The Major Phase-Variable Outer Membrane Protein of Escherichia coli Structurally Resembles the Immunoglobulin A1 Protease Class of Exported Protein and Is Regulated by a Novel Mechanism Involving Dam and OxyR

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Journal of Bacteriology, April 1999, p. 2132-2141, Vol. 181, No. 7
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

The Major Phase-Variable Outer Membrane Protein of Escherichia coli Structurally Resembles the Immunoglobulin A1 Protease Class of Exported Protein and Is Regulated by a Novel Mechanism Involving Dam and OxyR

Ian R. Henderson^* and Peter Owen

Department of Microbiology, Moyne Institute of Preventive Medicine, Trinity College Dublin, Dublin 2, Ireland

Received 14 October 1998/Accepted 24 January 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Here we report the characterization of an Escherichia coli gene (agn43) which encodes the principal phase-variable outer membraneprotein termed antigen 43 (Ag43). The agn43 gene encodes a precursorprotein of 107 kDa containing a 52-amino-acid signal sequence.Posttranslational processing generates an $alpha$ ⁴³ subunit (predicted M_r of 49,789) and a C-terminal domain ( $beta$ ⁴³) with features typical of a bacterial integral outer membraneprotein (predicted M_r of 51,642). Secondary structure analysispredicts that $beta$ ⁴³ exists as an 18-stranded $beta$ barrel and that Ag43 shows structuralorganization closely resembling that of immunoglobulin A1 proteasetype of exoprotein produced by pathogenic Neisseria and Haemophilusspp. The correct processing of the polyprotein to $alpha$ ⁴³ and $beta$ ⁴³ in OmpT, OmpP, and DegP protease-deficient E. coli strains pointsto an autocatalytic cleavage mechanism, a hypothesis supportedby the occurrence of an aspartyl protease active site within $alpha$ ⁴³. Ag43, a species-specific antigen, possesses two RGD motifs ofthe type implicated in binding to human integrins. The mechanismof reversible phase variation was studied by immunochemical analysisof a panel of well-defined regulatory mutants and by analysisof DNA sequences upstream of agn43. Evidence strongly suggeststhat phase variation is regulated by both deoxyadenosine methylase(Dam) and by OxyR. Thus, oxyR mutants are locked on for Ag43 expression,whereas dam mutants are locked off for Ag43 expression. We proposea novel mechanism for the regulation of phase switching in whichOxyR competes with Dam for unmethylated GATC sites in the regulatoryregion of the agn43gene.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Workers in this laboratory (33) have recently identified for Escherichia coli the phase-variable product which determinesboth colony morphology and the ability of cells to autoaggregatein liquid media (25). The product in question, termed antigen43 (Ag43), is the major phase-variable protein in the outer membraneand is present in copy numbers exceeding 5 × 10⁴ per cell (55). By multiple criteria, Ag43 has been shown toexist in situ as a hetero-oligomeric complex composed of two chemicallyand immunologically distinct protein subunits (termed $alpha$ ⁴³ and $beta$ ⁴³) present in 1:1 stoichiometry. The $alpha$ ⁴³ subunit (apparent M_r of 60,000) is surface expressed, can extendbeyond the O side chains of smooth lipopolysaccharide, and isbound to the cell through an interaction of its C-terminal domainwith $beta$ ⁴³, itself an integral outer membrane protein showing pronouncedproperties of heat modifiability (apparent M_rs of 37,000 [70°C]and 53,000 [100°C]). The $alpha$ ⁴³ and $beta$ ⁴³ polypeptides contain no detectable carbohydrate, identifiablecofactors, acyl groups, or inter- or intramolecular disulfidebonds. Nearest-neighbor analysis provides evidence that Ag43 isin close proximity to the ferric-enterochelin receptor, FepA (18,56, 57).

Although detailed electron microscopic studies have failed to reveal any morphologically recognizable structure for Ag43 (58),the antigen displays several properties suggestive of an adhesin.Thus, Ag43 enhances adherence of E. coli to certain tissue culturelines in a manner which can be inhibited by purified $alpha$ ⁴³. The $alpha$ ⁴³ (but not the $beta$ ⁴³) subunit can be selectively and almost quantitatively releasedfrom E. coli outer membranes by brief heating to 60°C. In addition,the N-terminal amino acid sequence of $alpha$ ⁴³ contains a six-residue motif (TVNGGT) which is also present inthe N termini of the major subunits of several enterobacterialfimbriae (58). Like expression of many adhesins, expressionof Ag43 is subject to reversible phase variation, the rates inliquid minimal medium from positive (Ag43⁺) to negative (Ag43) states and vice versa being $approx$ 2.2 × 10³ and $approx$ 10³, respectively (18, 56).

We have recently located the gene (agn43) encoding Ag43 to a region of the E. coli K-12 chromosome (min 44.6 to 44.8) betweenamn and sbcB and established its identity with flu (33), thefirst metastable gene to be mapped in E. coli (25). In thiscommunication, we report on the sequence of agn43 and flankingregions, show that Ag43 belongs to the class of proteins knownas bacterial autotransporters (for a review, see reference 32),and demonstrate that phase switching is regulated by a novel mechanisminvolving DNA methylation and OxyR, a LysR-type transcriptionalactivator better known for its ability to control expression ofproteins important in oxidative stress (26, 43, 44). Evidenceis presented which suggests that OxyR may act as a repressor ofAg43 transcription by binding to unmethylated GATC sites in theregulatory region of thegene.

