Silencing and Activation of ClyA Cytotoxin Expression in Escherichia coli

doi:10.1128/JB.182.22.6347-6357.2000

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Journal of Bacteriology, November 2000, p. 6347-6357, Vol. 182, No. 22
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Silencing and Activation of ClyA Cytotoxin Expression in Escherichia coli

Marie Westermark,¹ Jan Oscarsson,¹ Yoshimitsu Mizunoe,² Jurate Urbonaviciene,¹ and Bernt Eric Uhlin¹^,^*

Department of Microbiology, Umeå University, S-90187 Umeå, Sweden,¹ and Department of Bacteriology, Graduate School of Medical Sciences, Kyushu University, Fukuoka 812-8582, Japan²

Received 8 May 2000/Accepted 21 August 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Cytolysin A (ClyA) is a pore-forming cytotoxic protein encoded by the clyA gene of Escherichia coli K-12. Genetic analysissuggested that clyA is silenced by the nucleoid protein H-NS.Purified H-NS protein showed preferential binding to clyA sequencesin the promoter region, as evidenced by DNase I footprinting andgel mobility shift assays. Transcriptional derepression and activationof a chromosomal clyA::luxAB operon fusion were seen under conditionsof H-NS deficiency and SlyA overproduction, respectively. In H-NS-deficientbacteria neither the absence nor the overproduction of SlyA affectedthe derepressed ClyA expression any further. Therefore, we suggestthat overproduction of SlyA in hns⁺ E. coli derepresses clyA transcription by counteracting H-NS.The cyclic AMP receptor protein (CRP) was required for ClyA expression,and it interacted with a predicted, albeit suboptimal, CRP bindingsite in the clyA upstream region. Site-specific alterations ofthe CRP binding site to match the consensus resulted in substantiallyhigher levels of ClyA expression, while alterations that werepredicted to reduce CRP binding reduced ClyA expression. Duringanaerobic growth the fumarate and nitrate reduction regulator(FNR) was important for ClyA expression, and the clyA gene couldbe activated by overexpression of FNR. A major clyA transcripthaving its 5' end (+1) located 72 bp upstream of the translationalstart codon and 61 bp downstream of the CRP-FNR binding site wasdetected in the absence of H-NS. The clyA promoter was characterizedas a class I promoter that could be transcriptionally activatedby CRP and/or FNR. According to DNA bending analyses, the clyApromoter region has high intrinsic curvature. We suggest thatit represents a regulatory region which is particularly susceptibleto H-NS silencing, and its features are discussed in relationto regulation of other silencedoperons.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Bacteria having the ability to infect animals and humans are often capable of expressing virulence factors that can be offundamental importance for the interactions that occur betweenthe microorganism and the host. Molecular genetic analyes of differentvirulence determinants of enterobacteria encoding, e.g., cytotoxicsubstances, specific adhesins, and invasion proteins, have demonstratedthat pathogenic isolates have complex gene systems that appearto be regulated in response to environmental growth conditionsaround the bacteria (36). Both enteropathogenic and uropathogenicisolates of Escherichia coli have become good model systems forthis research. From analyses of genes controlling expression offimbrial adhesins and invasiveness it was earlier shown that histone-likebacterial proteins are important for the regulation of virulencefactors (20). The nucleoid-associated protein H-NS is knownto influence the regulation of many genes in E. coli, and it appearsthat H-NS may cause silencing of many different operons (1).Even bacteria belonging to the normal flora presumably need tohave their genes "tuned" to fit the environmental conditions withinthe host. Such regulation may be even more crucial for commensalorganisms.

Cytolysin A (ClyA) is a 34-kDa cytolytic protein encoded by the clyA gene (also referred to as sheA and hlyE [13, 21])located at 26.5 min on the E. coli K-12 chromosome. X-ray crystallographyhas shown that ClyA has unusual structural features and does notresemble any previously studied cytotoxin (59). We demonstratedrecently that highly purified ClyA protein from E. coli K-12 causeslysis of mammalian cells by pore formation in a Ca²⁺-independent fashion (40) and apoptosis in murine-derived macrophage-likecells (30). It is interesting that the gene encoding this potentiallytoxic protein is found in E. coli K-12, which is considered tobe nonpathogenic. In fact, it appears that most nonpathogenicstrains of E. coli carry this gene and have the capacity to expresscytotoxicity (39). Evidently, there is strict regulation ofthe clyA gene since it is phenotypically silent in E. coli K-12under many tested laboratory conditions (39). The clyA geneis derepressed in H-NS-deficient E. coli strains (58; J. M.Gómez-Gómez, J. Blazquez, F. Baquero, and J. L. Martinez, Letter,Mol. Microbiol 19:909-910, 1996; Y. Mizunoe and B. E. Uhlin,Abstr. 34th Intersci. Conf. Antimicrob. Agents Chemother., p.63, 1994), and strains overexpressing SlyA and MprA (13, 34,35, 41). SlyA and MprA belong to a family of proteins thoughtto regulate diverse physiological processes in bacterial pathogens(57). A direct interaction between purified His-SlyA_EC and theDNA upstream of the clyA-coding region was suggested from resultsobtained by band shift assays (41). In addition, ClyA expressionis activated in E. coli K-12 by the expression of HlyX from Actinobacilluspleuropneumoniae (21). HlyX has 73% identical amino acid sequencecompared with the oxygen-responsive transcriptional regulator,FNR, which binds to a putative FNR binding site in the clyA upstreamregion (21). Furthermore, it was recently shown that alteredFNR proteins, similarly to HlyX, could activate the expressionof clyA (43); i.e., minor alterations in a gene encoding a globalregulator have a profound effect on the production of cytotoxicfactors like ClyA. Because of the potential to express such ahost-damaging product, the clyA gene represents a novel classof genes not previously characterized in commensal bacteria. Inthe present paper we present data from experiments aimed at elucidatingfeatures about the strict regulation of clyA.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains and culture media. The relevant genotypes of strains and plasmids used in this work are listed in Tables 1 and 2, respectively. The strainswere grown in LB broth (4) with vigorous shaking or on LB brothsolidified with 1.5% (wt/vol) agar. Blood agar plates were 5%horse erythrocytes solidified with 1% (wt/vol) Columbia agar base(Oxoid Ltd.). Antibiotic selection for pFZY1-derived plasmidswas carried out using carbenicillin (25 µg · ml¹). In other cases the growth medium was supplemented with carbenicillin(50 µg · ml¹), kanamycin (50 µg · ml¹), chloramphenicol (10 µg · ml¹), or tetracycline (15 µg · ml¹). Anaerobic growth conditions were achieved by using the AnaeroGencompact atmosphere generation system of Oxoid Ltd., followingthe instructions of the manufacturer.

