Curli Fibers Are Highly Conserved between Salmonella typhimurium and Escherichia coli with Respect to Operon Structure and Regulation

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J Bacteriol, February 1998, p. 722-731, Vol. 180, No. 3
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Curli Fibers Are Highly Conserved between Salmonella typhimurium and Escherichia coli with Respect to Operon Structure and Regulation

Ute Römling,¹^,^* Zhao Bian,¹ Mårten Hammar,¹ Walter D. Sierralta,² and Staffan Normark¹

Department of Bacteriology, Microbiology and Tumorbiology Center, Karolinska Institutet, S-17177 Stockholm, Sweden,¹ and Max-Planck-Institut für Experimentelle Endokrinologie, D-30603 Hannover, Germany²

Received 27 August 1997/Accepted 12 November 1997

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Mouse-virulent Salmonella typhimurium strains SR-11 and ATCC 14028-1s express curli fibers, thin aggregative fibers, at ambienttemperature on plates as judged by Western blot analysis and electronmicroscopy. Concomitantly with curli expression, cells developa rough and dry colony morphology and bind the dye Congo red (calledthe rdar morphotype). Cloning and characterization of the twodivergently transcribed operons required for curli biogenesis,csgBA(C) and csgDEFG, from S. typhimurium SR-11 revealed the samegene order and flanking genes as in Escherichia coli. The divergenceof the curli region between S. typhimurium and E. coli at thenucleotide level is above average (22.4%). However, a high levelof conservation at the protein level, which ranged from 86% aminoacid homology for the fiber subunit CsgA to 99% homology for thelipoprotein CsgG, implies functional constraints on the gene products.Consequently, S. typhimurium genes on low-copy-number plasmidswere able to complement respective E. coli mutants, although notalways to wild-type levels. rpoS and ompR are required for transcriptionalactivation of (at least) the csgD promoter. The high degree ofconservation at the protein level and the identical regulationpatterns in E. coli and S. typhimurium suggest similar roles ofcurli fibers in the same ecological niche in the two species.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Proteinaceous, filamentous appendices on bacterial surfaces, called fimbriae or pili, enable the bacterial cell to make contactwith inanimate surfaces and eukaryotic or prokaryotic cells. Tightcontact, called adherence, precedes, e.g., colonization of surfacesand invasion of eukaryotic cells by the bacteria. Fimbriae arebest studied in the family Enterobacteriaceae, particularly inEscherichia coli and Salmonella enterica (49), in the contextof pathogen-host interactions (44). Related species, subspecies,and even particular strains can have a specific set of fimbrialgenes which are often located on pathogenicity islands on thechromosome or on plasmids (28, 31, 43, 45). The need forflexibility in the strategy of adhesion in order to overcome thehost immune system, for example, has also led to a variabilityin fimbrial genes derived from a common ancestor. The immunogenicand adhesive properties of these fimbriae, which can be encodedeither by the fimbrial subunit gene, as in the case of K88 fimbriae,or by separate genes, as in the case of the Pap pili, can be exchangedas gene cassettes in the context of a common frame (45). Therefore,fimbrial genes often do not appear to fit the phylogenetic classificationof the bacterium but are shared by more distantly related organismsoccupying the same ecological niche (45, 63).

Most of the fimbriae identified in Salmonella enterica subsp. enterica serotype Typhimurium (in this paper, referred to asS. typhimurium) have been described only phenotypically; the fewwhose genes have been cloned and sequenced (6, 15, 16,28, 56) are unique to S. enterica or a subset of its subspecies(5, 56). However, curli fibers, thin aggregative fibers,seem to be present and expressed in almost all Salmonella spp.and E. coli (5, 17, 23) and maybe also in other Enterobacteriaceae,such as Shigella, Citrobacter, and Enterobacter spp. (23). Sofar, two nomenclature systems exist (20, 34). The genes forcurli biogenesis (csg) in E. coli are called agf (thin aggregativefibers) in Salmonella enteritidis. For convenience, we use onenomenclature system in this communication.

Curli fibers detected, for example, on S. typhimurium strains causing acute salmonellosis in pigeons (32) and on E. coliisolates causing bovine mastitis (54) mediate binding to fibronectin(54), a variety of other human serum and tissue matrix proteins(7, 54, 62), and the dye Congo red (CR) (18). In E. coliMC4100, two divergently transcribed operons, csgDEFG and csgBA(C),which are separated by a 513-bp intergenic region are requiredfor the biogenesis of curli fibers (34). Transposon insertionsin the csgD gene, which encodes a transcriptional regulator belongingto the LuxR family as identified by the sequence similarity ofthe DNA binding helix-turn-helix motif, completely abolished transcriptionof the csgBA operon (34). Assembled by the extracellular nucleation-precipitationpathway, the secreted fiber subunit CsgA is polymerized on thesurface-exposed nucleator CsgB (35), which, in addition, ispresent along the filament in minor amounts (8). CsgA and CsgBshow 49% similarity and contain repeat regions whose interactiontriggers polymerization of CsgA (8, 35). The outer-membrane-locatedlipoprotein CsgG is required to protect CsgA and CsgB from proteolysis(48). The roles of csgE and csgF are just beginning to be elucidated.csgE is required for the fibronectin and CR binding propertiesof curli fibers but does not significantly affect polymerizationof the fiber subunit (36). The nucleation function is impairedin a csgF mutant, in which CsgA is released into the growth medium(37). Curli expression in E. coli MC4100 and YMel is highlyregulated by environmental conditions; it is restricted to lowtemperature on plates containing medium with a low salt concentration.

