Role of HrcA and CIRCE in the Heat Shock Regulatory Network of Bradyrhizobium japonicum

doi:10.1128/JB.182.1.14-22.2000

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Journal of Bacteriology, January 2000, p. 14-22, Vol. 182, No. 1
0021-9193/0/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Role of HrcA and CIRCE in the Heat Shock Regulatory Network of Bradyrhizobium japonicum

Alexander C. Minder, Hans-Martin Fischer, Hauke Hennecke, and Franz Narberhaus^*

Institut für Mikrobiologie, Eidgenössische Technische Hochschule, CH-8092 Zürich, Switzerland

Received 11 August 1999/Accepted 6 October 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

A large number of bacteria regulate chaperone gene expression by the CIRCE-HrcA system in which a DNA element called CIRCEserves as binding site for the repressor protein HrcA under non-heat-shockconditions. We have cloned the two consecutive genes hrcA andgrpE of Bradyrhizobium japonicum by using a complementation approachthat screened for GrpE function. In vivo and in vitro transcriptmapping demonstrated that both genes are transcribed separatelyfrom RpoH ( $sigma$ ³²)-dependent promoters. To investigate the supposed negative regulatoryfunction of HrcA, we compared the expression of putative targetgenes in the wild type with that in an hrcA mutant. Transcriptionof the CIRCE-associated chaperonin operons groESL₄ and groESL₅,as well as the $beta$ -galactosidase activity derived from correspondinggroE-lacZ fusions, was strongly elevated in the hrcA mutant evenat physiological temperatures. Expression of other heat shockregulons (RpoH or ROSE dependent) was not affected. To study theactivity of HrcA in vitro, we purified a histidine-tagged versionof the protein under nondenaturing conditions. Specific bindingto the CIRCE element was obtained with a soluble fraction of HrcAin gel retardationexperiments.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The survival of a cell depends on its ability to adapt to changing environmental conditions. For a sudden temperature upshift,all organisms cope with the increased amount of misfolded proteinsby an enhanced synthesis of so-called heat shock proteins (Hsps).This collection of proteins consists mainly of chaperones andproteases, which are involved in protein (re)folding and proteindegradation, respectively (for reviews see references 7 and18).

Both eukaryotic and prokaryotic cells have established a number of complex regulatory strategies to tightly control the transcriptionof heat shock genes under any given condition (21, 26, 27).Coordinate expression of heat shock genes in Escherichia coliis mediated by alternative sigma factors which direct the RNApolymerase to specific promoter sequences upstream of these genes.An increase in the cellular concentration of $sigma$ ³² (RpoH) after a sudden temperature upshift results in elevatedtranscription of more than 30 genes of the $sigma$ ³² regulon. The activity and stability of $sigma$ ³² are subject to feedback control by the DnaK machinery, whichsequesters the sigma factor under low-temperature conditions.Binding of $sigma$ ³² to the DnaK system prevents association with the RNA polymerasecore enzyme and promotes degradation of $sigma$ ³² by the FtsH protease. After a heat shock, denatured proteinspresumably titrate the DnaK chaperones away from $sigma$ ³², leaving the latter stable and competent for complex formationwith RNA polymerase (for recent reviews see references 14 and53).

In contrast to the positive regulation by alternative sigma factors, heat shock expression in a majority of bacteria was foundto be controlled by negative regulation (summarized in reference27). Our knowledge of such systems is far less advanced thanthat of the E. coli-type regulation. The regulatory principleis often based on a specific interaction between a repressor proteinand a DNA element that is located in the promoter regions of heatshock genes. Repression is relieved upon a temperature upshift,thereby allowing transcription of the downstream genes. A widespreadnegative control mechanism consists of the repressor protein HrcAand a DNA element called CIRCE (for controlling inverted repeatof chaperone expression [54]). The first evidence that thishighly conserved inverted repeat might act as a negative cis elementwas obtained by the observation that mutations in one or botharms of the inverted repeat resulted in elevated transcriptionof the downstream genes even at normal growth temperatures (47,54). Chromosomal mutations in Bacillus subtilis which affectedthe expression of CIRCE-dependent genes were localized in orf39,the first gene of the dnaK operon (44, 51). Disruption oforf39 in B. subtilis and of the equivalent gene in Caulobactercrescentus confirmed the function of the Orf39 protein as a negativeregulator of CIRCE-dependent genes and led to its designationas HrcA (for heat regulation at CIRCE) (38, 43). By analogywith the feedback control of $sigma$ ³² activity and stability by the DnaK machinery in E. coli, theactivity of B. subtilis HrcA was found to be modulated by theGroE chaperonin system (25). A direct correlation between thecellular GroESL level and HrcA activity suggested that the repressorrequires chaperonins for proper function in vivo (3, 25).Accordingly, heat stress would render HrcA inactive because GroESand GroEL become engaged in the refolding of denaturedproteins.

Unfortunately, attempts to confirm the proposed HrcA-CIRCE and HrcA-GroEL interactions in vitro were hampered by the insolubilityof overproduced HrcA, which tends to form inclusion bodies, requiringpurification under denaturing conditions. Despite this shortcoming,it has been possible to visualize the binding of purified HrcAof Staphylococcus aureus to the CIRCE element by atomic forcemicroscopy (35) and to document CIRCE binding of purified Bacillusstearothermophilus HrcA in gel retardation experiments (25).