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TABLE 1. Bacterial strains used in this work

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TABLE 2. Plasmids used in this work

Genetic techniques. Standard procedures were used in all general molecular applications (46). Generalized bacteriophage P1 transduction wasperformed as described by Willets et al. (61). Sequencing oligonucleotideswere made on an Applied Biosystems 394 synthesizer or obtainedfrom DNA Technology, Aarhus, Denmark. Dideoxy sequencing was carriedout using a T7 sequencing kit (Pharmacia Biotech) according tothe specifications of the manufacturer, using pYMZ62 as the template.For general purposes DNA sequencing was performed using the ABIPRISM Dye Terminator Cycle Sequencing Ready Reaction kit withAmpliTaq DNA polymerase and an ABI PRISM 377 DNA sequencer. Site-specificalterations of DNA sequences were obtained by using the QuickChangesite-directed mutagenesis kit of Stratagene, following the instructionsof the manufacturer. The desired mutations were always placedin the middle of the primer with approximately 15 bases of correctsequence on eachside.

Plasmid and strain constructions. The construct pYMZ83 was made by ligation of a 0.4-kb EcoRI-BglII restriction fragment from pYMZ80 into EcoRI-BamHI-digestedpFZY1, resulting in a clyA::lacZ transcriptional fusion havingits 5' end 290 bp upstream of the clyA start codon and its fusionjunction 76 bp into the clyA coding sequence. The plasmid pMWK4was constructed by ligating a blunt end-generated SmaI-BglII restrictionfragment from pYMZ80, containing the DNA 290 bp upstream of anddown to 76 bp within the clyA coding sequence, into EcoRV-digestedpCH257 suicide vector, using E. coli SY327( $lambda$ pir) as the host strain.The plasmid pMWK4 was integrated into the chromosome of MC1061by a single recombination event between the 366-bp clyA sequencein our construct and the corresponding region of clyA on the chromosome.The resulting strain was designated MWK2. BSN26, BSN27, and MWK6were transduced with P1 grown on MWK2 (clyA::luxAB), and transductantswere isolated by selection for chloramphenicol resistance, resultingin the strains JON33, JON34, and MWK10, respectively. The plasmidpMWK24 was constructed by using the PCR-based strategy describedabove and the primers crp5 (5'-CATTAAACATTGTGTGATATTTATCATATT-3')and crp6 (5'-AATATGATAAATATCACACAATGTTTAATG-3'), with pYMZ81 asthe template. The same approach was utilized, with pYMZ81 as thetemplate, to construct pMWK28 (primers crp7 [5'-CATTAAACATTGTTTAATATTTATCATATT-3']and crp8 [5'-AATATGATAAATATTAAACAATGTTTAATG-3'], pMWK29 (primerscrp9 [5'-TGACATTAAACATTGTCTAATATTTATCATATTAAT-3'] and crp10 [5'-ATTAATATGATAAATATTAGACAATGTTTAATGTCA-3'],pMWK31 (primers a-10 [5'-TCCCGCCCGGCTAACCACGAACTAGATGAAGTAAAA-3']and b-10 [5'-TTTTACTTCATCTAGTTCGTGGTTAGCCGGGCGGGA-3'], and pMWK9(primers crp1 [5'-CATTGTTTGATATAGATCACATTTATAGAAATAAAGAC-3'] andcrp2 [5'-GTCTTTATTTCTATAAATGTGATCTATATCAAACAATG-3']. The plasmidpMWK10 was constructed by the same method, with the primers crp3(5'-GACATTAAACAAAATGTGATCTAGATCACATTTATAG-3') and crp4 (5'-CTATAAATGTGATCTAGATCACATTTTGTTTAATGTC-3')and pMWK9 as the template. A BbrPI-BglII promoter fragment containingthe consensus cyclic AMP (cAMP) receptor protein (CRP) site (5'-AAATGTGATCTAGATCACATTT-3')(see reference 16 and references therein) was cloned into thecorresponding sites of the construct pJON78 to generate pMWK45.The derivative pJON78 is a 3.5-kb subclone of the clyA locus inthe suicide donor plasmid pKO3. Using the derivative pMWK45, theCRP consensus site was introduced onto the chromosome of MC4100,as previously described (31), to generate the strain MWK11.Strain BEU616 (hns::cat) was constructed by transduction of MC1063with P1 grown on a derivative of JC7623 carrying an hns::cat allelein the chromosome. JC7623 is recC22 recB21 sbcB15 sbc201 (24).MC1063 is MC1061 with trp::Tn10 (11). BEU701 and BEU705 wereconstructed by transduction of M182 fnr and M182 crp fnr, respectively,with P1 grown on BEU616. To construct a 429-bp in-frame deletionmutant of the slyA coding region, we used a PCR-based strategy(see above) and DH5 $alpha$ as the host strain: By using the primersSKO1 (5'-AATTATAAGGAGATGGAATTCGAATCGCCACTAGGT-3'), SKO2 (5'-ACCTAGTGGCGATTCGAATTCCATCTCCTTATAATT-3'),SKO3 (5'-ATTGAGTTACAGGCCGAATTCTGAAATGAAGGGGGC-3'), and SKO4 (5'-GCCCCCTTCATTTCAGAATTCGGCCTGTAACTCAAT-3'),and pJON22 as template, two new EcoRI restriction sites (underlinedsequences) were introduced in the slyA gene, at bp 4 to 9 andbp 433 to 438, respectively. The resulting plasmid clone, designatedpMWK11, was subsequently digested with EcoRI and religated togenerate pMWK12. To facilitate cloning into pKO3, a 1.5-kb PstIfragment of pMWK12, encompassing the constructed in-frame deletion,was cloned into PstI-digested pSL1180 cloning vector, resultingin the plasmid pMWK13, which was used as an intermediate. A 1.5-kbPmlI-BamHI fragment of pMWK13, containing the slyA in-frame deletion,was cloned into SmaI-BamHI-digested pKO3, resulting in the plasmidpMOJ2. This construct, containing the slyA in-frame deletion,was introduced into BSN27 as previously described (31) to generateMWK6.

ClyA expression assays. Lytic activity towards erythrocytes was scored by a clearance zone on blood agar plates after 16 to 17 h of incubation at37°C or by quantification of the release of hemoglobin from erythrocytesas described below. Bacteria were grown to late logarithmic phaseand diluted to 8.0 × 10⁶ cells ml¹ in 1× phosphate-buffered saline. Fifty microliters of bacterialsuspension was mixed with 50 µl of a horse erythrocyte suspensionin 1× phosphate-buffered saline in a 96-well microtiter plateand incubated for 120 min at 37°C prior to determination of therelease of hemoglobin, as described previously (47). $beta$ -Galactosidaseactivity was measured as previously described (36), with compensationfor the number of plasmid-free cells (51). Luciferase assayswere performed as described earlier (42).

Sodium dodecyl sulfate-PAGE and immunoblot analysis. For determination of the ClyA and SlyA protein content in cells, bacterial samples grown at 37°C were harvested at late logarithmicphase, or from agar plates after 16 to 17 h of incubation, priorto analysis by sodium dodecyl sulfate-polyacrylamide gel electrophoresis(PAGE) as previously described (29). Western immunoblottingwas performed using an antiserum raised against ClyA as describedpreviously (40) or using an antiserum raised against SlyA asdescribed below at final dilutions of 1:1,000 and alkaline phosphatase-conjugatedsecondary antibody at a final dilution of 1:3,000. Immunoreactivebands were visualized using the enhanced chemiluminescence Westernblotting detection system of Amersham Pharmacia Biotech, followingthe instructions of the manufacturer. Rabbit anti-SlyA antibodieswere raised against His-SlyA which had been purified as describedpreviously (41). An antiserum taken 8 weeks after the fourthinjection was affinity purified as previously described (56).