The alternative sigma factor RpoS ( $sigma$ ^S) is a global regulator controlling the expression of a large number of genes during starvationand other stress conditions in E. coli (52) and S. typhimurium(26). rpoS-deficient S. typhimurium strains are impaired intheir virulence in the mouse model for typhoid fever (22, 26);the rpoS deficiency also seems to be the cause of attenuationof common laboratory derivatives of strain LT2 (65, 68). Transcriptionby the RNA polymerase containing $sigma$ ^S at different promoters can include complex interactions withadditional regulators (25). The stationary-phase-induced transcriptionof the genes for curli biogenesis is dependent on $sigma$ ^S in E. coli. It has not been resolved whether rpoS is needed onlyfor transcription from the E. coli csgD promoter or also affectsthe CsgD-dependent csgBA promoter (34). Absence of H-NS hasbeen shown to make at least the csgD promoter independent of rpoS,suggesting an efficient repression of rpoD-dependent transcriptionby hns (2, 34).

Increasing osmolarity has been shown to shut off expression of curli genes at the transcriptional level (53) but to increasethe levels of RpoS (42). Therefore, other regulators must alsoinfluence the transcription from the csgD and csgBA promoters.OmpR is a transcriptional regulator which was studied mainly forits role in regulating transcription of the outer membrane proteinsOmpF and OmpC in response to surrounding osmolarity sensed byEnvZ in E. coli (55). Besides OmpF and OmpC, a tripeptide permease(TppB) is known to be regulated by OmpR in S. typhimurium (30).ompR mutants of S. typhimurium are attenuated in vivo (24) andunable to kill macrophages in vitro (47). ompR has been reportedto be required for transcriptional activation of both the csgBAand the csgDEFG promoters in E. coli (40); however, no experimentaldata have been reported so far.

In this paper, we report the cloning and characterization of the two operons for curli biogenesis from S. typhimurium SR-11.The highly conserved genes displayed the same arrangement in thesame chromosomal context as in E. coli. Consequently, S. typhimurium-derivedgenes on plasmids could functionally replace their E. coli counterparts,although not always to the wild-type levels. Regulation of curlibiogenesis in S. typhimurium SR-11 and ATCC 14028-1s was reminiscentof E. coli MC4100 and YMel. Curli biogenesis was restricted toambient temperature on plates, and transcription from the csgDEFGand csgBA promoters required rpoS and ompR. The conservation ofgenes and of the regulation pattern implies an important roleof curli fibers in the lifestyle of E. coli and Salmonella spp.in the same ecological niche.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Bacterial strains, plasmids, and growth conditions. Bacterial strains and plasmids used and constructed in this study are given in Tables 1 and 2, respectively. In the beginning,S. typhimurium SR-11 was used for the analysis of curli biogenesis.However, the initial lack of tools for genetic analysis led toa subsequent shift to strain ATCC 14028-1s, a virulent derivativeof the well-characterized LT2 strain. Curli expression in E. coliand S. typhimurium was monitored by growth on solid Yesca (35)and Luria-Bertani (LB) medium without salt, respectively. Mediawere supplemented with CR (40 µg/ml) and Coomassie brilliant blue(20 µg/ml) to judge colony morphology and color (34, 35).However, CR slightly inhibits the growth of S. typhimurium; therefore,the colony morphology develops later than on medium without CR.Recombinant clones were grown on LB medium supplemented with recommendedconcentrations of antibiotics (4), if required.

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TABLE 1. Bacterial strains used in this study

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TABLE 2. Plasmids used and constructed in this study

DNA techniques. Isolation of plasmid, cosmid, and chromosomal DNAs and all enzymatic manipulations (restriction digestion, ligation, phosphorylation,and PCR) were carried out by standard protocols (4, 58) withenzymes from Boehringer Mannheim or Biolabs. Southern blottingwas done as described previously (57). Individual PCR fragmentswere purified with a Quiaquick PCR purification kit (Quiagen);otherwise, a Geneclean II kit (Bio 101, Inc.) was used after electrophoresis.After polyethylene glycol precipitation (1), plasmids weresequenced with a Cycle Sequencing Ready Reaction kit (Perkin-Elmer).All sequence analyses were performed with the Genetics ComputerGroup package, version 8 or 9 (GCG, University of Wisconsin).

Cloning of the genes for curli biogenesis from S. typhimurium SR-11. The curli genes from S. typhimurium SR-11 were cloned in the following way. First, a DNA fragment downstream of the csgC genewas sought. Therefore, plasmid pCurli, containing a 3.1-kb HindIIIfragment (analogous to the fragment described in reference 17)from the non-curli-producing strain S. typhimurium SL2965 in pUC18,was integrated into the chromosome of a polA2 derivative of strainLB5010. After determination of appropriate restriction sites byhybridization with the vector, genomic DNA isolated from an integrantwas cut with PstI and ligated under conditions favoring the intramolecularreaction (pMU1). A HindIII/PstI digest with subsequent subcloningdepleted pMU1 from any DNA fragments containing curli sequences(pMU2).

As the second step, a resistance marker was placed downstream of csgC. The 6.6-kb HindIII/PstI fragment of pMU2 was clonedinto pMAK705 (pMU3a), and a Km^r cassette was introduced into a single NsiI site (pMU3b-1). TheKm^r marker was placed on the chromosome of SR-11 by a procedure describedbelow (see "Strain construction"), thereby creating the zcg-101::Km^r allele on the chromosome.

