FecR with FecI has been reduced to a region between aa 9 and 58. In contrast, ithas not been possible to determine the precise region of FecIthat interacts with FecR, since both deletion derivatives wereunable to form heterodimers. The interaction may take place overlarge or multiple domains of FecI, or the conformation of FecImay be disturbed by the deletions. We have some initial data basedon phage display library biopanning which indicate that the FecRinteractions take place over the entire FecI protein. FecI belongsto the family of ECF (extracytoplasmic function) sigma factors,which contain a number of functional domains. The deleted segmentsrepresent all of regions 2 and 4.2 of FecI. Initial data showthat FecI deletion mutants, which have region 3 removed, are stillable to interact with FecR. This would indicate, first, that deletionsin FecI do not necessarily lead to instability and, second, thatit is likely that there are sites within regions 2 and 4.2 whichinteract with FecR. The lack of interaction between the variousdeletion constructs indicates that the interaction of the variouscomponents of the Fec system is dependent on secondary structureconservation, and thus many deletions are likely to disrupt thestructural framework. Alternatively, the deletions we have constructedin FecR and FecI are unstable, and attempts to show the stabilityof all of the LexA fusions used were unfortunately unsuccessful.It was not possible to show the presence of these fusion proteinseither by Coomassie blue staining in the soluble or insolublefraction or by immunoblotting with either FecA or FecR antiserum.This would indicate that these proteins are expressed at verylow levels or, alternatively, that our antisera do not recognizethose regions fused to LexA_1-87. This is unlikely in thecase of FecR, where large regions of FecR are fused to LexA; however,in the case of FecA, this is a possible explanation since onlyabout 10% of the total length of the protein was fused toLexA.

Both the in vitro and in vivo data show interactions between the N terminus of FecA and the periplasmic domain of FecR andbetween the cytoplasmic domains of FecR and FecI. However, theseinteractions occurred in the absence of the ferric citrate inducer.We therefore conclude that the signal transduction from FecA toFecR and then to FecI is not due simply to the interaction itselfbut possibly to changes in interaction upon binding of ferriccitrate to FecA. Alternatively, the Fec proteins may show an interactionpattern similar to that seen in the aspartate receptor in thechemotaxis sensory signaling cascade. In this system, there isa stable complex consisting of the aspartate receptor, CheW, andCheA. The binding of aspartate does not change the associationconstant of these proteins; in fact, binding causes only a verysmall change in the aspartate receptor itself. It is now assumedthat this change is a piston-like motion of approximately 1 Åof the $alpha$ -helical transmembrane domains of the receptor. This motionis transmitted from the periplasmic to the cytoplasmic side ofthe membrane and it is assumed to be perceived by the methylationand phosphorylation enzymes (17). This system exemplifies thatprotein-protein interactions are able to occur in these systemsin the absence of an inducermolecule.

	ACKNOWLEDGMENTS

We thank A. Angerer and K. Hantke for helpful discussions and M. Granger-Schnarr for providing the plasmids and strains ofthe Lexsystem.

This work was supported by the Deutsche Forschungsgemeinschaft (SFB 323, project B1). U.H.S. was the recipient of an Alexandervon Humboldt ResearchFellowship.

	FOOTNOTES

^* Corresponding author. Mailing address: Mikrobiologie/Membranphysiologie, Universität Tübingen, Auf der Morgenstelle 28,D-72076 Tübingen, Germany. Phone: 49 7071 2972096. Fax: 49 7071294634. E-mail: volkmar.braun{at}microbiol.uni-tuebingen.de.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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Burton, C. L., Chhabra, S. R., Swift, S., Baldwin, T. J., Withers, H., Hill, S. J., Williams, P. (2002). The Growth Response of Escherichia coli to Neurotransmitters and Related Catecholamine Drugs Requires a Functional Enterobactin Biosynthesis and Uptake System. Infect. Immun. 70: 5913-5923 [Abstract] [Full Text]
Kiratisin, P., Tucker, K. D., Passador, L. (2002). LasR, a Transcriptional Activator of Pseudomonas aeruginosa Virulence Genes, Functions as a Multimer. J. Bacteriol. 184: 4912-4919 [Abstract] [Full Text]
Reischl, S., Wiegert, T., Schumann, W. (2002). Isolation and Analysis of Mutant Alleles of the Bacillus subtilis HrcA Repressor with Reduced Dependency on GroE Function. J. Biol. Chem. 277: 32659-32667 [Abstract] [Full Text]
Mahren, S., Enz, S., Braun, V. (2002). Functional Interaction of Region 4 of the Extracytoplasmic Function Sigma Factor FecI with the Cytoplasmic Portion of the FecR Transmembrane Protein of the Escherichia coli Ferric Citrate Transport System. J. Bacteriol. 184: 3704-3711 [Abstract] [Full Text]
Shen, J., Meldrum, A., Poole, K. (2002). FpvA Receptor Involvement in Pyoverdine Biosynthesis in Pseudomonas aeruginosa. J. Bacteriol. 184: 3268-3275 [Abstract] [Full Text]
Lamont, I. L., Beare, P. A., Ochsner, U., Vasil, A. I., Vasil, M. L. (2002). Siderophore-mediated signaling regulates virulence factor production in Pseudomonasaeruginosa. Proc. Natl. Acad. Sci. USA 99: 7072-7077 [Abstract] [Full Text]
Howard, S. P., Herrmann, C., Stratilo, C. W., Braun, V. (2001). In Vivo Synthesis of the Periplasmic Domain of TonB Inhibits Transport through the FecA and FhuA Iron Siderophore Transporters of Escherichia coli. J. Bacteriol. 183: 5885-5895 [Abstract] [Full Text]
Vanderpool, C. K., Armstrong, S. K. (2001). The Bordetella bhu Locus Is Required for Heme Iron Utilization. J. Bacteriol. 183: 4278-4287 [Abstract] [Full Text]
Pradel, E., Locht, C. (2001). Expression of the Putative Siderophore Receptor Gene bfrZ Is Controlled by the Extracytoplasmic-Function Sigma Factor BupI in Bordetella bronchiseptica. J. Bacteriol. 183: 2910-2917 [Abstract] [Full Text]
Stiefel, A., Mahren, S., Ochs, M., Schindler, P. T., Enz, S., Braun, V. (2001). Control of the Ferric Citrate Transport System of Escherichia coli: Mutations in Region 2.1 of the FecI Extracytoplasmic-Function Sigma Factor Suppress Mutations in the FecR Transmembrane Regulatory Protein. J. Bacteriol. 183: 162-170 [Abstract] [Full Text]
McClelland, M., Florea, L., Sanderson, K., Clifton, S. W., Parkhill, J., Churcher, C., Dougan, G., Wilson, R. K., Miller, W. (2000). Comparison of the Escherichia coli K-12 genome with sampled genomes of a Klebsiella pneumoniae and three Salmonella enterica serovars, Typhimurium, Typhi and Paratyphi. Nucleic Acids Res 28: 4974-4986 [Abstract] [Full Text]
Daines, D. A., Silver, R. P. (2000). Evidence for Multimerization of Neu Proteins Involved in Polysialic Acid Synthesis in Escherichia coli K1 Using Improved LexA-Based Vectors. J. Bacteriol. 182: 5267-5270 [Abstract] [Full Text]

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