An unusually complex network of both positive and negative regulatory mechanisms controls transcription of heat shock genesin Bradyrhizobium japonicum, the nitrogen-fixing root nodule symbiontof soybeans (27). Three different regulatory systems have beenidentified so far. One class of heat shock genes is transcribedfrom $sigma$ ³²-dependent promoters. The search for the corresponding sigma factorrevealed the existence of three disparately regulated rpoH geneswhose $sigma$ ³²-like products have different promoter specificities (30, 31).The expression of a second class of heat shock genes is negativelycontrolled by a highly conserved DNA element called ROSE (forrepression of heat shock gene expression) (29). Evidence fora third class of heat shock genes was deduced from the presenceof a CIRCE element in the promoter region of the heat shock-induciblechaperonin operons groESL₄ and groESL₅ (3). Elevated transcriptionfrom the groESL₄ promoter at normal temperatures, caused eitherby a deletion of 4 bp within the corresponding CIRCE element orby disruption of groEL₄, had clearly demonstrated the regulatoryfunction of CIRCE and, moreover, had indicated the presence ofa feedback regulatory mechanism. According to these observations,the existence of a CIRCE-specific repressor protein whose stabilityor activity or both are modulated by chaperonins wassuggested.

Here, we report the cloning of the B. japonicum hrcA gene and the assignment of its position in the complex heat shock networkof this organism. The function of the HrcA protein as a CIRCE-specificrepressor protein is demonstrated by a complementary set of invivo and in vitroexperiments.

	MATERIALS AND METHODS

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Bacterial strains, plasmids, and growth conditions. The bacterial strains and plasmids used in this work are listed in Table 1. E. coli cells were grown in Luria-Bertani medium(22) supplemented with ampicillin (200 µg/ml), chloramphenicol(20 µg/ml), kanamycin (30 µg/ml), or tetracycline (10 µg/ml) ifrequired. The growth temperature for E. coli strains was 37°Cexcept for E. coli DA259 (grpE mutant), which was grown at 30°C.B. japonicum strains were propagated aerobically at 30°C in PSYmedium (37) supplemented with 0.1% (wt/vol) arabinose. If appropriate,antibiotics were added at the following concentrations: chloramphenicol,20 µg/ml (for counterselection against E. coli donor strains);kanamycin, 100 µg/ml; spectinomycin, 100 µg/ml; and tetracycline,50 µg/ml.

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TABLE 1. Bacterial strains and plasmids used in this study

DNA manipulations. Recombinant DNA techniques were performed according to standard protocols (40). Construction of B. japonicum mutants bycointegrate formation or marker exchange mutagenesis and isolationof chromosomal DNA from B. japonicum were performed as describedpreviously (15). Southern blot hybridizations with digoxigenin-11-dUTP-labeledDNA probes were performed according to the manufacturer's instructions(Boehringer Mannheim). DNA was sequenced by the chain terminationmethod (41) with an ABI PRISM 310 genetic analyzer (AppliedBiosystems, Foster City, Calif.). The DNA region was sequencedand the deduced proteins were analyzed with the software packageof the Genetics Computer Group of the University of Wisconsin,Madison (version 8.0) and the National Center for BiotechnologyInformation BLAST network server. The CODONPREFERENCE programwas applied by using the B. japonicum codon usage table (36).

Construction of strains and plasmids. For the construction of hrcA deletion mutants the 2.0-kb NotI (position 2 in Fig. 1)-XmnI (position 2015) fragment of pRJ5530was ligated into the 6.7-kb NotI-SmaI vector fragment of pSUP202pol4.In the resulting plasmid the 561-bp SalI (position 706)-XhoI (position1267) internal fragment of hrcA was replaced by the 1.2-kb SalIfragment of pBSL15 containing the neomycin phosphotransferaseII cassette (Km^r). Both orientations of the resistance cassette relative to thehrcA gene were obtained, but for the subsequent work we used plasmidpRJ5549, in which the remaining portion of the hrcA gene and theresistance cassette are oriented in opposite directions. PlasmidpRJ5549 was mobilized from E. coli S17-1 into B. japonicum 110spc4for marker replacement mutagenesis, yielding strain 5549 (Fig.1).

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FIG. 1. Physical map of the B. japonicum hrcA gene region. Numbers indicate start and stop codon positions of open reading frames, the transcription start sites (horizontal arrows above gene map), the beginning (position 1) and the end (position 7681) of the sequenced gene region, and recognition sites of the following restriction enzymes: E, EcoRI; N, NotI; S, SalI; X, XhoI. The restriction site in parentheses was destroyed during the cloning procedure. The strategy to construct the B. japonicum hrcA deletion resulting in strain 5549 is indicated. The inserts of plasmids pRJ5523 and pRJ5530 are shown below the physical map.

In order to compare the expression of heat shock genes in a wild-type background with that in an hrcA mutant background, suitabletranslational lacZ fusions present on pSUP202pol4 derivates werecointegrated via homologous recombination into the chromosomeof wild-type B. japonicum and 5549 (Table 1). The correct genomicstructure of all mutant strains was confirmed by Southern blothybridization with appropriate digoxigenin-11-dUTP-labeled DNAprobes.

Plasmids used as templates for in vitro transcription experiments were based on pRJ9519, which contains the B. japonicum rrnterminator and in which different promoter regions were introduced(30). Plasmid pRJ5542 carries a 537-bp NotI (position 2 in Fig.1)-NruI (position 538) fragment containing the B. japonicum hrcApromoter region. The promoter region of B. japonicum grpE wasintroduced as a 691-bp SacI (position 1109)-FspI (position 1796)fragment yielding plasmidpRJ5543.