For cloning of the curli operons, after the position of the fragment containing the curli genes and the Km^r marker was checked by Southern hybridization of a PstI-digestedchromosomal DNA, the DNA fragments of respective size were isolatedfrom a gel by the Freeze-Squeeze method (66) and ligated withPstI-cut pLAFR3. The partial cosmid library was packed (GigapackIII Gold; Stratagene) and amplified in E. coli XL1 Blue MR inliquid culture with kanamycin resistance as an additional selectionmarker. The cells were plated for individual colonies to be examinedfurther, and subsequently one cosmid clone (pMU4) which complementedHLO7 [ $Delta$ (csgG-csgC)] was chosen for sequencing. Sequence identitybetween SR-11 and ATCC 14028-1s was confirmed for csgD and theintergenic region.

Strain construction. Phage P22 HT105/1 int-201 (60) was used for transduction of LT2 strains and SR-11 according to the recommended protocol(13, 50). In order to detect lytically infected cells, LT2strains were streaked on green plates. Lysogens were detectedby streaking LT2 derivatives against phage H5. Since SR-11 doesnot support the propagation of P22, the purification procedureswere skipped. DNA translocation into bacteria was also done byusing competent cells (41), electrocompetent cells (9), andconjugation by triparental mating. A deletion in csgA was constructedas follows. Primers CSGBD (dACGAAAGCTTGCACTGCTGTGGGTTG [HindIIIrestriction site underlined]), CSGA1 (dCGTCTGCAGGATTGCTGCGAATGCTGC[PstI site underlined]), CSGA2 (dCGTCTGCAGTGGAACGCTAAAAACTC [PstIsite underlined]), and CSGC (dCGAGGATCCGGCCATTGTTGTGATAAA [BamHIsite underlined]) were used to create fragments PCR1 (CSGBD $left-right-arrow$ CSGA1)and PCR2 (CSGA2 $left-right-arrow$ CSGC). After restriction digestion, PCR1 and PCR2were directly cloned into pMAK700 cut with HindIII and BamHI,which resulted in plasmid pUMR2b. Cloning of the Km^r cassette of pUC4K into the single PstI site of pUMR2b resultedin pUMR2c-1. The plasmids were passaged through LB5010 and finallyelectroporated into S. typhimurium wild-type strains. After propagationof the strains at 28°C, the temperature was shifted to 44°C inorder to integrate the pMAK derivative into the chromosome. ForpUMR2c-1, for which a selectable marker was available, individualcolonies were streaked on chloramphenicol and kanamycin platesin order to screen for a double crossover event. With pUMR2b,10 individual integrants were selected and incubated at 28°C inorder to resolve the plasmid again. Strains harboring a deletionwere selected by their white color on CR plates. All constructswere checked by Southern hybridization and/or PCR. A deletionin ompR was created in the same way. The ompR primers OMPR1 (dTGGAAGCTTTTGTTTGAGTGTTTCGT[HindIII site underlined]), OMPR2 (dCTTAGATCTCTCTTGCATTGTCTGT[BglII site underlined]), OMPR3 (dCCTGAGATCTGTCTTTGTACCGGAC [BglIIsite underlined]), and OMPR4 (dGGCTCTAGAACTTCTACCTGAAACCAG [XbaIsite underlined]) were selected on the basis of sequence X12374(EMBL database [46]). After restriction digestion, PCR fragmentsPCR3 (OMPR1 $left-right-arrow$ OMPR2) and PCR4 (OMPR3 $left-right-arrow$ OMPR4) were cloned into XbaI/HindIII-digestedpMAK705, yielding pUMR7a. Cloning of the ampicillin resistancegene from pWKS30 (BglII/BamHI digested) into the single BglIIsite resulted in pUMR7b-2.

Plasmid construction. Individual genes from the curli operon were cloned into low-copy-number vector pWSK29 or pWSK30. csgA was amplified by usingprimers CSGB2 (dCGTCTGCAGTGCAGAAACAGTCGCA [PstI site underlined])and CSGC (dCGAGGATCCGGCCATTGTTGTGATAAA [BamHI site underlined]),and for csgB primers CSGBD (HindIII) and CSGA1 (PstI) were used.The restriction sites at the primer ends were used to clone thefragments into pWKS30, yielding plasmids pCSGA and pCSGB, respectively.csgD was amplified with primers SP2 (dTTTCTCTTTCTGGATAATGGG) andSP5 (dTGTTTAACACGCATGACAGC), csgE was amplified with primers SP5and SP9 (dCCTGACGATTATCCCTACC), and csgF was amplified with primersSP6 (dGATTGTTAACCGACCATACC) and SP17 (dGCAGGTAAGTGCGTCAAATC).The ends of the PCR fragments were treated with Klenow polymerase.Primer pair SP2-SP5 was digested with EcoRI, SP5-SP9 was digestedwith BstYI, and SP6-SP17 was digested with EcoRI. SP2-SP5 andSP5-SP9 were cloned into pWSK29 digested with the respective restrictionenzymes, yielding pCSGD and pCSGE, respectively, and SP6-SP17was cloned into pWKS30 in order to create pCSGF. The gene sequencesfor csgEFG were also amplified by using primers CSGD2 (dTGGATGCATACCCAGGCAGTTTCATGG[NsiI site underlined]) and SP21 (dGCTTTGTCGTATTCATCAGG) and clonedinto pWSK29, yielding pCSGEFG.