RNA isolation and primer extension. Total RNA was isolated from late logarithmic phase cultures, which had been grown in LB broth, using the hot-phenol method(63). Primer extension analysis was carried out as follows.Oligomers were 5' end labeled using polynucleotide kinase and[ $gamma$ -³²P]ATP. A molar excess of the primer was annealed to 5 µg of totalRNA in 8 µl of an annealing buffer (50 mM Tris-HCl [pH 8.3], 60mM NaCl, 10 mM dithiothreitol [DTT]). Samples were heated for5 min at 80°C and subsequently chilled on ice for 5 min. Eightmicroliters of extension mixture (25 mM Tris-HCl [pH 8.3], 30mM NaCl, 15 mM MgCl₂, 1.25 mM DTT, a 1 mM concentration of eachdeoxynucleoside triphosphate) was added together with 3 U of avianmyeloblastosis virus reverse transcriptase, and samples were incubatedat 42°C for 60 min. The oligonucleotides used were cct1 (5'-CCGTTTTATCTGCAACGATTTCAGTC-3')and cct4 (5'-GGAGGCTGCCTGTGAATACTCCTGTTTAAAGCGACTTAAC-3'). Theextension products were analyzed by electrophoresis on 6% polyacrylamide-ureagels.

DNA bending analysis. Overlapping 300-bp DNA fragments of the clyA locus were generated by PCR using pYMZ62 as a template and the following oligonucleotideprimers from the clyA locus (see Fig. 2): for fragment a, $-$ 349(5'-GCGGAAAAGTCACAATTTCG-3') and $-$ 50b (5'-TTAATATGATAAATATCAAA-3');for fragment b, $-$ 250 (5'-CCAGCAGATCAATACTGATT-3') and +50b (5'-ATAAATTGTAATGAAACTCC-3');for fragment c, $-$ 150 (5'-ACGCTCATCCAGCAGAAATG-3') and +150b (5'-AAGATCTAATGCTCCATCTG-3');for fragment d, $-$ 50a (5'-ATAGAAATAAAGACATTGAC-3') and +250 (5'-CGGAGGCTGCCTGTGAATAC-3');for fragment e, +50a (5'-TATATTTAAAGAGGCGAATG-3') and +349 (5'-ATTGCGTCGCAACACCACAC-3');and for fragment f, +150a (5'-TTATAATAAATATCTCGATC-3') and +449(5'-TTCGTGATGCCGTCATCCAG-3'). The generated PCR fragments werecloned utilizing the pGEM-T Easy Vector System (Promega), as specifiedby the manufacturer, resulting in the constructs pMWK32 (position $-$ 349 to $-$ 50 [base pairs] relative to the clyA transcriptionalstart point), pMWK33 ( $-$ 250 to +50), pMWK34 ( $-$ 150 to +150), pMWK35( $-$ 50 to +250), pMWK36 (+50 to +349), and pMWK37 (+150 to +449).These constructs were digested with EcoRI and used for DNA bendinganalysis.

The fragments were run on 6% polyacrylamide-bis-acrylamide gels (30:0.8, vol/vol) in a 90 mM TBE buffer (90 mM Tris, 90 mMboric acid, 2.5 mM disodium EDTA, pH 8.3) at 6 mA for 10 h at5°C, room temperature, and 37°C, and subsequently stained withethidium bromide. The migration lengths were measured and comparedto a 1 Kb PLUS DNA Ladder molecular size standard (GibcoBRL).The ratio between the observed migration length (M_o) and the expectedmigration length (M_e) was plotted against the center positionof the DNAfragment.

Gel mobility shift assay. Band shift assays were performed with DNA fragments from the plasmid pYMZ80 obtained by digestion with DraI and EcoRI. PurifiedH-NS protein was obtained from a strain carrying an expressionplasmid (B. Sondén and B. E. Uhlin, unpublished data). DNA ata final concentration of approximately 36 nM was mixed with H-NSat a final concentration of 0.8 to 12 µM in buffer B (25 mM HEPES[pH 7.5], 0.1 mM EDTA, 5 mM DTT, 10% glycerol) in a total volumeof 10 µl. The samples contained 100 ng of poly(dI-dC), and KClwas added to 50 mM. The reactions were incubated for 15 min at26°C and then resolved by nondenaturing PAGE in a 6% gel usingTBE running buffer. The gel was subsequently stained with ethidiumbromide.

DNase I footprint analysis. DNase I footprint analysis with CRP was carried out essentially as described previously (19). The DNA fragments were obtainedby PCR of the strain MC1061, with the primers cct1 and umu1 (5'-AATATTTGTCGCTGC-3')and the latter primer had been labeled with [ $gamma$ -³²P]dATP using T4 polynucleotide kinase. Reactions were carriedout in a total volume of 50 µl. CRP was purified essentially asdescribed previously (64), with the exception that CRP was precipitatedwith (NH₄)₂SO₄ to obtain CRP free from cAMP instead of removingthe cAMP by chromatography. Samples of CRP (final concentration,4.7 to 38 nM) and/or RNA polymerase (22 to 87 nM) were added toapproximately 10 ng of DNA in buffer B plus 50 mM KCl. When included,cAMP was added to a final concentration of 20 mM. Fifty nanogramsof DNase I and MgCl₂ to a final concentration of 5 mM were addedto start the digestion. After 120 s (90 s for samples withoutprotein) the reactions were stopped by the addition of 12 µl ofstop mix (0.25 mM EDTA, 1.5 M NaCl, oyster glycogen [1.5 mg ml¹]). The samples were then phenol extracted, ethanol precipitated,and analyzed on 6% polyacrylamide-ureagels.

DNase I footprint analysis with H-NS was carried out essentially as described previously (19). The DNA fragments were obtainedby PCR of the plasmid pYMZ62, with the primers p73 (5'-GAATGTCTTTCTGGGCGG-3')and umu1, labeled with [ $gamma$ -³²P]dATP using T4 polynucleotide kinase. Reactions were carriedout in a total volume of 50 µl. Samples of H-NS (final concentration,4.8 to 9.6 µM) were added to approximately 30 ng of DNA in bufferB plus 50 mM KCl. Fifty nanograms of DNase I and MgCl₂ at a finalconcentration of 5 mM was added to start the digestion. After120 s (90 s for samples without protein) the reactions were stoppedby the addition of 12 µl of stop mix (defined above). The sampleswere then phenol extracted, ethanol precipitated, and analyzedon 6% polyacrylamide-ureagels.