To construct the overproduction plasmid pRJ5552, the hrcA gene was amplified from plasmid pRJ5530 by PCR with Taq DNA polymerase.The oligonucleotides used as primers were designed such that theyintroduced an NdeI recognition site overlapping the start codonand a NotI site immediately downstream of the stop codon of hrcA.The PCR-generated fragment was cut with both NdeI and NotI andligated into pET28a(+) digested with the same enzymes. The encodedrecombinant protein H₆-HrcA possesses an N-terminal extensionof 20 amino acids adding 2.1 kDa to the molecular mass of HrcA(39.2 kDa). The correct nucleotide sequence of the PCR-amplifiedhrcA fragment was confirmed by sequencing plasmidpRJ5552.

Transcript mapping. RNA isolation and primer extension analysis were performed as described previously (3). The following oligonucleotideswere used to determine the transcription start sites upstreamof hrcA and grpE: HrcA10 (hrcA; position 579), 5'-CAGCCGGGAAATATTGCGTGAGCCCACC-3';HrcA11 (hrcA; position 630), 5'-CAGATCGGCCATGACGTTGCGAACCGAG-3';GrpE4 (grpE; position 1742), 5'-CTTCCTTCTGCAACAGCTCGACCGAGCC-3';GrpE5 (grpE; position 1700), 5'-CGGGCATGATGTAGGGCTTCGACACCAC-3'.The numbers in parentheses indicate the positions of the 5' endsbased on the numbering used in the physical map shown in Fig.1.

In vitro transcription. Single-round transcription assays with B. japonicum RNA polymerase holoenzyme and core enzyme reconstituted with purifiedRpoH₂ were carried out as described previously (5, 30). SuitableRNA size markers were synthesized in vitro with T7 or T3 RNA polymeraseand with linearized pBluescript-based plasmids astemplates.

$beta$ -Galactosidase assay. B. japonicum cells were grown aerobically to exponential phase at 30°C in PSY medium with spectinomycin as the only antibiotic.The $beta$ -galactosidase assay was performed as described previously(22).

Overproduction and purification of H₆-HrcA. Freshly transformed E. coli BL21/pLysS cells carrying pRJ5552 were used for overproduction of H₆-HrcA. The cells were grownat 30°C in 1 liter of Luria-Bertani LB medium containing chloramphenicoland kanamycin. When the cultures had reached an optical densityat 600 nm of 0.5, production of the recombinant protein was inducedby addition of 0.1 mM isopropyl- $beta$ -D-thiogalactopyranoside (IPTG).After 2 h, the cells were harvested, washed, resuspended in 20ml of TEPDM buffer (50 mM Tris-HCl [pH 8.0], 1 mM EDTA, 1 mM phenylmethylsulfonylfluoride, 2 mM dithiothreitol, 25 mM MgCl₂, 100 mM KCl), and disruptedin a French pressure cell. The soluble protein fraction was obtainedby removing the cell debris and membranes in two subsequent centrifugationsteps at 4°C (1.5 h at 30,000 × g [Sorvall SS-34 rotor] and 1h at 116,000 × g [Beckman SW55 Ti rotor]).

All of the following purification steps were performed at 4°C. Binding buffer (8×) was added to the supernatant fraction toa final concentration of 500 mM NaCl before loading the fractiononto a 1.5-ml Ni-nitrilotriacetic acid-agarose column (Qiagen,Basel, Switzerland) which had been equilibrated with 1× bindingbuffer (20 mM Tris-HCl [pH 7.9], 500 mM NaCl, 5 mM imidazole).The column was washed with 15 ml of 1× binding buffer and thenwith 4.5 ml of 1× binding buffer containing 120 mM imidazole.The H₆-HrcA protein was eluted with 4.5 ml of 1× binding buffercontaining 300 mM imidazole and collected in fractions of 0.5ml. The fractions with the highest protein concentrations werepooled, dialyzed for 2 h against storage buffer (20 mM Tris-HCl[pH 8], 200 mM NaCl, 10% glycerol) and centrifuged at 13,000 ×g for 1 min. Aliquots of the supernatant were stored at $-$ 80°C.The concentration of purified H₆-HrcA protein was determined bythe Bradford method (6).

Gel retardation assay. The DNA-binding activity of H₆-HrcA was tested in gel shift experiments using a 269-bp PstI-KpnI fragment from pRJ5558 containingthe promoter region and the CIRCE element of groESL₅, a 168-bpHpaI-KpnI fragment from pRJ5556 containing the promoter regionand the CIRCE element of groESL₄, a 104-bp PCR amplification productcontaining the 5' region of the groESL₄ promoter region, or a94-bp PCR-generated fragment containing either the wild-type CIRCEelement of groESL₄ (CTAGCACTCgcgggcacaGACTGCTAA [nucleotides ininverted repeat shown in uppercase letters and nucleotides identicalto those in consensus sequence are underlined]) or a mutated DNAfragment in which the consensus sequence had been replaced (AGCTACAGAgcgggcacaAGACATCGA)(see Fig. 6B; CIRCE consensus sequence: TTAGCACTC-N₉-GAGTGCTAA[17]). These DNA fragments were purified from agarose gels andend labeled with [ $gamma$ -³²P]ATP according to standard protocols. Labeled fragments (25,000cpm; approximately 10 to 20 fmol of DNA) were mixed with purifiedH₆-HrcA protein in DNA binding buffer (12 mM HEPES [pH 7.9], 4mM Tris-HCl [pH 8], 6 mM KCl, 3 mM MgCl₂, 0.5 mM dithiothreitol,6 mM EDTA; Stratagene, La Jolla, Calif.) in a final volume of25 µl. If appropriate, the E. coli chaperones DnaK, DnaJ, andGrpE or GroES and GroEL (Epicentre Technologies, Madison, Wis.)were added to H₆-HrcA, and the mixture was preincubated at roomtemperature for 10 min in DNA binding buffer containing ATP (1.2mM) and magnesium acetate (23 mM) before the binding reactionwas started by the addition of DNA. The DNA-protein mixtures wereincubated for 5 or 10 min at room temperature, mixed with 5 µlof loading dye (30% glycerol, 0.02% bromphenol blue in water),and then loaded onto 6% nondenaturing polyacrylamide gels (cross-linkerratio of 29:1 in 1× TBE buffer [pH 8; 89 mM Tris base, 89 mM boricacid, 2.5 mM EDTA]) containing 1 mg of Triton X-100/ml. Gels wererun in 1× TBE buffer at 4°C, dried under vacuum, and exposed ona phosphorimager screen. Signal intensities of free DNA and retardedbands were quantified with a phosphorimager and the program ImageQuant(version 3.3; Molecular Dynamics, Sunnyvale, Calif.).