	MATERIALS AND METHODS

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Bacterial strains, plasmids, and culture conditions. The bacterial strains and plasmids used in this study are described in Table 1. All strains were grown on Luria-Bertani agaror broth, supplemented with ampicillin (100 µg/ml), kanamycin(50 µg/ml), and chloramphenicol (25 µg/ml) as appropriate.

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TABLE 1. Bacterial strains and plasmids used

Protein preparation and analysis. Cell envelopes were isolated and the $alpha$ ⁴³ subunit was purified essentially as described by Caffrey and Owen (18). Cell lysateswere analyzed by emulsifying one colony in Laemmli sample buffer,before sodium dodecyl sulfate-polyacrylamide gel electrophoresis(SDS-PAGE). One dimensional SDS-PAGE was performed as detailedelsewhere (46), using 12.5% (wt/vol) polyacrylamide separatinggels and 4.5% (wt/vol) polyacrylamide stacking gels. After electrophoresis,proteins were either stained with Coomassie brilliant blue R250or transferred to a nitrocellulose filter for Western blotting.Western immunoblotting and colony immunoblotting were performedessentially as described by Caffrey et al. (19), using specificanti-Ag43 or anti- $alpha$ ⁴³ rabbit polyclonal antibodies as appropriate. Slide immunofluorescencemicroscopy was based on the method of Nowicki et al. (54) andhas been described in detail elsewhere (33). The discontinuousSDS-PAGE system of Schägger and von Jagow (67) was used forthe separation of protease cleavage products generated followingincubation of either undenatured or heat-denatured (100°C, 5 min) $alpha$ ⁴³ with Staphylococcus aureus V8 protease. Peptides for N-terminalamino acid sequencing were separated on 15% (wt/vol) polyacrylamidegels and were electroblotted to polyvinylidene difluoride membranes,using a transfer buffer containing 10 mM 3-[cyclohexylamino]-1-propanesulfonicacid, 10% (vol/vol) aqueous methanol, and sufficient 4 M NaOHto adjust the buffer to pH 11. Transfer was performed at roomtemperature for 2 h at 200 mA. Amido black-stained bands wereexcised from the polyvinylidene difluoride membrane, and the N-terminalamino acid sequences were determined by the automated sequentialEdman degradation procedure using an Applied Biosystems model470A protein sequencer. Amino acid sequence alignments were generatedby using the FASTA alignment program (62) at Ecole pour lesEtudes et la Recherche en Informatique et Electronique, Nimes,France. Electrospray mass spectroscopy was performed by E. C.Barton, Department of Chemistry, University ofCambridge.

Strategy for sequencing the agn43 gene. To obtain internal amino acid sequence data for cloning purposes, the N-terminal sequences of three internal peptides, $alpha$ ^a, $alpha$ ^b, and $alpha$ ^c, obtained by digestion of heat-denatured $alpha$ ⁴³ with S. aureus V8 protease, were determined and identified asGTANTTVVYAGGDQTV, GAIATGTVINXKGXQVV, and KGSSFTLNAGDTATDTTVN,respectively. Similar proteolysis experiments performed on undenatured $alpha$ ⁴³ revealed two main products. One (M_r of 48,000) had an N-terminalsequence identical to that of native $alpha$ ⁴³ (viz., ADIVVHPGETVNGGTLANH [56]). The other had an apparentM_r and N-terminal sequence identical to those of $alpha$ ^c. The N-terminal sequence of $beta$ ⁴³ was confirmed as PTNVTLASGATWNIPDNA (56).

To localize the agn43 gene, mixtures of oligonucleotides, corresponding to the sequences ADIVVHP and FTLNAGDT from the N-terminalends of $alpha$ ⁴³ and $alpha$ ^c, respectively, were used as primers in PCR performed with chromosomalDNA as the template. An 1,150-bp PCR fragment, amplified fromthe chromosome, was cloned into pBluescript II (pIH1) and thensequenced. Subcloning from pIH1 of 673-bp NsiI/NcoI, 417-bp NsiI/PstI,and 262-bp PstI/NcoI fragments into complementary sites in pGEM-5gave rise to pIH2, pIH3, and pIH4, respectively. Additional subclonespIH5 and pIH6 were constructed from the products of further PCRswhich used the original $alpha$ ⁴³ and $alpha$ ^c primers and oligonucleotides designed from a knowledge of thenucleotide sequence of subclones pIH2 and pIH4. Analysis of thetranslated sequence of the 1,150-bp PCR product indicated thatthe cloned fragment represented part of the Ag43 codingsequence.

Previous work had located the agn43 gene to two overlapping $lambda$ clones in the Kohara miniset library at 44.6 to 44.8 min onthe physical map of the E. coli chromosome (33, 53). However,all attempts to subclone agn43 from these $lambda$ clones or from restrictedchromosomal DNA into the vectors pBluescriptII SK+, pGEM5, andpUC19 proved unsuccessful. In view of this fact, PCR was usedin attempts to isolate and sequence agn43. In this respect, primerswere designed from a knowledge of the N-terminal amino acid sequenceof $beta$ ⁴³ and from known sequences within the genetic elements IS2F andsbcB flanking the chromosomal region presumed to contain the agn43gene. These and other primers were used in PCRs to create clonespIH7 to -10, covering the balance of the agn43 gene together withflanking DNA. DNA was sequenced by primer walking at least twicein both directions using independentclones.