Computer projection of DNA curvature. Projections of calculated DNA curvature were obtained by using the BEND program of the DNASTAR software package, which usesa wedge model to predict the helix trajectory. The dinucleotidebending angles used were according to published data (5).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Effects of H-NS deficiency and SlyA overproduction on clyA transcription as monitored by a chromosomal clyA::luxAB operon fusion. To determine at which level H-NS affects the expression of clyA, and to quantitatively monitor the transcription of clyA inhns mutant and SlyA-overproducing strains during different growthphases, we used the strains JON33 and JON34, which have a transcriptionalclyA::luxAB fusion at the site of the clyA locus (see Materialsand Methods). We investigated the transcription of clyA in isogenichns wild-type and mutant strains (JON33 and JON34) by monitoringthe expression of the chromosomal clyA::luxAB fusion throughoutthe growth cycle. As shown in Fig. 1, the luciferase activityof the hns strain JON34 peaked in late logarithmic phase and showeda more-than-fourfold increase in activity compared with the hns⁺ strain. In parallel we studied the activation of clyA by SlyAby assaying the expression of the chromosomal clyA::luxAB fusionthroughout the growth cycle, using JON33 (hns⁺) as the host strain. As shown in Fig. 1, the luciferase activityof the SlyA-overproducing strain JON33/pJON22 peaked in late logarithmicphase and showed a more-than-fivefold increase in activity comparedwith the vector control strain JON33/pACYC177. Similar resultswere obtained when expression was monitored at the translationallevel using contact hemolysis assays with erythrocytes (see Materialsand Methods; data not shown). These results were in accordancewith the observation of a peak ClyA activity in samples takenfrom MprA- or SlyA-overproducing strains at late logarithmic phase(13, 34). Therefore, we conclude that the expression of clyAis mainly controlled at the transcriptional level and that H-NSis responsible for silencing the transcription of clyA. Furthermore,upon relief of this silencing (hns mutants and SlyA-overproducingstrains), the highest expression of the chromosomal clyA::luxABfusion occurred in the late logarithmic phase.

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FIG. 1. A. Effects of H-NS deficiency and SlyA overproduction on the transcription of clyA throughout the growth curve. (A) Expression of luciferase activity from a chromosomal clyA::luxAB fusion in the strains JON33 (hns⁺) (

), JON34 (hns) ( $open circle$ ), JON33/pACYC177 (vector control) (

), and JON33/pJON22 p(SlyA) (

). The expressed luciferase activity was quantified by the luciferase assay (see Materials and Methods), and LUX units were displayed as millivolts/(milliliters × optical density at 600 nm). The growth curves are indicated with dotted lines. (B) DNA sequence of the clyA promoter region down to 76 bp into the clyA coding sequence, which is the position of the lux and lac fusion junctions. The positions of the transcriptional initiation point (+1) and putative regulatory elements, i.e., binding sites for CRP and FNR, Shine-Dalgarno (S.D.) sequence, and $-$ 10 and $-$ 35 boxes are shown. The mutational alterations in the plasmid pMWK31 are shown in parentheses below the $-$ 10 region sequence.

Site of initiation of derepressed clyA transcription and promoter analysis in hns mutant E. coli. Analysis of clyA transcription by Northern blot hybridization suggested that it is a monocistronic operon (41). In orderto further localize the clyA promoter active in the absence ofH-NS, the clyA transcript was assayed by primer extension analysis.RNA was extracted from the hns strain, BEU616, that expressesphenotypically detectable levels of the ClyA protein. The clyAprimer extension resulted in a distinct product that should representone major transcript with the 5' end 72 nucleotides upstream ofthe ATG translational start codon of the clyA structural gene(data not shown). Therefore, we concluded that the observed clyAtranscriptional start point (+1) in the hns mutant strain wasthe same as in strains in which the clyA gene was activated bythe cloned slyA locus (34). To functionally assess the predicted $-$ 10 promoter box (TATGAAT) (Fig. 1B), we introduced site-specificalterations in the clyA upstream sequence, using a PCR-based strategy(see Materials and Methods) and the plasmid pYMZ81 as the template.This plasmid contains the clyA sequence cloned in the oppositeorientation to the promoter of the vector, the gene thus beingcontrolled by its native promoter region only. The resulting construct(plasmid pMWK31), with the $-$ 10 sequence changed to (CACGAAC),had lost its promoter activity according to the in vivo tests.As shown below, DH5 $alpha$ harboring pMWK31 showed a lack of expressionof ClyA protein and cytolytic activity compared with DH5 $alpha$ /pYMZ81.Thus, the predicted $-$ 10 promoter box is important for clyA expression,and we conclude that this analysis localised the promotersequences.

H-NS shows preferential interaction in vitro with clyA sequences. To examine whether there is a direct interaction between H-NS and the clyA locus, electrophoretic mobility shift assays wereperformed as described in Materials and Methods, using purifiedH-NS protein and clyA DNA. An initial indication of preferentialbinding of H-NS to clyA DNA (fragments 3 and 5) was observed usingEcoRI-DraI-digested pYMZ80 as the target DNA (Fig. 2B). It wasalso observed that one of the vector DNA fragments in this experiment(fragment 1) shifted in the presence of H-NS, which is consistentwith previous findings of H-NS interaction with the plasmid carriedbla promoter region (33, 65). DNase I footprinting assaysshowed that H-NS interacted preferentially with two regions ofthe clyA promoter region (Fig. 2C). The H-NS protein interactedboth in the downstream region of the promoter (designated I inFig. 2C) and in the upstream region (designated II in Fig. 2C).These findings support a model where H-NS directly interacts with,and negatively affects, clyA transcription.

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FIG. 2. Binding of purified H-NS to clyA. (A) Schematic drawing of the plasmid pYMZ80. Relevant features, positions of the restriction endonuclease sites (D, DraI; E, EcoRI), and the extent of the resulting restriction endonuclease fragments used in gel shift assays with H-NS are indicated. Fragments bound preferentially by H-NS are indicated by thick black horizontal bars, and fragments showing no specific shift are indicated by thin black horizontal bars. Cloned chromosomal DNA encompassing the clyA locus is indicated in grey. (B) Gel shift assay of the clyA gene with purified H-NS protein. The different DraI and EcoRI restriction fragments generated from pYMZ80 are indicated within the figure. Lanes: a, DNA ladder; b, no protein; c, 0.8 µM H-NS; d, 1.7 µM; e, 2.5 µM; f, 3.4 µM; g, 4.2 µM; h, 5.0 µM; i, 6.7 µM; j, 8.4 µM, k, 10 µM; 1, 12 µM. (C) DNase I footprint assay of the clyA promoter region with H-NS. Addition of H-NS was as indicated at the top. Lanes 1 and 9 show samples without any H-NS added and lanes 2 to 8 show samples with increasing amounts (4.8, 5.6, 6.4, 7.2, 8.0, 8.8, and 9.6 µM) of H-NS added. The positions of the clyA promoter ( $-$ 10 and $-$ 35 regions) and the CRP-FNR site are shown by solid lines along the left side. The two main regions of H-NS interaction (labelled I and II) are shown by dashed lines along the right.