RNA techniques. Total RNA was prepared from 10 mg of S. typhimurium cells by the hot-phenol method. Cells were resuspended in 300 µl of 0.3M sucrose-0.01 M sodium acetate (pH 4.5) and the same amount of0.01 M sodium acetate (pH 4.5)-2% sodium dodecyl sulfate (SDS).After being mixed with an equal amount of hot acidic phenol, thecells were incubated at 65°C for 5 min. The extraction was repeatedonce with hot acidic phenol and twice with cold acidic phenol.After precipitation, the remaining DNA was digested with 10 Uof RQ1 DNase (Promega) for 30 min in 0.05 M Tris (pH 7.5)-0.05M NaCl-0.01 M MgCl₂, and phenol-CHCl₃ extraction was carried outtwice. The concentration of the RNA dissolved in water was determinedspectroscopically. A 10-µg sample of RNA was loaded on a 1.2%morpholine propanesulfonic acid (MOPS)-formaldehyde gel (4)which was run for 4 h at 4 V/cm with a 0.24- to 9.5-kb RNA ladder(Life Technologies) as a standard. After the gel was soaked inH₂O twice (20 min each), the RNA was transferred to an AmershamHybond-N membrane overnight by capillary blotting with 20× SSC(1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate) (4). Single-strandedprobes complementary to the RNA template on the blot were constructedby an asymmetric PCR with primers CSGB2 and SP2 on symmetric PCRtemplates spanning the region of the csgA (primers CSGB2 and SP8[dCTAAATTAATACTGGTTGA]) and csgD (primers SP2 and SP24 [dTAACTCTGCTGCTACAATCC])genes, respectively, and labeled with the RadPrime Labelling System(Life Technologies) using 30 µCi of [ $alpha$ -³²P]dCTP (3,000 Ci/nmol; Amersham). Hybridization (using less than6 ng of probe per ml) and washing of blots were carried out accordingto standard procedures (4). The quality of transfer to themembrane was checked by probing with part of the 16S RNA sequencefrom plasmid pKK3535 (11) cut by HindIII. Signals were analyzedwith a radioisotope imaging system (PhosphorImager 445SI; MolecularDynamics) and quantified by integration over all bands detectedby a single probe.

For primer extension, 10 µg of RNA and 2 pmol of primer PEXD1 (dTGACAGATGTTGCACTGCTG) were diluted in 9 µl of 1× avian myeloblastosisvirus (AMV) reverse transcriptase buffer (Boehringer Mannheim).A 10-pmol amount of PEXD1 had been labeled with 30 µCi of [ $gamma$ -³²P]ATP (3,000 Ci/nmol; Amersham) by use of 10 U of polynucleotidekinase (Boehringer Mannheim). After incubations at 95°C for 5min, 67°C for 3 min, and 50°C for 5 min, 5 U of AMV reverse transcriptase(Boehringer Mannheim) and 5 mM deoxynucleoside triphosphates (Pharmacia)were added, and primer extension was performed at 50°C for 1 h.The reaction mixture, containing 5 µl of formamide loading buffer,was heated at 95°C for 5 min and cooled on ice, and 6 µl was analyzedon a 7% denaturing polyacrylamide gel (4). A sequencing laddergenerated with a T7 Sequencing kit (Pharmacia) using the PEXD1primer and pUMR10-7 as template DNA was run as a standard.

Western blotting. Bacteria were grown for 48 to 60 h on plates at 28°C and for 17 to 24 h at 37°C. In order to depolymerize the curli fiberinto subunits, the cells have to be treated with strong acids(19). After resuspension of the cells in 100 µl of 99% formicacid and incubation for 10 min on ice, the liquid was removedby evaporation in a Speed Vac. The pellet was resuspended in 200µl of SDS-polyacrylamide gel electrophoresis sample buffer (4),while 3 µl was loaded on a gel (15% separating gel with a 4% stackinggel, with a double concentration of buffer used in the separationgel and the running buffer). Proteins were transferred to polyvinylidenedifluoride membranes (Immobilon P; Millipore). The membranes wereblocked and incubated with a 1:4,000 dilution of an anti-E. coliCsgA antiserum (34); a secondary goat antibody against rabbitimmunoglobulin G conjugated with horseradish peroxidase was usedfor detection according to the protocol of the manufacturer (BoehringerMannheim).

Electron microscopy. Bacteria were grown on plates under the same conditions used for Western blotting. A concentrated bacterial suspension inwater was allowed to adhere to a carbon-coated copper grid for2 min. The liquid was removed by blotting, and staining was carriedout for 30 s with 0.7% ammonium molybdate-150 µg of bacitracinper ml. The samples were examined with a Zeiss microscope at 80kV.

Nucleotide sequence accession number. The nucleotide sequence of the genes for curli biogenesis has been submitted to the EMBL data library under accession no.AJ002301.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Detection of curli expression in S. typhimurium SR-11 and ATCC 14028-1s on plates. The mouse-virulent strains SR-11 and ATCC 14028-1s exhibited distinct colony morphologies when grown on CR plates at differenttemperatures; a white and smooth colony morphology was seen at37°C, while a red, dry, and rough colony morphology was displayedat 28°C (Fig. 1). We called the two morphotypes saw₃₇ and rdar₂₈,respectively. Morphotypes similar to the rdar morphotype werepreviously described for E. coli MC4100 and YMel (34) and Salmonellaenteritidis (18) and shown to be tightly linked to the expressionof a thin aggregative fiber called curli fiber or SEF 17, respectively.