PCR and molecular cloning procedures. PCR amplifications were performed with 500 ng of chromosomal DNA as the template and 0.2 µM (each) primer in a 100-µl reactionmixture containing 2 U of Taq DNA polymerase, 50 µM (each) deoxynucleosidetriphosphate, 1.5 mM MgCl₂ and 10 µl of the manufacturer's buffer.Forty cycles of 1 min of denaturation at 94°C, 1 min of primerannealing at 65°C, and 1-min extension by Taq polymerase at 72°Cwere carried out. E. coli ML308-225 derivatives were constructedby P1 transduction (52) from E. coli K-12 strains harboringthe mutations of interest. DNA analysis and manipulations wereperformed according to standard methods (3).

DNA sequence determination and analysis. Initial DNA sequencing reactions were performed as instructed by the manufacturer with the FLASH thermal cycle sequencingkit (Genpak Ltd.) and M13 universal forward and reverse primers.Primer-walking sequencing reactions were carried out by usingdye terminator chemistry at Kings College School of Medicine andDentistry, London, England. All samples were electrophoresed withan ABI 373A sequencer. DNA sequence analysis was performed withthe Genetics Computer Group software package from the Universityof Wisconsin. Sequence similarity searches were carried out withthe BLAST program at the National Center for Biotechnology Information(2).

Southern hybridization. Southern blotting was performed by a modification of the method described by Southern (70) in which a vacuum blotter system(VacuGene; LKB) was used for transfer of DNA to nitrocellulosefilters. Hybridizations were performed at 65°C with random-labeledprobe essentially as described elsewhere (70). The Prime-a-Genekit (Promega) and 20 µCi of [ $alpha$ -³²P]dATP were used to radiolabel purified DNA fragments (25 to 50ng) by nick translation. After incubation, the labeled probe waspassed through a Nick column (Pharmacia) to remove unincorporatedradiolabelednucleotide.

Structural predictions. Computational analysis was performed with different algorithms suited for secondary-structure predictions developed by Kyteand Doolittle (45), Jähnig (37), or Emini et al. (29) whichare available in the HUSAR program package of the Deutsches Krebsforschungszentrum(Heidelberg, Germany). The location of surface sites was alsopredicted by the method of Parker et al. (61). The presenceof coiled-coil segments (8, 48, 49) was assessed by usingthe MultiCoil program (75a).

Nucleotide sequence accession number. The DNA sequence described here has been deposited in the GenBank library and has been assigned accession no. U24429.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Nucleotide sequence of the region encompassing agn43. The total contiguous sequence of 7,738 bp generated by the sequencing strategy detailed in Materials and Methods contained,as expected, an IS2 element 5' to the putative agn43 gene (positions38 to 1363), a large open reading frame (ORF) of 3,275 nucleotides(positions 2477 to 5752) and a bacteriophage P2 attachment site(position 6876 to 7168; GenBank entry U24429). That the largeORF encodes agn43 and that the first ATG codon (position 2636)corresponds to the start site of the gene is supported by a putativetranslation product which shows (i) the presence between residuesM¹ and A⁵² of a region bearing all the hallmarks of an extended signal sequence(see below); (ii) the presence, beginning at residues A⁵³, G²²⁸, G¹⁶¹, K⁴¹⁹, and P⁵⁵², of sequences of amino acids corresponding precisely to thosedetermined empirically for the N termini of $alpha$ ⁴³, $alpha$ ^a, $alpha$ ^b, $alpha$ ^c, and $beta$ ⁴³, respectively; and (iii) excellent correlation for both subunitsbetween the predicted and empirically determined amino acid compositions(18). A sequence similar to a rho-independent transcriptionterminator is present beginning 32 nucleotides beyond the stopcodon and contains interrupted inverted repeats with the potentialfor forming a hairpin structure containing a loop of 11 basesand a stem of 3 bases. The predicted ribosome binding site witha sequence TAAGG was identified 8 bp upstream of the proposedATG start codon and is followed by a stretch of four adenosineresidues which are presumed to confer maximal efficiency of initiationof translation. The overall G+C content of the agn43 gene is 57.6%.Two additional ORFs of 708 and 1,536 bp were identified up- anddownstream of agn43, respectively. Neither ORF displayed significanthomology to any knowngenes.

The putative promoter region revealed sequences (TTGTCA and TATGTT) in good agreement with the consensus sequences predictedfor the $-$ 35 (TTGACA) and $-$ 10 (TATAAT) sites of E. coli genes,though they are separated by only 14 nucleotides. An interestingfeature of this region was the nucleotide sequence homology (39.5%identity) shared between it and the promoter regions of the momand oxyR genes, both of which are known to bind OxyR, a LysR-typetranscriptional activator (12, 22). Moreover, direct comparisonof the OxyR and MuC binding sites of the mom regulatory regionwith that of agn43 shows a region displaying 65.6% identity atthe nucleotide level (Fig. 1). This includes a 6- and a 7-bp stretchof nucleotides identical to those seen at the beginning and theend of the MuC binding domain (13), respectively. The putativepromoter region of agn43 also possesses three GATC sites whichhave the potential for methylation by Dam methylase (Fig. 1).These sites are positioned at points almost identical to thoseobserved for the mom gene. No GATC sites are present in the sameregion of the oxyR promoter.