SlyA is not required for clyA expression in hns mutant E. coli. Since SlyA, when overexpressed, activates the expression of ClyA, we wanted to investigate the requirement of SlyA for derepressionof clyA in the absence of H-NS. We introduced (see Materials andMethods) a slyA in-frame deletion into the slyA locus of the hnsstrain BSN27, resulting in the strain MWK6, and a clyA::luxABfusion into the clyA locus of MWK6, resulting in the strain MWK10.We found that there was no significant difference in luciferaseactivity throughout the growth curve in strain JON34 comparedwith MWK10 (data not shown), indicating that SlyA is not requiredfor clyA expression in H-NS mutant strains. We also found thatBSN27 and MWK6 showed similar ClyA activity on blood agar (Table3) and quantified lytic activity using the erythrocyte assay(data not shown). This was in accordance with overproduction ofSlyA in the hns clyA::luxAB strain JON34/pJON22 (data not shown),in the hns strain JON31/pJON22, and in the hns slyA strain MWK6/pJON22(Table 3), which did not result in an additive effect on ClyAexpression compared with the control strains JON34/pACYC177, JON31/pACYC177,and MWK6/pACYC177. We therefore concluded that SlyA was not essentialfor clyA expression when H-NS was absent.

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TABLE 3. Expression of ClyA as evidenced by lysis^a of erythrocytes in agar

The clyA promoter is dependent on CRP for efficient expression. Analysis of the clyA promoter region revealed a potential CRP binding site (5'-TTGTTTGATATTTATCATATTA-3') that matched theconsensus in 13 out of 22 bases. The CRP binding site partly overlappedwith a previously identified FNR binding site (21). To investigatethe requirement of CRP for the transcription of clyA, a cat (Cm^r) gene block was introduced into the hns locus of the strainsM182 and M182 crp, resulting in the strains JON31 and JON32, respectively(see Materials and Methods). The low-copy (one to two copies perchromosome) clyA::lacZ reporter system pYMZ83 (based on the mini-Fvector pFZY1) was used in these strains to study the level ofclyA expression (Fig. 3). JON31 showed a more-than-sixfold-greaterexpression of $beta$ -galactosidase activity than JON32, which expressedthe same low levels as the crp⁺ hns⁺ strains (even lower $beta$ -galactosidase activity was observed inhns⁺ crp strains). This was consistent with a much reduced cellularlevel of ClyA protein in the hns crp double mutant strain, asevidenced by Western immunoblotting (data not shown) and a substantiallyreduced lysis of erythrocytes in agar (Table 3). In addition,the results with the clyA::lacZ fusion indicated that the regulatoryDNA sequences required for control of clyA transcription are presentwithin the region spanning from 290 bp upstream of the clyA codingsequence to 76 bp into the clyA structural gene (the operon fusionjunction). The reduced ClyA activity of JON32 could be restoredby the reintroduction of CRP on a plasmid (pDW300). Thus, we concludedthat CRP is required for derepression of clyA in hns strains.To investigate whether CRP is also required for the SlyA-mediatedrelief of H-NS silencing, we introduced the plasmid pJON22 (encodingSlyA) into the crp mutant and wildtype E. coli strains, M182 crpand M182, respectively. As shown in Table 3, overexpression ofSlyA resulted in a strong cytolytic phenotype in M182, but onlya weak cytolytic phenotype in M182 crp. This suggested that CRPis important for activation of ClyA expression by SlyA. The absenceof CRP did not affect the level of SlyA protein, which was similarin M182/pJON22 and M182 crp/pJON22 as evidenced by western immunoblotting(data not shown), using an antiserum raised against SlyA (seeMaterials and Methods). Therefore, we concluded that the clyApromoter is dependent on CRP for efficient clyA expression.

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FIG. 3. CRP-dependent transcription of clyA. Shown is the quantification of clyA transcription from a clyA::lacZ reporter system on the plasmid pYMZ83 in the following strains grown under aerobic (solid black bars) and anaerobic (grey bars) conditions for 16 to 17 h at 37°C on LB agar: wt, M182; crp, M182 crp; fnr, M182 fnr; crp fnr, M182 crp fnr; hns, JON31; and hns crp, JON32. $beta$ -Galactosidase ( $beta$ -gal.) activity was measured as described in Materials and Methods. A relative $beta$ -galactosidase activity of 1.0 equals the activity of the wild-type strain, M182/pYMZ83, under aerobic growth conditions (350 Miller units). Error bars indicate standard errors of the means from three separate experiments.

CRP interaction at the clyA promoter in vitro. The involvement of CRP in the regulation of clyA gene expression and the presence of a potential CRP binding site in the clyAupstream region suggested a direct interaction of CRP with theclyA promoter. To investigate whether CRP could directly bindto the clyA promoter region, gel mobility shift assays and DNaseI footprint analysis with purified CRP and the clyA DNA were carriedout as described in Materials and Methods. A weak interactionbetween CRP and the clyA promoter was indicated by results fromgel shift assays (data not shown). In the footprint analysis weaklyfootprinted regions were obtained only when CRP and RNA polymerasewere both present. A region of protection from position $-$ 53 to $-$ 72, which encompasses the putative CRP binding site, was causedby CRP in the presence of cAMP and RNA polymerase (Fig. 4). Apparenthypersensitivity at positions $-$ 55 and $-$ 64 was caused by CRP inthe presence of cAMP and RNA polymerase and by RNA polymeraseat positions $-$ 21 and $-$ 22, which is similar to the hypersensitivesites $-$ 24, $-$ 25, and $-$ 54, noted in footprint analysis with FNR,HlyX, and RNA polymerase (21). Additional hypersensitive siteswere found at position $-$ 98 with RNA polymerase (diminished bythe addition of CRP and cAMP), at positions +35 and +36 with RNApolymerase plus CRP and cAMP, and at position +63 with RNA polymerase(diminished by the addition of CRP and cAMP). Evidently CRP interactedin a cAMP-dependent manner with the postulated suboptimal bindingsite. Based on the above observations we suggest a direct rolefor CRP in the positive regulation of clyA expression.

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FIG. 4. Binding of purified CRP to clyA. DNase I footprint assay of the clyA promoter region with CRP and RNA polymerase. The additions of CRP, RNA polymerase (RNAp), and cAMP were as indicated at the top. The extent of the DNA fragment used is shown by the indicated positions (base pairs). The position of the putative CRP binding site is shown by a solid line along the left side. The approximate region of interaction with RNA polymerase is shown by a dashed line along the right. Hypersensitive sites are indicated with arrows. When included, cAMP was added at a concentration of 20 mM. Lanes: a, no protein; b, CRP (4.7 nM) plus RNA polymerase (0.5 U); c, CRP (9.4 nM) plus RNA polymerase (22 nM); d, CRP (4.7 nM) plus cAMP plus RNA polymerase (22 nM); e, CRP (9.4 nM) plus cAMP plus RNA polymerase (22 nM); f, CRP (19 nM) plus cAMP plus RNA polymerase (22 nM); g, CRP (9.4 nM); h, CRP (19 nM); i, CRP (38 nM); j, CRP (9.4 nM) plus cAMP; k, CRP (19 nM) plus cAMP; 1, CRP (38 nM) plus cAMP; m, RNA polymerase (22 nM); n, RNA polymerase (44 nM); o, RNA polymerase (87 nM); p, no protein; q, no protein.