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FIG. 1. Colony morphology and color of S. typhimurium ATCC 14028-1s and SR-11 and their respective derivatives. (A) Cells grown at 28°C on LB medium plates without salt containing the dye CR. SR-11 and ATCC 14028-1s (here shown as the Nal^r derivatives UMR3 and UMR1, respectively) developed a rough colony morphology with a dry surface and showed a deep red color by binding the dye CR, the rdar morphotype. The strains with deletions in csgA (MAE1, MAE2, and MAE5) were also rough but had a shinier surface. Binding of the dye CR led to a pinkish color of the colonies (the pdar morphotype). The strains with deletions in rpoS (MAE40 and MAE29) and ompR (MAE46 and MAE34) were white. (B) The same strains as in panel A but grown at 37°C. All cells were white and smooth, the saw morphotype.

Both S. typhimurium strains were analyzed for expression of curli fibers by immunoblot analysis using a polyclonal antiserumagainst CsgA (34), detection of fibers on the surface of thecells by electron microscopy, and gene replacement of csgA, thefiber subunit gene, the sequence of which was taken from the onepublished for S. enteritidis (17). In accordance with the colonymorphology, a signal for CsgA was detected only at 28°C in bothstrains (Fig. 2). By electron microscopy, an abundance of fiberswas detected at 28°C (Fig. 3), while very few were occasionallyseen at 37°C (data not shown). However, electron micrographs mightnot reflect the actual amount of curli fibers present on the cellsat 28°C, since the cells clump together and only a fraction ofthem can be released from the tight extracellular matrix. Replacementof the curli subunit gene csgA with a Km^r cassette (MAE1 and MAE2) or an in-frame deletion of csgA (MAE5)abolished the rdar₂₈ phenotype. Instead of rdar, mutant strainsof SR-11 and ATCC 14028-1s, MAE2 and MAE1, respectively, and MAE5displayed a pink colony which developed a delayed roughness, thepdar₂₈ morphotype (Fig. 1). This phenotype seems to be more commonin Salmonella spp., since it was also described for S. enteritidis27655-3b after gene replacement of csgA (17), whereas E. coliMC4100 and YMel gave white colonies after knockout of the fibersubunit gene (34, 35). All these experiments showed that thecurli fibers are expressed in SR-11 and ATCC 14028-1s in a temperature-and surface-dependent manner; therefore, the curli operon fromSR-11 was cloned and characterized (see Materials and Methods).The organization of the two divergently transcribed csg operons,csgDEFG and csgBAC, is shown in Fig. 4.

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FIG. 2. Western blot analysis of fiber-derived CsgA from whole cells grown at 28 and 37°C. The cell pellets were immediately resuspended in SDS sample buffer ( $-$ ) or treated with formic acid (+) as described in Materials and Methods. Minor signals for the fiber subunit which could vary in their intensities were regularly found in the slot (s) and in the gel corresponding to a dimer (d), while the major signal was consistent with the running behavior of a monomer (m). SR-11 and ATCC 14024-1s showed a signal for CsgA only at 28°C and not at 37°C. csgA knockouts did not show any signal at all. Lanes: 1, SR-11; 2, MAE2; 3, ATCC 14028-1s; 4, MAE1.

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FIG. 3. Electron micrograph of negatively stained ATCC 14028-1s cells grown at 28°C on LB agar without salt. The cells which are surrounded by a thick layer of curli fibers show a different cell morphology. Bar, 1 µm.

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FIG. 4. Organization of the csg region on the S. typhimurium SR-11 chromosome. A restriction map containing sites important for the cloning and localization of the csg region is shown. The positions of the genes required for curli biogenesis, csgDEFG and csgBAC (boxes), the position of the transcriptional start sites and the direction of polymerization (flags), and the position of the promoter (circle) are indicated. Experimentally confirmed RNA full-length transcripts (arrows above gene boxes) and open reading frames for which transcriptional analysis had not been carried out or for which no transcript had been detected so far (boxes with arrowheads inside) are also shown. The DNA fragments used as probes in RNA transcript analysis (dotted lines), primers used for the PCR amplification of DNA fragments (arrowheads above dotted lines), and subclones used to complement E. coli isolates with mutations in the csg genes (pCSGA, pCSGB, pCSGD, pCSGE, pCSGF, pCSGG, and pCSGEFG) (bars with small arrows indicating the transcription from the lacZ promoter) are indicated. B, BstYI; E, EcoRI; H, HindIII; N, NsiI; P, PstI; S, SacI.

Transcriptional analysis of the two curli operons. Primer extension analysis of the csgD operon revealed the nucleotide G 174 bp upstream of the putative translation start ofthe csgD transcript as the transcription start site in S. typhimuriumATCC 14028-1s (Fig. 5). Transcription initiation of the E. colicsgD operon takes place 2 bp further upstream (34). A signalwas obtained only when RNA isolated from cells grown on platesat 28°C, and not at 37°C, was used. Primer extension analysisof the csgBAC operon confirmed previous results (2, 17; alsodata not shown).

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FIG. 5. Primer extension analyses for the determination of the transcriptional start site of the csgDEFG operon. RNA was prepared from strains UMR1 and MAE40 (the rpoS derivative of ATCC 14028-1s) grown at 28°C on plates, and primer extension was carried out as described in Materials and Methods. An extension product is seen for UMR1 but not for MAE40. Primer PEXD1, located 58 bp downstream of the csgDEFG start codon, was used for the extension reaction as well as for the sequencing reaction on pUMR10-7 as a template. The sequence derived from the PEXD1 primer on pUMR10-7 is complementary to the RNA template, so the coding strand is automatically shown. The transcriptional start site (asterisk) and bases belonging to the putative promoter sequences (boxed) are indicated.