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FIG. 1. Locations and alignment of OxyR binding sites. The extents of the OxyR binding sites for mom and oxyR have been determined (12, 44). The MuC binding site has been determined for mom (13). MuC and OxyR binding sites are overlined by thick lines. Dashes represent gaps introduced for better alignment. GATC sites are underlined. Identical nucleotides conserved between the three (putative) promoter regions are indicated by dots; identical nucleotides between agn43 and mom sequences are indicated by boldface letters. Only the autoregulatory site of oxyR is shown. Nucleotides are given in the standard single-letter code.

An interesting feature of the DNA region encoding agn43 is the presence of 14 direct repeats of 10 bp or longer and an additional31 repeat stretches of 12 bp or longer which contain one nucleotidemismatch, all of which are translated in the same reading frame.These are located predominantly toward the 5' end of the geneand give rise to repeats in amino acid sequence. The sequenceof agn43 of E. coli ML308-225 (U24429) shows 98% identity atthe nucleotide level to the corresponding gene subsequently sequencedfor E. coli K-12 (AE000291).

Amino acid sequence of the Ag43 precursor. The Ag43 ORF encodes a primary translation product of 1,039 amino acids with a molecular mass of 107,067 Da. The N-terminalregion possesses the characteristics of an enlarged signal sequencewith (i) four positively charged amino acids between residues28 and 33 (R²⁸ARGKR) followed by (ii) a hydrophobic region spanning 12 neutralamino acids and (iii) a sequence (V⁵⁰LA) compatible with the consensus for a signal peptidase recognitionsite (36) (Fig. 2).

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FIG. 2. Comparison of the N-terminal segments of Ag43 and other autotransporters. The leader sequence of Ag43 (this work) has been aligned with those of Tsh (GenBank accession no. I54632), AIDA-I (Q03155), EspC (U69128), SepA (Z48219), Pet (AF056581), Hia (U38617), AIDA-I (I64138), Hsf (U41852), EspP (AB011549), ShMu (U35656), UspA1 (U57551), and HMW-1 (A43855). The N-terminal sequence of HMW-2, which is identical to that of HMW-1, is not shown. The cleavage sites are indicated by <>. The positions of the N, H, and C domains which are characteristic of a signal sequence (36) are also shown.

The mature (signal peptidase processed) protein begins at A⁵³, is composed of 987 amino acids, and has a calculated molecularmass of 101,413 Da. This figure approximates the combined molecularmasses of both subunits as estimated by SDS-PAGE and gel filtration(18). This, together with the fact that the N terminus of mature $beta$ ⁴³ starts at P⁵⁵² (56), suggests that agn43 is initially translated as a polyproteinprecursor which undergoes at least two posttranslational processingsteps, viz. (i) removal of the 52-residue signal peptide and (ii)internal cleavage between D⁵⁵¹ and P⁵⁵² to yield $alpha$ ⁴³ (predicted M_r of 49,789) and $beta$ ⁴³ (predicted M_r of 51,642). That release of $beta$ ⁴³ from the polyprotein precursor involves a single cleavage eventoccurring between D⁵⁵¹ and P⁵⁵² is supported by the results of electrospray mass spectroscopy,which indicate an M_r for purified $alpha$ ⁴³ of 49,807 ± 24.11, in good agreement with the predictedvalue.

The predicted Ag43 polyprotein is notable for the abundance of glycine and threonine residues and the presence of only a singlecysteine residue, which features in the leader peptide. Indeed,the four residues A, T, G, and V constitute 45% of the precursormolecule. $alpha$ ⁴³ has a calculated isoelectric point of 4.85, a value which agreeswell with experimental values (18). The corresponding valuepredicted for $beta$ ⁴³ is 6.15.

Amino acid sequence similarities. Notable sequence similarities were detected between distinct regions of the Ag43 polyprotein and various secreted or surface-exposedproteins in gram-negative bacteria. For example, similaritieswere detected in the signal sequence region between the Ag43 precursorand those of several potential virulence determinants (Fig. 2).An interesting common feature of these signal sequences is that,without exception, they begin with M¹N(R/K) closely followed at residue 9 of Ag43 by a motif (Y/F/W,X, I/L/V, X, or Y/F/W) containing conserved aromatic and hydrophobicresidues. In addition, the sequence V²¹VASELAR observed for Ag43 features in only slightly modified formin the other sequences. Except in Hsf, aidA-I, and Hia, otherregions of the signal sequence, i.e., the N, H, and C domains,show very little sequencesimilarity.

Analysis of $alpha$ ⁴³ alone revealed strong homology (31.2 to 25% identity; 64.7 to 52.5% similarity) with AIDA-I, Tsh, Yejo, andYpjA of E. coli, SepA and IcsA of Shigella flexneri, Hia, aidA-I,and Hsf of Haemophilus influenzae, and BrkA of Bordetella pertussis.Highest scores were achieved with AIDA-I (where alignment extendsfor the 499 amino acids of $alpha$ ⁴³, giving 31.2% identity and 62% similarity) and with the E. coliconceptual translation products termed YpjA (30.5% identity and60.7% similarity) and Yejo (29.6% identity and 58.1% similarity).All alignments began at the first residue of the predicted matureproteins.

In contrast, $beta$ ⁴³ showed only low homology to the C-terminal domains of the same proteins. However, comparison of the C-terminalextremity of $beta$ ⁴³ with corresponding domains of known autotransporters revealedcommonalities in as much as all terminate with an aromatic residue(F or W), which is preceded by aromatic or aliphatic residuesat a periodicity of two residues (32). This is a feature of $beta$ -barrel-forming integral membrane proteins (seebelow).