An altered CRP site in the clyA promoter results in altered expression of ClyA protein. Since the potential CRP binding site in the clyA upstream region shows only partial homology (13 out of 22 bases) with theproposed consensus sequence, (5'AAATGTGATCTAGATCACATTT-3') (16),we wanted to investigate whether the sequence features of thissite are relevant for the regulation of ClyA expression. We thereforeintroduced site-specific changes in the clyA upstream sequenceof the plasmid pYMZ81 (see Materials and Methods) (Fig. 5A). Site-specificalterations in the upstream pentamer of the potential CRP siteresulted in the plasmid clones pMWK24 (TGTGA), pMWK28 (TTTAA),and pMWK29 (TCTAA). In addition, we substituted four positionsin the predicted CRP binding site, resulting in the plasmid pMWK9,having an altered CRP site (5'-TTGTTTGATATAGATCACATTT-3') whichmatches the consensus in 17 out of 22 bases. The construct pMWK10contains an altered CRP site (5'-AAATGTGATCTAGATCACATTT-3') thatperfectly matches the consensus. We subsequently quantified thecytolytic activity of different E. coli strains carrying theseconstructs by using the erythrocyte assay (Fig. 5B) and by monitoringthe cellular levels of ClyA protein with Western immunoblotting(Fig. 5C). Compared with DH5 $alpha$ /pYMZ81, substantial decreases incellular ClyA protein and cytolytic activity were exhibited byDH5 $alpha$ /pMWK28 and DH5 $alpha$ /pMWK29. This is consistent with previousfindings (25) which suggested that alterations in the upstreampentamer (TGTGA) at position two (G $right-arrow$ C) and at position four (G $right-arrow$ A)abolish CRP binding. DH5 $alpha$ /pMWK24, which has an improved CRP site(T $right-arrow$ G) at position two in the upstream pentamer, showed an increasedcellular level of ClyA protein and a stronger cytolytic activitythan DH5 $alpha$ /pYMZ81. An even greater increase in cellular ClyA proteinand cytolytic activity was exhibited by DH5 $alpha$ carrying pMWK9 orpMWK10. That the clyA expression was CRP-dependent in these caseswas confirmed by tests with a crp mutant strain. Only a low, barelydetectable level of cellular ClyA protein and cytolytic activityin the crp strain M182 crp carrying pMWK9, pMWK10, and pYMZ81was observed (data not shown). We also constructed a strain withthe CRP consensus DNA binding site in the clyA promoter regionon the chromosome of the hns⁺ strain MC4100. The resulting derivative (strain MWK11) showeda strong hemolytic phenotype on blood agar plates, and there wasa high level of ClyA protein in the cells detected by Westernblot analysis (Fig. 6). These findings support a model where CRPis involved in expression of ClyA. We concluded that the sequencefeatures of the CRP binding site are important for the positiverole of CRP in the regulation of clyA expression.

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FIG. 5. Effect of site-specific alterations in the CRP DNA site and $-$ 10 sequence of the clyA promoter on clyA expression from various plasmids in DH5 $alpha$ . The construct pMWK31 contains an altered $-$ 10 promoter box (TATGAAT $right-arrow$ CACGAAC). The strains were grown to late logarithmic phase and treated as described in Materials and Methods. (A) Sequences of the CRP binding sites in wild-type and mutant clyA clones. The consensus CRP binding site (see reference 16 and references therein) and positions showing identity to the consensus are shown in boldface type. Pentamers referred to in the text are underlined. (B) Cytolytic activity of the different strains towards erythrocytes. The cytolytic activity was measured as described in Materials and Methods, and the activity of the strain DH5 $alpha$ /pYMZ81 was arbitrarily set to 1.0. (C) Determination of ClyA protein content in the different strains by Western immunoblotting using a ClyA-specific antiserum (see Materials and Methods). Strains were grown in LB broth to late logarithmic phase. Approximately 10⁷ bacteria were used for the extract loaded in each lane. The lower panel shows a prolonged exposure, and the ClyA reactive band is indicated with an arrow.

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FIG. 6. Effect of alterations in the CRP binding site in the clyA promoter region on the chromosome to match the consensus sequence (5'-AAATGTGATCTAGATCACATTT-3'). (Upper panel) MC4100 and MWK11 on a blood agar plate after incubation at 37°C for 17 h. (Lower panel) Detection of ClyA protein content in MC4100 and MWK11 by Western immunoblotting using a ClyA-specific antiserum (see Materials and Methods). Strains were grown in LB broth to late logarithmic phase. Approximately 10⁷ bacteria were used for the extract loaded in each lane.

The interaction by CRP with typical binding sites may cause local bending of the DNA, which may affect the curvature propertiesof a nearby promoter. We noted that the clyA promoter region isrich in A-T base pairs (73.1% for the 186-bp region upstream ofthe start codon) and the region shows features typical of curvedDNA. We studied the potential DNA bending properties by usingoverlapping DNA fragments in a gel migration analysis and by computerprojection (see Materials and Methods). The results confirmedthat, in particular, the region containing the 5' end of clyAmay be intrinsically curved (Fig. 7).

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FIG. 7. (A) Schematic drawing of the umuD clyA intercistronic region. The DNA site for CRP-FNR is shown as a grey box, and transcriptional start points for clyA and umuD are indicated by horizontal arrows. The extents of the overlapping DNA fragments generated by PCR, which were used in DNA bending analysis experiments, are shown as horizontal lines. (B) Mapping of the center of the sequence directed bend. M_os as distances from the top of the gel were divided by the M_e for each fragment. The M_o/M_e value was plotted against the center position (in base pairs) of the DNA fragment. RT, room temperature. (C) The upper panel shows a computer projection analysis of 1,402 bp from the clyA DNA region, which includes the 912-bp clyA coding sequence with 372 bp upstream of the clyA start codon and 118 bp downstream of the clyA stop codon. The positions of the translational start and stop codons of clyA are indicated by arrows. The lower panel shows an enlargement of the predicted curvature pattern in the clyA promoter region from position 200 to 400. The positions of the predicted CRP binding site ( $-$ 72 to $-$ 51), the $-$ 35 sequence ( $-$ 35 to $-$ 30), the $-$ 10 sequence ( $-$ 12 to $-$ 6), and the transcriptional start point (+1) are indicated.