In order to determine the expression state of both csg operons, analysis of the steady-state levels of the RNA transcriptsof csgD, the transcriptional regulator, and csgA, the fiber subunitgene, was carried out by Northern blot analysis (Fig. 6). By usinga probe encompassing the whole csgD gene, four major bands of2.3, 1.3, 0.9, and 0.7 kb which could correspond to the transcriptscsgDEFG, csgDEF, csgDE, and csgD (with theoretical sizes of 2.5,1.6, 1.2, and 0.8 kb, respectively) were detected; the csgA probehybridized to three bands of 0.9, 0.6, and 0.5 kb, as in S. enteritidis(17). Signals of the same intensity were detected for ATCC 14028-1sand SR-11 after the cells were grown at 28°C for 24 or 48 h onplates but not for cells grown at 37°C for 17 or 28 h. Therefore,detection of csgD and csgA transcripts is concomitant with theexpression of CsgA at 28°C, and transcripts are present long afterentrance into the stationary phase.

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FIG. 6. Northern blot analysis of RNA transcripts of the csg region using S. typhimurium ATCC 14028-1s and SR-11 grown on LB medium plates without salt at 28 and 37°C for different periods. Probes covering the whole csgD and csgA genes were used; their locations are indicated in Fig. 4. Lanes: 1, UMR3; 2, UMR1. The sizes of the bands detected by the respective probes are shown on the left, calculated by using a 0.24- to 9.5-kb RNA ladder (Life Technologies) as a standard. (A) Hybridization with the csgD probe; (B) hybridization with the csgA probe; (C) control hybridization with 16S RNA as described in Materials and Methods.

Comparative sequence analysis of the curli region. The csg genes are located at the same positions on the chromosomes of E. coli K-12 and S. typhimurium LT2 (26 centisomes [20]).In S. typhimurium, two divergently transcribed operons, csgBACand csgDEFG, flank a 521-bp intergenic region (Fig. 4), a situationas in E. coli MC4100 (34). The nucleotide sequences of the twospecies showed an identity of 77.6%, a value which is below theaverage sequence conservation of 84.4% (61). The overall G+Ccontents in S. typhimurium and E. coli are similar; however, singlegenes show some variability in G+C content conservation (Table3). The intergenic region between the transcriptional start siteshas a low G+C content and is the least conserved (71%) (Table3). However, the intergenic region has not homogeneously divergedbut can be subdivided into four regions. Only four nucleotidesubstitutions occurred in the 60 bp upstream of the transcriptionstart site of the csgD operon. The csgD promoter shares the characteristicsof promoters transcribed by $sigma$ ^D both in S. typhimurium and E. coli, with the E. coli $-$ 35 boxbeing closer to the consensus sequence. The region upstream ofthe csgD promoter has a very low G+C content (21.2%) which isidentical in S. typhimurium and E. coli, and a conspicuous peakof curvature at position $-$ 147 (data not shown) was found by calculationwith the DNase I-based parameters using the bend.it server (29).Sequence identity drops to 42.7% between 165 and 443 bp upstreamof the transcriptional start site of csgD. The csgB promoter hasa $-$ 10 box, which resembles more the proposed consensus sequenceof $sigma$ ^S than that of $sigma$ ^D (38). Two alternative $-$ 35 boxes have been found which bothsuggest an unusually wide spacing of 19 or 21 bp between the $-$ 35and $-$ 10 boxes. Some promoters whose transcription can be initiatedin the absence of specific $-$ 35 hexamer contacts contain an upstreamextension of the $-$ 10 element (10) by 5'-Tgn-3', a sequence whichwas not found at the csgB promoter.

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TABLE 3. Properties of the csg genes and surrounding open reading frames

The putative proteins encoded by the genes of the two operons showed variability in sequence conservation. With the exceptionof CsgC, whose role has not been unambiguously determined, theproteins for the fiber subunit, CsgA, and the nucleator, CsgB,displayed the lowest amino acid identities (74.8 and 82.1%, respectively).These values lie at the lower end of gene conservation betweenS. typhimurium and E. coli, which ranges from 100 to 74.3% aminoacid identity (61), but are surprisingly high when homologiesamong fimbriae, even of common origin within a species, are considered(45). In addition, the amino acid identities of CsgA, CsgB,and CsgC were 100% when the proteins of S. typhimurium SR-11 andS. enteritidis 27655-36 were compared (see reference 17 forfurther characterization of the genes).

The degree of conservation of the CsgD, CsgE, CsgF, and CsgG proteins between S. typhimurium and E. coli is high and liesbetween 89.5 and 96% amino acid identity (Table 3). The lipoproteinCsgG, which has a putative molecular mass of 30 kDa, was mostconserved and showed only conservative amino acid exchanges. Thehelix-turn-helix DNA binding motif of CsgD, the putative transcriptionalregulator of 25 kDa, is completely conserved between the two species.Classified according to the sequence similarity of the DNA bindingmotif, CsgD belongs to the LuxR family. The closest sequence homologyis to regulators belonging to a two-component sensory transductionsystem, such as DegU of Bacillus subtilis and NarP of E. coli.