Plant infection test. The symbiotic phenotype of the B. japonicum hrcA mutant was determined in a soybean plant infection test as described previously(12, 15).

Nucleotide sequence accession numbers. The nucleotide sequence of the B. japonicum hrcA and dnaK gene region has been deposited in the GenBank-EMBL database underaccession no. Y09633.

	RESULTS

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Cloning the B. japonicum hrcA gene region. In contrast to those of several other organisms, the B. japonicum hrcA gene is not part of the dnaK operon (23). Our initialattempts to identify the gene by heterologous hybridization withDNA or oligonucleotide probes derived from hrcA homologs failed.The fact that the C. crescentus hrcA gene is closely linked togrpE (38) prompted us to search first for a grpE homolog ofB. japonicum by a complementation approach. Assuming that B. japonicumGrpE would be functional in E. coli, we attempted to rescue theheat-sensitive grpE-deficient E. coli strain DA259 (kindly providedby D. Ang, Geneva, Switzerland) with B. japonicum DNA cloned intopUC18. The inability of this strain to grow at 39 or 42°C couldbe fully complemented by the presence of plasmid pRJ5523, whichcontains a 3.9-kb EcoRI fragment of B. japonicum (Table 2; Fig.1). DNA sequence analysis revealed an open reading frame codingfor a protein with a high degree of similarity to all known GrpEproteins. As we had hoped, an open reading frame (3' end) codingfor the C terminus of an HrcA-like protein was present upstreamof grpE. Incidentally, the 5' end of B. japonicum dnaK was foundonly 2.4 kb downstream of the hrcA-grpE cluster (Fig. 1). Thecomplete B. japonicum hrcA region was subcloned as a 3-kb NotIfragment originating from a suitable cosmid, resulting in plasmidpRJ5530 (Fig. 1).

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TABLE 2. Temperature-dependent growth of E. coli DA259 transformed with different plasmids

To address the question of whether there is more than one copy of the hrcA or grpE gene in the B. japonicum chromosome, asit is the case for groESL (10) and rpoH (32), suitable hrcAand grpE probes were hybridized under low-stringency conditions(5× SSC [1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate], 56°C)with B. japonicum chromosomal DNA that had been digested withdifferent restriction enzymes. No evidence for an hrcA or grpEgene family wasobtained.

Nucleotide sequence of the hrcA gene region. The DNA sequence of the B. japonicum hrcA gene region, extending from the NotI site at position 2 to the XhoI site at position3451, was established (Fig. 1), expanding the previously describedsequence of the dnaKJ gene region (23). Significant similaritiesof the deduced amino acid sequences to sequences of C. crescentusHrcA (54% identical amino acids) and GrpE (44%) (38) led tothe more precise assignment of B. japonicum hrcA (position 433to 1521) and grpE (position 1619 to 2224). The hrcA gene beginswith the alternative start codon GTG and encodes a predicted proteinof 362 amino acids (M_r, 39,165). An alignment of the B. japonicumhrcA product with 18 HrcA-like proteins deposited in the publiclyavailable databases displayed only limited sequence similarity(overall sequence identity generally around 30% with the exceptionof HrcA proteins from related organisms, such as B. japonicum,Agrobacterium tumefaciens, and C. crescentus, that have about50% identical amino acids). The similarity is restricted mainlyto three previously described conserved regions (43).

The deduced gene product of grpE consists of 201 amino acids and has a molecular weight of 21,655. Further investigation ofthe DNA region upstream of dnaK and hrcA revealed three additionalopen reading frames, all divergently oriented to hrcA and dnaK.The first open reading frame (orf>86) starts at position 258 andcodes for the amino-terminal end of a polypeptide of at least86 amino acids with a high degree of sequence similarity to theputative tRNA nucleotidyltransferase RnpH of C. crescentus (67%identical amino acids) encoded by the rph gene (38). Moreover,the genetic organization of orf>86, hrcA, and grpE is similarto that of C. crescentus. The gene product of orf240 (M_r, 25,406)shows a high degree of sequence similarity to pyrazin nicotinamidases(e.g., 41% of the amino acids are identical to those of the putativepncA gene product of Aquifex aeolicus [8]). The orf313 product(M_r, 33,241) exhibits no significant similarity to any known proteinsequence in thedatabase.