In view of the sequence similarity between Ag43 and AIDA-I, it was of interest to determine whether the two were immunologicallyrelated. Analysis of AIDA-I-producing E. coli 2787 (6) by colonyand Western immunoblotting and by immunofluorescence microscopyusing anti- $alpha$ ⁴³ antibodies revealed the presence of a 60-kDa phase-variable surfaceantigen, analogous to $alpha$ ⁴³. However, no cross-reacting proteins in the molecular mass range(~100 kDa) anticipated for AIDA-I could be detected in eithercolony lysates or purified cell envelopes (data notshown).

Amino acid motifs. An interesting property of AIDA-I is a region near the N terminus where 21 repeats built up of 19 to 20 amino acid residuesare followed, after a short interruption, by an additional 10repeats (7). In view of the homology displayed between AIDA-Iand Ag43, and the repeat structure observed within agn43, theamino acid sequence of Ag43 was aligned with the conserved consensusmotif observed in AIDA-I (Fig. 3). The major differences notedbetween the repetitive regions of Ag43 and AIDA-I are (i) a smallernumber of repeats in Ag43 with a more variable length (12 to 20residues); (ii) a paucity of serine residues in the Ag43 sequence;and (iii) an additional T or D residue at the start of the Ag43repeat.

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FIG. 3. Comparison of the amino acid sequence of the N-terminal region of Ag43 with the repeat motif of AIDA-I. Alignment begins at T⁶² of the precursor protein. Amino acids are given in the standard single-letter code. The consensus sequence shown at the bottom represents the amino acids most commonly found in the appropriate position.

With regard to functional motifs, the $alpha$ ⁴³ subunit contains a stretch of amino acids (L³⁸⁶LADSGAAVSGT) whose sequence is compatible with the consensus observedfor an aspartyl protease active site (30, 64) and $beta$ ⁴³ contains a sequence (G⁶³¹GRATGKT) compatible with that proposed to form a loop (the P loop)involved in binding ATP or GTP (66). In addition, each subunitpossesses (i) an RGD motif (at R²⁰⁸ and R⁹⁷⁰) implicated in the binding of human integrins (35) and (ii)potential glycosaminoglycan attachment sites at S⁴⁹⁵GNG and S⁶⁵⁴GKG (14). A recent survey has shown the presence of similarmotifs in other autotransporters (32).

Processing of Ag43 in protease-deficient host strains. The possible role of several endogenous membrane-associated proteases, viz., DegP, OmpP, and OmpT, in processing the Ag43precursor to $alpha$ ⁴³ and $beta$ ⁴³ was investigated in protease-deficient mutants. The degP mutationwas transduced from parent strain KS474 (degP) into E. coli ML308-225.The resulting transductant (IRH11) and the ompT ompP strain UT5600were screened for the correct processing of Ag43 by Western blottingusing specific anti-Ag43 antibodies. As shown in Fig. 4, normalprocessing of the Ag43 precursor to $alpha$ ⁴³ and $beta$ ⁴³ occurs in the absence of the DegP, OmpP, and OmpT proteases.Additionally, it should be noted that both subunits retain outermembrane localization (57) in the mutants (data not shown) andthat all attempts to prevent cleavage of the Ag43 precursor toits $alpha$ ⁴³ and $beta$ ⁴³ subunits by the addition, at or before lysis, of a cocktail ofprotease inhibitors (phenylmethylsulfonyl fluoride, N $alpha$ -p-tosyl-L-lysinechloromethyl ketone, and benzamidine HCl) have proved unsuccessful.Normal processing of the Ag43 precursor was also observed in dsbAmutants JCB571 and IRH10 lacking a functional periplasmic disulfideoxidoreductase (Fig. 4).

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FIG. 4. Processing of the Ag43 precursor in E. coli strains carrying the ompT, ompP, and degP mutations. Lane 1, E. coli ML308-225 expressing Ag43; lane 2, ompT ompP strain UT5600; lane 3, ML308-225 degP derivative IRH11; and lane 4, dsbA derivative IRH10. After Western blotting, $alpha$ ⁴³ and $beta$ ⁴³ were detected by using anti-Ag43 antibodies as the primary probe. Note that the differential intensities observed for the $alpha$ ⁴³ and $beta$ ⁴³ subunits are a function of the polyclonal antiserum used and not a reflection of apparent subunit stoichiometry (which is 1:1). The molecular masses of marker proteins are indicated on the right.