Complementation of E. coli csg mutants with S. typhimurium genes. Considering the high homology of the Csg proteins between S. typhimurium and E. coli, functional complementation of gene productsseemed likely. In order to test this hypothesis, PCR-generatedgene fragments from S. typhimurium were cloned into the low-copy-numbervectors pWSK29 and pWKS30 so that transcription occurred fromthe lacZ promoter (see Materials and Methods). All E. coli csgmutants were white and, with the exception of MHR480 (the csgEmutant), produced no curli fibers. MHR261 (csgB2) and MHR426 (csgF4)secrete CsgA in a soluble form (35, 36), but the soluble formof the protein was not detected in the whole-cell preparationsused here (Fig. 7). Complementation was judged by the developmentof a red and rough colony morphology type and by Western blotsdetecting CsgA as an acid-sensitive polymer (Fig. 7 and Table4). As seen in Table 4, all S. typhimurium genes complementedthe respective E. coli csg mutants, although to different degrees.Single csgB, csgD, and csgE genes complemented the respectiveE. coli mutants to the wild-type phenotype. The csgA and csgFmutations could be only very poorly replaced by the copy on theplasmid. In the case of csgA, two signals of almost equal intensitywere seen on an overexposed Western blot, one of which has a slightlyhigher molecular weight than the wild-type signal and is mostlikely a premature form of CsgA (data not shown). In addition,the very low signal intensity could be explained by a lower specificityof the anti-E. coli CsgA antiserum against CsgA from S. typhimurium.MHR426, the csgF mutant used in this study, has a polar effecton csgG expression, leading to decreased amounts of CsgG (36).The reduced amount of CsgG might limit the full complementationof MHR426 by pCSGF, as occurs with the respective E. coli gene(36). Neither the vector control nor the csgA, csgD, csgE, andcsgF genes cloned in the direction which would allow transcriptionfrom the T7 promoter gave a change in the color of the coloniesor their morphology with respect to the wild type or in signalintensity of CsgA on Western blots (data not shown). We concludefrom the available data that interspecies complementation of thecsg genes is possible in principle.

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FIG. 7. Western blot analysis of the complementation of the E. coli csg mutants. Results for whole-cell preparations treated with formic acid are shown. The mutant ( $-$ ) and the mutant harboring the respective complementing plasmid (+) were run next to each other. Except for MHR480 ( $Delta$ csgE3), none of the E. coli mutants showed a CsgA signal derived from polymerized fibers. MHR261 (csgB2) and MHR503 (csgD6) were complemented to wild-type levels by using plasmids with the single genes. MHR426 (csgF4) was complemented to wild type only when a plasmid carrying csgEFG was used. Faint signals of CsgA were detected when pCSGA was introduced into MHR204 (csgA::Tn105).

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FIG. 8. Northern blot analysis of RNA transcripts from S. typhimurium ATCC 14028-1s and rpoS and ompR derivatives grown on LB medium plates without salt at 28 and 37°C. Probes covering the whole csgD and csgA genes were used; their locations are indicated in Fig. 4. Lanes: 1, UMR1; 2, MAE40 (rpoS); 3, MAE46 (ompR). The sizes of the bands detected by the respective probes are shown on the left, calculated by using a 0.24- to 9.5-kb RNA ladder (Life Technologies) as a standard. (A) Hybridization with the csgD probe; (B) hybridization with the csgA probe; (C) control hybridization with 16S RNA as described in Materials and Methods.

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TABLE 4. Complementation of E. coli csg mutants with S. typhimurium genes

Analysis of the effect of rpoS and ompR mutations on colony morphology and transcription from the csg promoters. For E. coli, it was demonstrated that transcription of the csgD and csgBA operon requires $sigma$ ^S. Transduction of the mutant rpoS allele from SF1005 into ATCC14028-1s and SR-11 gave white and smooth colonies, a saw₂₈ morphotype(Fig. 1). Transcriptional analysis with the csgD and csgA probeson RNA extracted from the rpoS mutant of ATCC 14028-1s (MAE40)grown at 28 and 37°C detected no signal for either probe (Fig.8). In addition, no extension product was seen in the latter strainby primer extension analysis (Fig. 5). Therefore, rpoS is alsorequired for transcription of the csg operons in S. typhimuriumstrains.

It is also known that ompR is necessary for transcription from both the csgBA and the csgD promoters in E. coli (40). AnompR mutant was constructed by introducing a deleted ompR genecarrying an Amp^r cassette instead of the major part of its open reading frameinto the chromosome of ATCC 14028-1s and SR-11 by double crossover,yielding strains MAE46 and MAE34, respectively (Table 1; seeMaterials and Methods). The ompR mutants were white at 28 and37°C (Fig. 1). No CsgA signal was detected for MAE46 in Westernblots (data not shown). Northern blot analysis of RNA extractedfrom strain MAE46 grown at both temperatures gave no signal forcsgD or csgA (Fig. 8). Since ompR was shown to be necessary forthe transcription of the csgD and csgBA promoters, the intergenicregion was examined for putative ompR binding sites. One nucleotidesequence which has one mismatch base pair to the recently proposedconsensus sequence for independent binding was found (39). Thissequence is centered at position $-$ 50.5 relative to the transcriptionalstart site of the csgD promoter. If this sequence is used forOmpR binding, it can be imagined that transcriptional regulationtakes place mainly at the csgD promoter. CsgD may then act uponthe csgBA promoter to initiate transcription there.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Although many fimbrial gene clusters have been isolated from Salmonella spp. and E. coli, variation in operon structure andgenes encoding regulatory control features of pili from the samestructural class suggests frequent remodeling of DNA sequencesdue to the necessity to respond flexibly to changing environmentalconditions and various host environments (49). In contrast tothis behavior of fimbrial operons, the operons for curli biogenesisembedded in the same context on the chromosome (reference 20and this study) are remarkably conserved between E. coli and S.typhimurium. In addition, the sequence similarities at the aminoacid level of all proteins in the operon, ranging from the fibersubunit CsgA (86%) to the transcriptional regulator CsgD (96%)and the lipoprotein CsgG (99%), are higher than the homologiesfor most functionally and sequentially related fimbrial gene products,even within a species (49, 51, 56). It is therefore suggestedthat the thin aggregative fibers in Salmonella be named curlifibers, as for the products of the homologous E. coli genes (csg)(59).