Transcriptional analysis of the hrcA gene region. The transcription start sites within the B. japonicum hrcA gene region were determined by primer extension analysis with oligonucleotidescomplementary to the 5' ends of hrcA and grpE. A single startsite was detected for each gene: 21 nucleotides upstream of theproposed translational start site of hrcA (Fig. 2A) and 36 nucleotidesupstream of grpE (Fig. 2B). Both transcripts were clearly heatinducible, as indicated by 2.3- and 19-fold increases of the reversetranscription products for hrcA and grpE, respectively, aftera 30-min temperature shift of the cells from 30 to 43°C. The deducedpromoter regions displayed characteristic sequence motifs of heat-inducible $sigma$ ³²-dependent promoters (Fig. 2C).

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FIG. 2. Determination of the transcription start sites of hrcA (A) and grpE (B) by primer extension mapping. Total RNA was isolated from B. japonicum 110spc4 cells harvested before (0) and 30 min after a heat shock from 30 to 43°C (30). The extension and sequencing reactions (TCGA) were performed with the primers HrcA11 (A) and GrpE4 (B). The transcription start sites are marked with arrows, and the deduced promoter sequences are shown below (C). Nucleotides matching those of the E. coli $sigma$ ³² consensus promoter (52) and transcriptional start sites are in boldface.

The presumed $sigma$ ³²-dependent transcription of hrcA and grpE was further confirmed by in vitro transcription of both genes withthe B. japonicum core RNA polymerase reconstituted with purifiedRpoH₂-H₆ protein, a C-terminally histidine-tagged version of thisprotein. The RpoH₂ factor is responsible for expression of $sigma$ ³²-dependent genes under normal growth conditions. The resultinghrcA and grpE transcripts derived from plasmids pRJ5542 and pRJ5543,respectively, are of the expected lengths (286 and 373 nucleotides,respectively; Fig. 3), as judged from a comparison with RNA sizemarkers (not shown) and the dnaKJ transcript (358 nucleotides),which was previously shown to be synthesized efficiently by coreRNA polymerase reconstituted with RpoH₂-H₆ (Fig. 3A) (30). Thecore enzyme alone produced only small amounts of transcript (Fig.3A), most probably due to some residual $sigma$ ³² protein present in the preparation, as described elsewhere (30).Similarly, hrcA and grpE transcripts were obtained with the B.japonicum RNA polymerase holoenzyme, which contains a significantamount of RpoH protein (30). According to these results we concludethat hrcA and grpE belong to the rpoH regulon of B. japonicumtogether with the genes coding for the DnaK machinery.

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FIG. 3. In vitro transcription from the B. japonicum grpE and dnaK (A) and hrcA (B) promoters. The enzymes used were B. japonicum RNA polymerase core enzyme (Core), purified RpoH₂-H₆ protein (RpoH₂), and B. japonicum RNA polymerase holoenzyme (Holo). Plasmids pRJ5099, pRJ5542, and pRJ5543 were used as templates to transcribe the 5' ends of dnaK, hrcA, and grpE, respectively. Numbers on the left mark transcript lengths (in nucleotides) of the expected transcripts; lengths were confirmed with suitable in vitro-synthesized RNA size markers (not shown). The signal extending across the entire gel (A) was caused by overloaded RNA size markers on the left.

Heat shock gene expression in an hrcA deletion mutant. The B. japonicum hrcA mutant 5549 was constructed by replacing an internal hrcA fragment with a kanamycin resistance cassette(Fig. 1; see also Materials and Methods). The effect of the hrcAdeletion on the expression of heat shock genes was determinedby both primer extension analysis and $beta$ -galactosidase measurementsof suitable translational lacZfusions.

The analysis of RNA isolated from wild-type B. japonicum and strain 5549 revealed strongly derepressed transcription of theCIRCE-dependent genes groESL₄ and groESL₅ under non-heat-shockconditions (Fig. 4). The transcription intensity slightly surpassedeven the intensity of heat-induced transcription after a 30-minheat shock from 30 to 43°C. By contrast, transcription of $sigma$ ³²-dependent genes (e.g., groESL₁ and hrcA) and heat shock genesregulated by the ROSE element (e.g., hspA) was not influencedby the lack of HrcA. In line with the absence of a CIRCE elementupstream of B. japonicum hrcA, the gene is not subject to autoregulationas it is in B. subtilis (43).

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FIG. 4. Effect of an hrcA mutation on the transcription of different heat shock genes in B. japonicum. Total RNA was isolated from wild-type (WT) B. japonicum and 5549 (hrcA mutant) cells harvested before (0) and 30 min after a heat shock from 30 to 43°C (30) and analyzed by primer extension experiments. The extension reactions were performed with the primers ES5UP2 (groESL₅) (3), 702 (groESL₄ and groESL₁) (3), HrcA11 (hrcA), and Sig107 (hspA) (29). The mode of regulation of each gene or operon is indicated.

Table 3 shows the expression of different lacZ fusions that were integrated into the chromosome of wild-type B. japonicumand strain 5549 (see Materials and Methods for the constructionof the strains). The two CIRCE-regulated fusions (groEL₄'-'lacZand groEL₅'-'lacZ) exhibited an increased expression in the absenceof HrcA, which supports the primer extension results. However,the calculated induction factors (3.2 for groEL₄'-'lacZ and 2.3for groEL₅'-'lacZ) appeared to be lower as compared with the stronglyincreased transcription of the corresponding genes in strain 5549(Fig. 4). This is probably due to a posttranscriptional effectof CIRCE, which functions as an mRNA destabilizer promoting therapid turnover of CIRCE-containing transcripts (19, 50).