Predicted organization of $alpha$ ⁴³ and $beta$ ⁴³ in the outer membrane. Previous studies have clearly shown that $alpha$ ⁴³ is a peripheral surface-expressed protein anchored to the outer membrane via anoncovalent interaction with $beta$ ⁴³ (18, 56). To further elucidate the possible organizationof the subunits in the outer membrane, secondary-structure analyseswere performed. Hydrophobicity plots generated for each subunitaccording to the algorithm of Kyte and Doolittle (45) showedno linear stretch of 20 to 24 hydrophobic amino acids of the typeoften associated with the $alpha$ -helical transmembrane segments ofplasma membrane proteins, nor did either subunit show significantevidence of amphipathic $alpha$ -helical coiled-coil structure (8,48, 49). In contradistinction, $beta$ sheets consisting of alternatinghydrophobic and hydrophilic amino acid residues were predictedwith a high probability for the $beta$ ⁴³ subunit. According to Jähnig (37), amphipathic $beta$ strands ideallyexist with high probability if (i) the calculated values for hydrophobicity[H(i)] vary with a periodicity of two residues between H(i) $>=$ 1.6 and H(i + 1) $<=$ 0.4; (ii) this occurs over at least10 residues; and (iii) for the validity of the prediction, theprotein must form at least an eight-stranded $beta$ -barrel structure.According to these predictions, $beta$ ⁴³ consists of at least 18 membrane-spanning amphipathic $beta$ strandsinterrupted by external loops and generally short periplasmicloops. Regions of high surface probability, predicted accordingto the method of Emini et al. (29) or Parker et al. (61),are in good agreement with this topological arrangement sincesuch areas are always located between the $beta$ strands (data notshown). Accordingly, we propose that the 18 $beta$ sheets are arrangedas depicted in Fig. 5 and form a $beta$ -barrel structure harboringa pore for the translocation of $alpha$ ⁴³ to the cell surface. $alpha$ ⁴³ itself shows five (i.e., <8) potential amphipathic $beta$ strandsand numerous regions, including N⁷⁰ to D⁷², Y⁹¹ to A⁹⁷, A¹¹⁰ to K¹¹², D¹⁷¹ to G¹⁷³, T²¹⁴ to R²²¹, T²⁸⁸ to R²⁹⁴, G³³⁶ to A³³⁸, A³⁵⁷ to V³⁶², G³⁹⁷ to G⁴⁰², and T⁴⁵⁶ to N⁴⁶⁸, of high surface probability.

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FIG. 5. Proposed topology of $beta$ ⁴³ in the outer membrane. According to the secondary structure prediction, $beta$ ⁴³ is composed of 18 amphipathic $beta$ strands with 11 to 17 amino acid residues per strand. Amino acids in amphipathic $beta$ -sheet structure are indicated by diamonds. Amino acids in boldface diamonds are hydrophobic and face the lipid phase of the outer membrane, while hydrophilic side chains facing the interior pore of the molecule are shown in lightface diamonds. The transmembrane segments are interrupted by large extracellular loops and shorter periplasmic loops. The $beta$ -barrel structure is completed by interaction of the first transmembrane strand with the last antiparallel C-terminal strand.

agn43 homologues in other members of the family Enterobacteriaceae. To assess the presence of agn43 homologues in other members of the Enterobacteriaceae, Southern hybridization experimentswere conducted on BamHI- and EcoRI-restricted DNA isolated fromthe Shigella, Salmonella, Enterobacter, Klebsiella, Edwardsiella,Erwinia, Proteus, and Serratia strains listed in Table 1. However,the only hybridizing signal detected with the $alpha$ ⁴³-specific 1,150-bp gene probe was that arising from control E.coli ML308-225 DNA. Even after prolonged exposure, no signal couldbe detected from the other enterobacterial DNA preparations, indicatingthat these strains do not possess genes with strong nucleotidesequence homology to agn43 of E. coli.

Involvement of OxyR and Dam in Ag43 phase variation. To examine the roles of global regulatory proteins in the expression of Ag43, a variety of E. coli derivatives carrying definedmutations in genes encoding a range of well-documented regulatoryproteins were screened (together with parental strains [Table1]) by immunofluorescence for the presence of Ag43. Subsequently,these same mutations were transduced into control strain ML308-225.Analysis of the resulting transductants containing deletions inthe hns, hupA, hupB, crp, cya, mbf, gyrA, gyrB, fis, topA, andrpoS genes by immunofluorescence microscopy and colony immunoblottingrevealed that all retained the ability to undergo reversible phasevariation (data not shown) in much the same manner as controlpopulations of E. coli ML308-225 (Fig. 6A and B). In contrast,neither Ag43 nor an anti- $alpha$ ⁴³ cross-reactive protein could be detected in either of two Dammethylase mutants (E. coli GM2929 or E. coli GM3819) or correspondingE. coli ML308-225 dam transductants (IRH12 and IRH13) when theywere screened by colony immunoblotting, Western blotting (Fig.6I) or immunofluorescence microscopy (Fig. 6C). These strainsall appeared to be locked off.

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FIG. 6. Expression of Ag43 in dam and oxyR mutants assessed by slide immunofluorescence microscopy using anti- $alpha$ ⁴³ antibodies (A to H) and by Western immunoblotting (I). (A) An Ag43⁺ (phase on) population of E. coli ML308-225 showing ~65% positive cells; (B) an Ag43 (phase off) population of E. coli ML308-225 showing ~5% positive cells; (C) dam derivative IRH13; (D) oxyR derivative IRH14; (E) IRH16 (IRH14[pAQ25]); (F) IRH17 (IRH14 [pGSO68]); (G) IRH18 (IRH14[pGSO69]); (H) IRH19. (I) Lanes A to H of the immunoblot contain cell lysates of strains shown in panels A to H, respectively. The position of the $alpha$ ⁴³ subunit is indicated. Previous work has documented that the presence of $alpha$ ⁴³ is indicative of the presence of both $alpha$ ⁴³ and $beta$ ⁴³ in equal stoichiometry.