Involvement of both CRP and FNR in regulation of clyA expression during anaerobic growth conditions. It was previously reported that overproduction of the FNR homolog HlyX of A. pleuropneumoniae in anaerobically grown E. coliK-12 results in binding to the FNR site and activation of clyAexpression, while overproduction of the E. coli FNR protein resultsin less efficient activation (21). The requirement of CRP andFNR for anaerobic clyA expression was subsequently investigated.The low-copy clyA::lacZ reporter system pYMZ83 was used in differentstrains to study the level of clyA expression (Fig. 3), and acat (Cm^r) gene block was introduced into the hns locus of the strainsM182 fnr and M182 crp fnr, resulting in the strains BEU701 andBEU705, respectively (see Materials and Methods). During anaerobicgrowth a clearly reduced $beta$ -galactosidase activity was observedin both fnr and crp strains (most reduced in the crp fnr doublemutant strain) (Fig. 3), suggesting an involvement of both CRPand FNR in the transcriptional regulation of clyA expression.As evidenced by the lysis of erythrocytes in agar (Table 3),the absence of CRP, but not of FNR, reduced the level of clyAderepression in anaerobically grown hns strains. The attenuatedlytic activity of BEU705 could be restored both with and withoutthe presence of oxygen by the introduction of CRP on a plasmid(pDW300), and to some extent, under anaerobic conditions only,by the introduction of FNR (plasmid pGS24) or altered FNR proteinshaving CRP binding specificities (plasmids pGS215 and pGS297).We concluded that the clyA promoter is dependent on CRP also duringanoxic growth conditions and that FNR to some extent can complementthe requirement for CRP during anaerobic growthonly.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Silencing of clyA by H-NS and relief of silencing by SlyA. The clyA locus in the E. coli K-12 chromosome does not seem to be expressed under most laboratory growth conditions, and ourpresent evidence established that the gene is subject to silencingby H-NS. The slyA and mprA genes have been shown to activate theexpression of clyA when present in multiple copies (13, 34,35, 41). In the present work we demonstrate that the majorclyA transcript in the hns strain BEU616 has a 5' end (+1) located72 nucleotides upstream of the start of the clyA coding sequence.Thus, upon relief of the H-NS silencing, either in hns mutants(this work), or by overproduction of SlyA (34), the same promoterappeared to be active. Site-specific alterations of the putative $-$ 10 clyA promoter box (TATGAAT $right-arrow$ CACGAAC) resulted in a significantlydecreased expression of ClyA, establishing that this particularpromoter is crucial for ClyAexpression.

When H-NS acts as a silencer or repressor it binds to AT-rich, curved sequences and thereby blocks transcription of the genein question (6). The DNA of the clyA promoter (the 186 bp immediatelyupstream of the clyA start codon) is notably A-T rich (73.1%).Computer bend predictions of the clyA locus suggested sharp bendsboth in the promoter and in the structural gene, and DNA bendinganalysis of the clyA promoter showed that it contains intrinsiccurvature (Fig. 7). By studying the interaction with purifiedH-NS and the clyA gene in vitro using electrophoretic mobilityshift and DNase I footprint assays (Fig. 2), it could be concludedthat H-NS binds preferentially to DNA fragments upstream and downstreamof the clyA transcriptional start point (+1). The protection ofthe clyA $-$ 10 and $-$ 35 regions was less pronounced than for surroundingsequences, something that has also been seen with the promoterfor the proU operon, encoding a glycine betaine transport system(33). Hence, it appears that the very low level of clyA expressionin E. coli K-12 strains is due to a direct interaction of H-NSwith the clyA locus. By monitoring the expression from a chromosomalclyA::luxAB fusion, we observed that the highest clyA transcriptioncoincided with the late logarithmic phase in both H-NS mutantsand SlyA-overproducing strains (Fig. 1), which was consistentwith previous observations with ClyA activity in MprA and SlyA-overproducingstrains (13, 34). SlyA was not essential for clyA expressionin an hns strain background, since the hns slyA strain MWK6 andthe hns slyA clyA::luxAB strain MWK10 did not show a reduced ClyAexpression. In addition, the overexpression of SlyA in the hnsstrain JON31/pJON22, the hns clyA::luxAB strain JON34/pJON22,and the hns slyA strain MWK6/pJON22, did not result in a furtherelevation of ClyA expression. Based on our findings, demonstratingno absolute requirement of SlyA for ClyA expression, but rathera copy number effect, we suggest that SlyA may not be involvedspecifically in the natural regulation of clyA. The observed regulatoryeffects on clyA with SlyA (and likely also MprA) may well be ofa more general nature, e.g., competing with H-NS binding at theclyA locus. It has been suggested that SlyA-related proteins playkey roles in the global regulation of diverse aspects of bacterialphysiology (57). It has also been implied that rather than beinga classical transcriptional activator, MprA may act like somehistone-like E. coli proteins, modulating the transcription ofspecific promoters by locally altering DNA topology (14). InSalmonella, SlyA was demonstrated to regulate the expression ofmultiple proteins during stationary phase and during infectionof macrophages (8), but the role of SlyA in E. coli is notyet understood. When present in multiple copies in E. coli K-12,the cloned slyA locus affected the expression of more than 50proteins according to analyses using two-dimensional PAGE (39).This indicates that SlyA may not be specifically linked with theregulation of the H-NS-silenced clyAlocus.

The clyA promoter is dependent on CRP for efficient expression. In addition to the strict control exerted by H-NS, the clyA locus appeared to be controlled by the global regulatory proteinCRP. According to our data CRP is required for efficient ClyAexpression. A much reduced transcription of clyA in hns crp doublemutants compared with hns mutants was evident by using a transcriptionalclyA::lacZ fusion, and in line with these findings a substantialdecrease in cellular ClyA protein and cytolytic activity was observed.The relief of H-NS silencing by SlyA was also much less efficientin the absence of CRP, since only a very weak cytolytic activitycould be detected in CRP-deficient strains overexpressing SlyA(Table 3). Results from DNase I footprint experiments were consistentwith the idea that the role of CRP in ClyA expression is to directlyinteract with the clyA promoter region (Fig. 4). Further evidencesupporting the model that CRP is involved in the expression ofClyA was obtained by altering the sequence of the potential CRPbinding site in the clyA upstream region, both located on theplasmid and on the chromosome (Fig. 5 and 6). By altering theDNA site for CRP to reduce its similarity to the consensus, ClyAexpression was significantly lowered. In contrast, the alteredCRP binding site that matched the consensus more closely resultedin substantially increased ClyA expression in crp⁺ but not crp strains. These findings supported a model in whichthe clyA promoter is dependent on CRP for efficient expression,and where the predicted DNA site for CRP is important for thisregulation.

Anaerobic regulation of clyA involves both CRP and FNR. Results from experiments using a low-copy plasmid-borne clyA promoter-lacZ fusion were consistent with the idea that bothCRP and FNR are involved in the transcriptional regulation ofclyA under anaerobic growth conditions (Fig. 3). Our findingssuggest that FNR and CRP bind to the same sequence in the clyApromoter. There are other examples of binding of FNR and CRP tothe same site (48). Evidently, CRP, and not FNR, was requiredfor the expression of ClyA in hns mutants under anoxic conditions,although it appeared that FNR could partly complement CRP. Wealso observed that the clyA-lacZ fusion in the wild-type strain(M182) was expressed at a higher level (more than twofold) duringanaerobic growth, suggesting that the clyA locus may be less repressedin the absence than in the presence of oxygen. It was shown previouslythat when expressed in anaerobically grown E. coli K-12, the FNRhomolog HlyX of A. pleuropneumoniae and, although much less effective,FNR, are able to activate ClyA expression, presumably by bindingto the FNR binding site in the clyA upstream region (21).