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TABLE 3. Effect of an hrcA deletion on the expression of chromosomally integrated 'lacZ fusions in B. japonicum

The lack of HrcA did not affect the expression of the lacZ fusions to groEL₁, grpE and dnaK ( $sigma$ ³² regulated), hspA (ROSE regulated), and groEL₂ (constitutivelyexpressed) (Table 3). The finding for groEL₂ supports an earliernotion that the putative element homologous to CIRCE in the promoterregion of groESL₂ might not be functional (3). Although transcriptionfrom the hrcA promoter was not influenced by a deletion of thecorresponding gene (Fig. 4), the expression of the hrcA'-'lacZfusion was increased 2.8-fold in strain H5559 (Table 3). Posttranscriptionalevents, not further investigated here, might be responsible forthiseffect.

Complementary evidence that derepression of the groESL₄ and groESL₅ operons in the hrcA mutant raised the cellular GroEL poolwas obtained from immunoblots performed with anti-E. coli GroELserum and by two-dimensional gel analysis (data notshown).

Phenotypic characterization of an hrcA deletion mutant under symbiotic and heat shock conditions. As it was known that GroEL is critical for nitrogen fixation in B. japonicum (11), we tested whether the elevated GroESL₄and GroESL₅ concentrations in the hrcA mutant would affect theperformance of B. japonicum in root nodule symbiosis and underheat stress conditions. Strain 5549 (hrcA mutant) was indistinguishablefrom the wild-type strain with respect to the ability to nodulatesoybean roots and to fix nitrogen. Strain 5549 was further analyzedfor its ability to survive a temperature upshift from 30 to 48°C,which is lethal to wild-type B. japonicum (33). The survivalrate of strain 5549 after exposure to the nonpermissive temperatureshowed no significant deviation from that for the wild type. Sincethe elevated GroEL concentration caused by the hrcA deletion didnot improve the heat tolerance of B. japonicum, we conclude thatthe GroEL pool in wild-type B. japonicum cells is not limitingunder the conditionstested.

Purification of soluble H₆-HrcA. To obtain in vitro evidence for a physical interaction between CIRCE and HrcA we aimed at performing gel retardation assayswith purified components. To this end, an amino-terminally histidine-taggedversion of B. japonicum HrcA (H₆-HrcA) was expressed in E. coli.In contrast to overproduced HrcA from other organisms, a largefraction of B. japonicum H₆-HrcA remained in the supernatant evenafter ultracentrifugation (Fig. 5). This allowed purificationunder nondenaturing conditions, yielding approximately 4 mg ofpurified protein per liter of E. coli culture.

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FIG. 5. Overexpression and purification of H₆-HrcA. Crude extracts of the H₆-HrcA-overproducing E. coli strain harvested before and after induction with IPTG, aliquots from each purification step, and 2 µl of the dialyzed protein fraction, which was subsequently used for in vitro experiments, were separated on an SDS-12% polyacrylamide gel. The proteins were stained with Coomassie blue. Supernatants 1 and 2 mark aliquots of the soluble protein fraction after centrifugation at 30,000 and 116,000 × g, respectively (see Materials and Methods). The apparent molecular masses (in kilodaltons) of H₆-HrcA (41.3) and the marker proteins are indicated.

Specific binding of purified HrcA to CIRCE. Gel retardation experiments with increasing amounts of H₆-HrcA and with radioactively labeled DNA fragments containing CIRCEand the promoter region of groESL₄ or groESL₅ showed a protein-dependentDNA retardation (Fig. 6A). The groESL₄ fragment was used to furtherdelineate the DNA region responsible for HrcA binding (Fig. 6B).Clear DNA binding of H₆-HrcA was observed only with the 94-bpsubfragment that contained the $-$ 10 promoter region and CIRCE (Fig.6C), not with a comparable fragment in which the CIRCE elementwas replaced by a sequence that had no similarity to CIRCE (Fig.6D; for details see Materials and Methods). The fact that evenvery high concentrations of the repressor (approximately a 100,000-foldmolar excess of protein over DNA) did not result in an appreciableband shift with CIRCE₄* clearly demonstrates the requirement ofa CIRCE sequence for HrcA binding.

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FIG. 6. Gel retardation experiments with purified B. japonicum HrcA. DNA-binding reactions were performed with DNA fragments derived from the promoter region of groESL₅ (A) and groESL₄ (A, C, and D). (B) groESL₄ fragments represented schematically. CIRCE₄* represents a DNA fragment in which the CIRCE element was mutated (see Materials and Methods). The amount of H₆-HrcA used is indicated above each lane in all panels. The positions of radiolabeled free DNA (f) and retarded bands (r) are marked.

In an additional set of gel retardation experiments, we attempted to lend support to the concept that the HrcA DNA-bindingactivity might be chaperonin dependent. H₆-HrcA was preincubatedin binding buffer containing either E. coli GroEL and GroES (approximatemolar ratio of protomers of HrcA, GroEL, and GroES, 3:10:1 or3:40:4) or E. coli DnaK, DnaJ, and GrpE (approximate molar ratioof protomers of HrcA, DnaK, DnaJ, and GrpE, 10:10:1:1 or 10:40:4:4).Each DNA binding assay was started by the addition of a radiolabeled168-bp DNA fragment containing the promoter region and the CIRCEelement of groESL₄. The DNA-binding activity of our soluble HrcApreparation was not improved by the presence of either the DnaKor GroE chaperone machinery. In fact, the addition of GroESL ledto a reduction of HrcA-CIRCE complexes (data not shown). In controlexperiments we confirmed that the GroE preparation had chaperoninactivity in the buffer system we used for the gel retardationexperiments. This was done by measuring its ability to reactivateheat-denatured malate dehydrogenase (data notshown).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