The involvement of OxyR in expression of Ag43, suggested from a consideration of promoter sequence homologies (Fig. 1) andother data (33, 75), was confirmed following transductionof the $Delta$ oxyR::kan ( $lambda$ _Y2055 oxyS-galK) mutation from E. coli GS05and the $Delta$ oxyR::kan mutation from GS09 into E. coli ML308-225 (IRH14and IRH15). In contradistinction to the dam mutants, the oxyRmutants are firmly locked on for Ag43 expression, as judged bycolony blotting, Western immunoblotting (Fig. 6I), and slide immunofluorescencemicroscopy (Fig. 6D). Reintroduction into strain IRH14 of thewild-type oxyR gene on plasmid pAQ25 by CaCl₂ transformation generatedampicillin-resistant transformants displaying a restored phase-variablephenotype in which both Ag43⁺ and Ag43 variants could be detected (Fig. 6E), albeit the percentage ofpositive variants was lower than normal (~1%). Results similarto those for complementation with pAQ25 were obtained followingtranscomplementation experiments with pGSO68, which contains anoxyR gene carrying a mutation (C199S) in the redox center (Fig.6F). This mutation locks the molecule in the reduced form andprevents transcriptional activation of antioxidant genes associatedwith oxidative response. In contrast, similar experiments conductedwith pGSO69, which contains an oxyR gene carrying a mutation (A233V)that causes constitutive expression of antioxidant genes, failedto restore phase variation of Ag43, with the transformants retainingthe locked-on state of Ag43 expression observed for recipientstrains (Fig. 6G). Analysis of a strain (IRH19) containing mutationsin both the dam and oxyR genes indicates that the expression ofAg43 remains in the locked-on state (Fig. 6H).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The goals of this study were to identify the gene encoding Ag43, a major bipartite outer membrane protein which mediates autoaggregationand colony form variation in E. coli (33), to elucidate thelikely export and assembly mechanisms involved and to establishthe factors controlling the phase-variable expression of theantigen.

The strategy used to identify and sequence the agn43 gene (see Results) involved a knowledge of the N-terminal amino acidsequences of $alpha$ ⁴³, $beta$ ⁴³, and internal peptides $alpha$ ^a, $alpha$ ^b, and $alpha$ ^c, generated by V8 protease digestion of $alpha$ ⁴³. Three separate lines of evidence indicate that the 3,275-bpORF, identified by this strategy, encodes Ag43: (i) the aminoacid sequences determined empirically for the N termini of $alpha$ ⁴³, $beta$ ⁴³, and the three internal peptides can be found at anticipatedlocations within the predicted sequence of the primary translationproduct; (ii) the predicted M_r of $alpha$ ⁴³ (49,789) is consistent with that determined by electrospray massspectroscopy and gel filtration; and (iii) the predicted aminoacid compositions of the two subunits agree with those determinedempirically for the purified subunits (18).

The autotransporters, a family of proteins from gram-negative bacteria, utilize the recently designated type IV secretionsystem to reach the extracellular milieu. The secretion systemis intimately linked to the unifying structure possessed by theseproteins which, in general, comprises an N-terminal leader sequence,a mature protein ( $alpha$ ) which is translocated across the outer membrane,and a C-terminal ( $beta$ ) domain which forms a $beta$ -barrel pore to allowtranslocation of the mature protein (32). On the basis of aminoacid sequence similarities and of several structural commonalities,it appears that Ag43 belongs to the autotransporters. Thus, theagn43 gene encodes a precursor of 107 kDa which must be processedto the mature bipartite outer membrane complex by at least twocleavage events. Cleavage by a signal peptidase after A⁵² is presumed since (i) this residue immediately precedes the sequencecorresponding to the N terminus of mature $alpha$ ⁴³ and (ii) the upstream sequence shares many of the primary structuralfeatures characteristic of a general secretory pathway (GSP) peptide.Interestingly, the Ag43 signal sequence contains a 27-residueN-terminal extension showing striking sequence similarities withN-terminal extremities of a number of autotransporter proteinsand the HMW (high-molecular-weight) proteins of H. influenzae.The presence of a common motif upstream from the classical signalsequences suggests that this region might have a particular function,perhaps in targeting and export of these outer membrane proteinsor in induction of correctfolding.

Final expression of Ag43 on the cell surface as the mature 1:1 complex (predicted M_r of 101,431) composed of the 495-amino-acid $alpha$ ⁴³ subunit and a 492-amino-acid $beta$ ⁴³ subunit (M_r of 51,642) also requires posttranslational cleavageof the precursor protein between residues D⁵⁴⁷ and P⁵⁴⁸. This could be effected by a membrane-bound protease other thanOmpT, OmpP, or DegP (32, 40) or by an autoproteolytic event.The latter explanation is more attractive especially in view ofthe demonstration of a consensus sequence for an aspartyl proteaseactive site (30) and the observation that retroviral aspartylprotease is encoded as a segment of a polyprotein precursor andis involved in the correct maturation of the polyprotein by autocleavage(64). However, it should be recognized that (i) autoprocessinghas not been convincingly demonstrated in vitro for Ag43 or indeedseveral other autotransporters (see reference 32 for a recentreview) and (ii) the aspartyl protease active site of $alpha$ ⁴³ may have an additional or alternative functional role in cleavageof an as yet unidentified hostsubstrate.