The clyA promoter: an H-NS silenced class I promoter. Unlike the situation in eukaryotes, where gene expression is thought to be generally repressed by packaging of the DNA intonucleosomes, the DNA of prokaryotes is generally considered tobe available for transcription at all times (55). There are,however, certain prokaryotic gene loci that are apparently notexpressed under tested growth conditions. Such loci are referredto as cryptic, and some of them are efficiently silenced by thenucleoid-associated protein H-NS (3, 62). The clyA locusis an interesting new example of H-NS-silenced operons. The locushas some features in common with the cryptic $beta$ -glucoside (bgl)operon of E. coli, which is thought to be kept in a silenced stateby a repressing nucleoprotein complex consisting of H-NS and othercellular factors. The complex renders the bgl promoter inaccessibleto RNA polymerase and CRP (49). Silencing of the bgl operonis relieved by various mutations, including (i) mutations in hns(initially termed bglY) (12, 20) and in genes encoding thesubunits of DNA gyrase (15), (ii) integration of insertion elementsin cis to the promoter (44), and (iii) deletion of either oneof the silencer sequences (32). These mutations may all, directlyor indirectly, affect the locked conformation of the upstreamregion so that they allow more-efficient transcription at thebgl promoter. In addition, point mutations that improve the CRPbinding site within the bgl promoter, resulting in CRP bindingwith higher affinity, cause activated bgl transcription (45).It appears that clyA, similar to the bgl operon, has a weak promoterand no classical operator site. The presence of a $-$ 10 promoterbox (TATGAAT) centered at $-$ 9, a $-$ 35 sequence (TTGACG) centeredat $-$ 32.5, and binding sites for CRP and FNR centered at $-$ 61.5suggested that this clyA promoter is a class I promoter that couldbe transcriptionally activated by CRP or FNR. Another case ofan H-NS silenced operon in which CRP has a positive role is thepap fimbrial adhesin determinant found in uropathogenic E. coli(19). However, transcription of pap is independent of CRP activationin the E. coli K-12 mutant lacking H-NS (18). That finding ledto the suggestion of a new role for CRP: it can mediate its positiveregulatory function by alleviating transcriptional silencing.In contrast to the situation found in the clyA locus, the bindingsite for CRP in pap is located relatively far from the promotersand the protein-DNA interaction there is rather clearly shownby in vitro footprint analysis (19). It is possible that CRPmay also alleviate the action of H-NS in the case of clyA, e.g.,by altering the local DNA conformation and/or by interfering withits DNA binding. An indication of such a role was obtained whenthe CRP site on the chromosome was altered to perfectly matchthe consensus, resulting in derepression of the clyA gene. However,the results were also consistent with the suggestion that CRPdirectly interacted with the RNA polymerase. The genetic evidencesuggested a positive role for CRP both in the absence of H-NSand during SlyA overproduction. The suboptimal design of its bindingsite in the clyA DNA evidently did not allow for any efficientCRP-mediated alleviation of H-NS silencing, but there was a needfor additional factors. The tight control of clyA transcriptionin wild-type E. coli during laboratory cultivation is intriguing,and it remains to be seen if there are different pathways forinduction of its expression. For example, it will be of interestto consider whether or not CRP may act in direct cooperation withother factors under some conditions. It is also possible thatexpression of ClyA could be initiated at some stage during aninfection process, as has been shown for the bgl operon (27).Considering the potent cytotoxic properties of this cytolysin,it appears reasonable that it would be strictly regulated, especiallyin nonpathogenicstrains.

	ACKNOWLEDGMENTS

We thank Monica Persson for skillful technical assistance and J. R. Guest for kindly providing fnrplasmids.

This work was supported by grants from the Swedish Natural Science Research Council, the Swedish Medical Research Council,and the Göran Gustafsson Foundation for Research in Natural SciencesandMedicine.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, Umeå University, S-90187 Umeå, Sweden. Phone: 46-90-7856731.Fax: 46-90-772630. E-mail: bernt.eric.uhlin{at}micro.umu.se.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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31. Link, A. J., D. Phillips, and G. M. Church. 1997. Methods for generating precise deletions and insertions in the genome of wild-type Escherichia coli: application to open reading frame characterization. J. Bacteriol. 179:6228-6237[Abstract/Free Full Text].

32. Lopilato, J., and A. Wright. 1990. Mechanisms of activation of the cryptic bgl operon of Escherichia coli K-12, p. 435-444. In K. Drlica, and M. Riley (ed.), The bacterial chromosome. American Society for Microbiology, Washington, D.C.

33. Lucht, J. M., P. Dersch, B. Kempf, and E. Bremer. 1994. Interactions of the nucleoid-associated DNA-binding protein H-NS with the regulatory region of the osmotically controlled proU operon of Escherichia coli. J. Biol. Chem. 269:6578-6586[Abstract/Free Full Text].

34. Ludwig, A., S. Bauer, R. Benz, B. Bergmann, and W. Goebel. 1999. Analysis of the SlyA-controlled expression, subcellular localization and pore-forming activity of a 34 kDa haemolysin (ClyA) from Escherichia coli K-12. Mol. Microbiol. 31:557-567[CrossRef][Medline].

35. Ludwig, A., C. Tengel, S. Bauer, A. Bubert, R. Benz, H. J. Mollenkopf, and W. Goebel. 1995. SlyA, a regulatory protein from Salmonella typhimurium, induces a haemolytic and pore-forming protein in Escherichia coli. Mol. Gen. Genet. 249:474-486[CrossRef][Medline].

36. Mekalanos, J. J. 1992. Environmental signals controlling expression of virulence determinants in bacteria. J. Bacteriol. 174:1-7[Free Full Text].

37. Miller, J. H. 1972. Experiments in molecular genetics. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

38. Miller, V. L., and J. J. Mekalanos. 1988. A novel suicide vector and its use in construction of insertion mutations: osmoregulation of outer membrane proteins and virulence determinants in Vibrio cholerae requires toxR. J. Bacteriol. 170:2575-2583[Abstract/Free Full Text].

39. Oscarsson, J. 1999. Ph.D. thesis. Umeå University Medical Dissertations, New Series no. 628, Umeå, Sweden.

40. Oscarsson, J., Y. Mizunoe, L. Li, X. H. Lai, Å. Wieslander, and B. E. Uhlin. 1999. Molecular analysis of the cytolytic protein ClyA (SheA) from Escherichia coli. Mol. Microbiol. 32:1226-1238[CrossRef][Medline].

41. Oscarsson, J., Y. Mizunoe, B. E. Uhlin, and D. J. Haydon. 1996. Induction of haemolytic activity in Escherichia coli by the slyA gene product. Mol. Microbiol. 20:191-199[Medline].

42. Owen-Hughes, T. A., G. D. Pavitt, D. S. Santos, J. M. Sidebotham, C. S. Hulton, J. C. Hinton, and C. F. Higgins. 1992. The chromatin-associated protein H-NS interacts with curved DNA to influence DNA topology and gene expression. Cell 71:255-265[CrossRef][Medline].

43. Ralph, E. T., J. R. Guest, and J. Green. 1998. Altering the anaerobic transcription factor FNR confers a hemolytic phenotype on Escherichia coli K12. Proc. Natl. Acad. Sci. USA 95:10449-10452<

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