This work presents an in-depth in vivo and in vitro investigation of a representative CIRCE-HrcA system, which is responsiblefor a widespread heat shock control mechanism in bacteria. Ithas become evident during the last decade that repressor mechanismsare probably much more abundant among prokaryotes than the E.coli-type $sigma$ ³² control of heat shock genes (27). In B. japonicum, the CIRCEsystem is embedded in a complex regulatory network. To elucidatethe role of CIRCE in this network, it was imperative to clonethe structural gene of HrcA, the putative repressor binding tothis DNA element. The amino acid sequences of known HrcA proteinsdeviate greatly despite the high degree of sequence conservationof the CIRCE elements to which they bind (38, 43). This makesthe search for an hrcA gene with nucleotide probes rather difficult(13). Here, we made use of the close genetic linkage betweenhrcA and grpE that is often observed and established a novel approachthat facilitated the isolation of the B. japonicum hrcA gene bycomplementing a temperature-sensitive, grpE-deficient E. colistrain.

Both hrcA and grpE are transcribed separately from heat-inducible $sigma$ ³²-dependent promoters. The control of the HrcA repressor by a heatshock sigma factor demonstrates that different regulatory mechanismsinvolved in the B. japonicum heat shock response do not act independentlybut form a complex network. Evidence for a similar network ofpositive and negative heat shock regulatory mechanisms was alsoobtained from C. crescentus, in which hrcA transcription dependson a heat-inducible $sigma$ ³²-like promoter (38). Moreover, its groESL operon is subjectto dual control by a heat-inducible $sigma$ ³²-dependent promoter and a CIRCE element which is involved in thecell cycle-regulated gene expression (4). Importantly, basalexpression of B. japonicum hrcA at normal growth temperatureswas observed, thus guaranteeing a sufficient amount of HrcA proteinto repress the CIRCE regulon. The sigma factor RpoH₂ appears tobe responsible for this basal transcription, as it is for a certainthreshold level of DnaK (30). Although not proven rigorously,it is reasonable to predict that RpoH₁, the heat shock-inducedRpoH factor of B. japonicum, is responsible for temperature inductionof hrcAexpression.

Elevated levels of GroESL in an hrcA mutant had no influence on free-living growth and symbiotic nitrogen fixation of B. japonicum.Similarly, no obvious effect with regard to growth under normaland stress conditions was observed for C. crescentus and Streptomycesalbus hrcA mutants (13, 38). However, comparable studies ofB. subtilis showed that the hrcA mutant was able to recover froma shift to lethal temperatures whereas the wild type was not (51).A possible reason for this discrepancy between the bacterial specieslies in the fact that B. japonicum, C. crescentus, and S. albushrcA mutants enhance only the concentration of GroE chaperoninswhereas the lack of HrcA in B. subtilis leads to an overexpressionof both chaperone complexes, DnaKJ-GrpE and GroESL. Probably,only increased levels of the complete set of major chaperonesimprove the capacity of bacterial cells to survive temperatureupshifts. This interpretation is also supported by the model inwhich DnaK and GroE chaperone complexes interact with each otherin order to cope with heat shock situations (16).

Previous attempts to perform in vitro studies with HrcA have been impeded by the insolubility of this protein. Gel retardationexperiments could only be performed with cell extracts containingHrcA (9, 20) or with renatured HrcA that had been purifiedunder denaturing conditions (25). By contrast, we found thata large fraction of B. japonicum H₆-HrcA remained in a solubleform upon overproduction and during purification. The reason forthe comparatively high solubility of B. japonicum HrcA remainsunknown at present. Gel mobility experiments performed with thispreparation corroborated the in vivo results in showing a sequence-specificbinding of HrcA to CIRCE. However, a large excess of HrcA overDNA was necessary to obtain a band shift. This might be due toan intrinsic tendency of the repressor to aggregate or to reacha nonfunctional conformation. It should be noted that our B. japonicumHrcA preparation also tended to precipitate from solution overtime. Thus, only a small fraction of the purified protein mightreally be active. Another, physiologically more relevant reasonfor the poor retardation activity might be an inherently weakor transient interaction between CIRCE and its repressor. Thiscould explain why both CIRCE-dependent operons in B. japonicumare only partially repressed in vivo at normal growth temperatures,resulting in an appreciable basal transcription of the correspondinggenes (Fig. 4) (3). Leaky transcription from CIRCE-regulatedpromoters was also reported for B. subtilis, Clostridium acetobutylicum,C. crescentus, and other organisms (28, 38, 42), indicatingthat the CIRCE binding site is not permanently occupied by HrcA.It thus appears that the CIRCE-HrcA system is not designed forcomplete repression of heat shock genes under physiological temperaturesbecause major chaperones are also required for folding processesduring normalgrowth.