One of the most striking features of autotransporters is the ability of the C-terminal domain to form, within the outer membrane,a $beta$ -barrel pore composed of amphipathic antiparallel $beta$ sheets,through which the N-terminal ( $alpha$ ) domain is secreted. Consistentwith the proposal that Ag43 is an autotransporter is the secondarystructural prediction that the $beta$ ⁴³ domain forms a pore of 18 amphipathic $beta$ sheets. The lengths ofthese predicted $beta$ strands (10 to 16 residues) are in good agreementwith the sizes of $beta$ strands identified in the OmpF and PhoE porinstructure (38). It should be noted that Loveless and Saier havealigned the autotransporter $beta$ domains and have predicted thatall autotransporters possess 14 conserved nine-residue $beta$ strands(47). However, this analysis did not include Ag43, whose unusuallylong $beta$ domain ( $beta$ ⁴³) shows no significant homology with any other autotransporter.Additional evidence that $beta$ ⁴³ forms a $beta$ barrel is indicated by the fact that $beta$ ⁴³ possesses three terminal residues (VTF) which are observed insimilar positions in the $beta$ domains of other autotransporters andwhich are supposedly involved in targeting of the proteins tothe outer membrane (32).

A number of outer membrane proteins and bacterial surface structures have been shown to be phase variable. In most cases,the precise biological significance of phase variation remainsspeculative. However, the most likely role is to provide the organismwith a strategy to survive and persist in a particular ecologicalniche (26, 27). An important feature of previous studies wasthe unequivocal demonstration that Ag43 undergoes reversible phasevariation at frequencies similar to those observed for other phase-variablesystems (56). It is clear from the present study that Dam playsa critical role in phase variation of agn43 since dam mutantsproduce no detectable levels of Ag43, as judged by a variety ofcriteria. Dam binds to GATC sequences and methylates adenosineat the N⁶ position. Most of the estimated 18,000 GATC sites in E. coliare methylated by Dam in this fashion (31). However, a numberof these have been shown to be differentially protected from methylationand that such protection is involved in regulating transcriptionof certain genes. This is the case with pap, which is controlledby Dam and Lrp (31, 74). However, the mechanisms of regulationof the pap and agn43 genes are quite distinct inasmuch as OxyRand not Lrp appears to act as the methylation blocking factoraffecting expression of Ag43. Thus, mutants lacking a functionalgene product constitutively express Ag43 and complementation ofthe oxyR mutation reinitiates the on $left-right-arrow$ off switch. The fact thatthe mutagenized oxyR gene (C199S) restores phase variation ofAg43 in complementation experiments, in a manner similar to thatof the wild-type gene, suggests that OxyR may have to be in thereduced form to inhibit agn43 transcription. In contradistinctionto the above, reintroduction of an oxyR gene carrying an A233Vmutation does not lead to restoration of phase variation. Themutated alanine residue (A²³³) is located in a C-terminal region which shows homology withother LysR-type transcriptional regulators and which may be involvedin contact with RNA polymerase and/or in the multimerization ofOxyR (44, 73). Thus, a multimerized OxyR may be required toprevent Ag43transcription.

Based on the extensive nucleotide homology present in the regulatory regions agn43 and other genes (oxyR and mom) known tobe negatively regulated by OxyR, one can predict an OxyR bindingregion upstream of the agn43 gene and extending between positions $-$ 95 and $-$ 49. Analysis of the OxyR footprint of the mom and oxyRloci indicates that the essential protein-DNA contacts are madewith the first 5 bp of the protected region, covering the firstGATC site in mom (13). However, analyses of the mom promoterregion have indicated that methylation of all GATC sites by Dammethylase is required for successful transcription of the momgene (39, 63). Of particular note in this respect was theobservation of three GATC sites in the putative promoter regionof the agn43 gene with a spatial distribution almost identicalto that observed in the mom promoter region. This suggests thata similar methylation pattern is required to allow transcriptionof the agn43 gene and that all sites have to be methylated toprevent binding of OxyR to the agn43 promoter. No GATC sites arepresent in the oxyR promoter region, an observation consistentwith the fact that DNA methylation is not involved in regulatingOxyR expression. The presence within the mom and agn43 regulatoryregions of 7-bp (AATAACC) and 6-bp (CGATTA) homologous sequences(corresponding to the extremities of the MuC binding domain ofmom [13]) suggests that another protein apart from OxyR andperhaps analogous to MuC may be required for agn43transcription.

In summary, the evidence presented here strongly suggests that Ag43 is an autotransporter whose phase-variable expressionis transcriptionally regulated by DNA methylation and by OxyR.Based upon analysis of mutants and upon sequence comparisons,it is proposed that OxyR may act as a repressor of Ag43 transcriptionby binding to unmethylated GATC sites in the regulatory regionof the gene and that methylation of these sites prevents OxyRbinding. Although analogous to the system involved in regulatingexpression of the mom gene of phage Mu, the phase variation mechanismproposed for agn43 is, to the best of our knowledge, a novel onein bacteria and one which is amenable to direct testing, e.g.,by mutation of critical GATC sequences and by in vitro and/orin vivo footprintanalysis.

	ACKNOWLEDGMENTS

This research was supported in part by grant HRB 32-91 from the Health Research Board ofIreland.

We thank James P. Nataro for helpful review of the manuscript and G. Storz for the kind gift of strains. Many thanks go toMary Meehan for her patience, help, expertise, and scientificdiscussions.

	FOOTNOTES

^* Corresponding author. Present address: Center for Vaccine Development, 685 W. Baltimore St., Baltimore, MD 21201. Phone: (410)706-7376. Fax: (410) 706-6205. E-mail: ihenders{at}umaryland.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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