The sequence similarity at the amino acid level is reflected by the successful complementation of individual csg gene mutantsof E. coli by S. typhimurium genes. The S. typhimurium csgB genecould complement the homologous E. coli gene to wild-type levels,showing that the four-repeat structure consisting of 22-amino-acid-longputative $beta$ -strand-turn- $beta$ -strand-turn units (35) which are allrequired for organelle assembly (8) functions between the species.It can be imagined that interspecies exchange of organelle subunitscan occur in a natural environment where bacteria are tightlypacked, such as the gut flora. The consensus sequence for therepeat structure of CsgB was determined to be NLA-I-Q-GS-N-A-I-Q-G--,where the underlined amino acids show 100% conservation betweenS. typhimurium and E. coli. The consensus motif for CsgA, whichhas five 23-amino-acid-long units, is NS--T-TQYG-GN-AT-DQTAA-.There may be several reasons for the lack of complementation toa full wild type for some genes, such as functional restrictionof the proteins, imbalance of protein ratios, or instability ofthe RNA message created from the plasmid, which remain to be elucidated.Alternatively, polar effects of the csg mutations on downstreamgenes may prevent the full complementation to the wild-type phenotype.

The high degree of conservation at the protein level contradicts the low conservation at the nucleotide level. The nucleotidesequences encoding csgDEFG diverged more than average, and sodoes K_S (0.94 on the average), a value for the estimation of thenumber of synonymous substitutions per site (Table 3). csgE hasa K_S value of 1.5 and is therefore almost saturated with substitutions.The high rate of nucleotide substitutions could reflect the chromosomallocation of the csg operons proximal to the terminus of replication,where more nucleotide changes take place, and/or the low expressionstate of the genes from the csgDEFG operon (61). The high conservationof proteins could indicate a lack of selective pressures, suchas the immune response in a host, on the fibers or functionalconstraints on the macromolecules and their specificities, whichdo not tolerate an evolution which develops too far from a commonancestor (45).

The two csg operons are flanked by the same open reading frames as in the fully sequenced E. coli MG1655 strain (EMBL accessionno. ecae205, ecae206, and ecd740 to ecd742). The homologous ORF179ashowed the same ambivalent conservation scheme as the curli genes,low conservation on the nucleotide level and high conservationof the amino acid sequence (Table 3); the intergenic region betweencsgG and ORF179a showed no homology. Downstream of csgC, the nucleotidehomology already starts to decline at the end of csgC (the stopcodon has changed with respect to E. coli) to a level of 60%,which continues within ORF103.

Another fiber, type 1 fimbria, which seems to be present in all Salmonella species, shares morphological and adhesive propertieswith E. coli type 1 fimbria. However, the different location onthe chromosome in the two species and the high degree of sequencediversity and gene rearrangements (14), together with differentregulation schemes having no overlapping regulating factors, suggestthat these genes were acquired independently by S. typhimuriumand E. coli and subject to evolutionary pressures (45). Therefore,curli genes are the only fimbrial genes detected which were alreadypresent in a common ancestor of E. coli and Salmonella spp.

The regulation of the curli genes in S. typhimurium SR-11 and ATCC 14028-1s by temperature, rpoS, and ompR is identical tothat in E. coli MC4100 and YMel (2, 3, 34, 40, 53),implying that fiber expression responds to the same environmentalcues in general. The complementation to wild-type levels of theE. coli csgD gene by the respective S. typhimurium gene showsthat the recognition sites for the transcriptional activator arealso conserved between the species. The correspondence in regulationpattern in addition to gene conservation points to a similar oridentical function of the curli fibers in the two species in thesame ecological niche. The expression pattern on plates at lowtemperature and low osmolarity suggests a role for curli fibersprimarily outside a host, on surfaces. A participation of curlifibers in a bacterial network such as a biofilm (21) is possible,considering the adhesive nature of the fibers and the colony morphologyof cells. However, more environmental studies need to be performedbefore a firm role of curli fibers in biofilm formation can beconcluded.

	ACKNOWLEDGMENTS

We thank the following people for providing plasmids, strains and antibodies: D. G. Guiney for SF1005, S. R. Kushner for pWSK29and pWKS30, A. Lazdunski for pLAFR3, H. Loferer for HLO7, E. Morfeldtand S. Arvidson for anti-OmpA antiserum, and M. Rhen for 146,LB5010, and pCurli. We are grateful to H. Loferer for helpfultechnical advice.

U.R. was the recipient of a fellowship from the program "Infektionsbiologie" from the German Bundesministerium für Forschungund Technologie (BMFT). This work was supported by grants fromthe Swedish Medical Research Council (B96-16X-10843-03A) and theSwedish Natural Science Research Council and by an unrestrictedgrant for infectious disease research from the Bristol-Myers SquibbCompany to S. Normark.

	FOOTNOTES

^* Corresponding author. Mailing address: Karolinska Institutet, Microbiology and Tumorbiology Center (MTC), Box 280, S-17177Stockholm, Sweden. Phone: (46) 8-728-7409. Fax: (46) 8-342651.E-mail: ute.roemling{at}mtc.ki.se.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
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