There is compelling in vivo evidence that HrcA activity depends on the presence of GroESL (3, 25). The interpretationof these findings was an appealing titration model in which theavailability of GroE chaperones controls HrcA activity. Our failureto simulate this feedback control in vitro appears incompatiblewith this model. While gel retardation of a CIRCE fragment withB. stearothermophilus HrcA was significantly improved in the presenceof GroEL (25), our gel shift experiments showed that the additionof the complete GroE machinery rather impaired the formation ofB. japonicum HrcA-CIRCE complexes. One obvious difference betweenour experiments with B. japonicum HrcA and those with B. stearothermophilusHrcA is that the latter were performed in the presence of 0.5M urea after it had been completely denatured during purification(25). It is thus conceivable that GroEL conferred a rather generalchaperone activity on this partially denatured HrcA preparation,as was indicated by the prevention of HrcA aggregation in thepresence of GroEL. Moreover, it remains unclear why stimulationof gel retardation was observed even in the absence of GroES andATP (25). The prevention of aggregate formation in the presenceof urea might enable partially unfolded HrcA protein to reachan active DNA-binding conformation and, hence, a measurable gelretardation activity with a CIRCE fragment. Experiments with C.acetobutylicum HrcA (OrfA), which had been purified under denaturingconditions, revealed that HrcA aggregation was prevented by theaddition of DnaK, DnaJ, or the whole DnaK chaperone machinery(39), indicating that urea-denatured HrcA is a substrate notonly for the GroE chaperone machinery but also for the DnaK system.While the specific interaction between the CIRCE element and HrcAis well established now, it becomes evident that resolution ofthe more-debated matters of a physical interaction between HrcAand GroEL and the thermosensing by HrcA must await furtherstudies.

	ACKNOWLEDGMENTS

We are indebted to Debbie Ang for providing plasmid pBW401 and the E. coli strains DA258 and DA259, to Christoph Beck forB. japonicum RNA polymerase, and to Michael Kowarik for purifiedB. japonicum RpoH₂-H₆ protein. We thank Christopher Kaestner forhelp in automatic DNA sequencing and Michael Spring, StephanieHäussler, and Domenic Graf for technical assistance. We thankMartin Münchback and Peter James for performing two-dimensionalgelelectrophoresis.

This work was supported by grants from the Swiss National Foundation for Scientific Research and the Federal Institute ofTechnology, Zürich,Switzerland.

	FOOTNOTES

^* Corresponding author. Mailing address: Institut für Mikrobiologie, ETH-Zentrum, Schmelzbergstrasse 7, CH-8092 Zürich, Switzerland.Phone: 41-1-632-2586. Fax: 41-1-632-1148. E-mail: fnarber{at}micro.biol.ethz.ch.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Alexeyev, M. F. 1995. Three kanamycin resistance gene cassettes with different polylinkers. BioTechniques. 18:52-54.
2.	Ang, D., and C. Georgopoulos. 1989. The heat-shock-regulated grpE gene of Escherichia coli is required for bacterial growth at all temperatures but is dispensable in certain mutant backgrounds. J. Bacteriol. 171:2748-2755[Abstract/Free Full Text].
3.	Babst, M., H. Hennecke, and H. M. Fischer. 1996. Two different mechanisms are involved in the heat shock regulation of chaperonin gene expression in Bradyrhizobium japonicum. Mol. Microbiol. 19:827-839[CrossRef][Medline].
4.	Baldini, R. L., M. Avedissian, and S. L. Gomes. 1998. The CIRCE element and its putative repressor control cell cycle expression of the Caulobacter crescentus groESL operon. J. Bacteriol. 180:1632-1641[Abstract/Free Full Text].
5.	Beck, C., R. Marty, S. Kläusli, H. Hennecke, and M. Göttfert. 1997. Dissection of the transcription machinery for housekeeping genes of Bradyrhizobium japonicum. J. Bacteriol. 179:364-369[Abstract/Free Full Text].
6.	Bradford, M. M. 1976. A rapid sensitive method for the quantification of microgram quantities of protein utilizing the principle of protein-dye binding. Anal. Biochem. 72:248-254[CrossRef][Medline].
7.	Bukau, B., and A. L. Horwich. 1998. The Hsp70 and Hsp60 chaperone machines. Cell 92:351-366[CrossRef][Medline].
8.	Deckert, G., P. V. Warren, T. Gaasterland, W. G. Young, A. L. Lenox, D. E. Graham, R. Overbeek, M. A. Snead, M. Keller, M. Aujay, R. Huber, R. A. Feldman, J. M. Short, G. J. Olsen, and R. V. Swanson. 1998. The complete genome of the hyperthermophilic bacterium Aquifex aeolicus. Nature 392:353-358[CrossRef][Medline].
9.	Duchêne, A. M., C. J. Thompson, and P. Mazodier. 1994. Transcriptional analysis of groEL genes in Streptomyces coelicolor A3(2). Mol. Gen. Genet. 245:61-68[CrossRef][Medline].
10.	Fischer, H. M., M. Babst, T. Kaspar, G. Acuña, F. Arigoni, and H. Hennecke. 1993. One member of a groESL-like chaperonin multigene family in Bradyrhizobium japonicum is co-regulated with symbiotic nitrogen fixation genes. EMBO J. 12:2901-2912[Medline].
11.	Fischer, H. M., K. Schneider, M. Babst, and H. Hennecke. 1999. GroEL chaperonins are required for the formation of a functional nitrogenase in Bradyrhizobium japonicum. Arch. Microbiol. 171:279-289[CrossRef].
12.	Göttfert, G., S. Hitz, and H. Hennecke. 1990. Identification of nodS and nodU, two inducible genes inserted between the Bradyrhizobium japonicum nodYABC and nodIJ genes. Mol. Plant-Microbe Interact. 3:308-316[Medline].
13.	Grandvalet, C., G. Rapoport, and P. Mazodier. 1998. hrcA, encoding the repressor of the groEL genes in Streptomyces albus G, is associated with a second dnaJ gene. J. Bacteriol. 180:5129-5134[Abstract/Free Full Text].
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