Background

Bacillus cereus is a common cause of bacterial foodborne disease, characterized by either emetic or diarrhoeal syndromes [1]. Three chromosomally encoded toxins are generally linked to diarrhoeal illness: Haemolysin BL (Hbl) [2], Non-haemolytic enterotoxin (Nhe) [3] and Cytotoxin K (CytK) [4]. Hbl and Nhe are three-component toxins composed of proteins L2, L1 and B, and NheA, NheB and NheC, respectively. The genes encoding all three enterotoxins are found to a similar extent in most species of the B. cereus group [5, 6], and their expression is positively regulated by the PlcR/PapR quorum sensing system [7, 8].

B. cereus NVH 391/98, isolated in 1998 from an outbreak causing fatal enteritis, has been shown to express neither Hbl nor Nhe [9], and was the strain in which CytK was first identified [4]. Phylogenetic studies have shown that this strain is placed uniquely distant from main B. cereus group clusters [10]. It is currently being subjected to complete genome sequencing by the DOE Joint Genome Institute (USA). We previously found that this strain carried a particularly cytotoxic variant of the CytK protein, named CytK-1, which partly explained why NVH 391/98 was highly pathogenic [11]. Results also indicate that the high cytotoxicity of this strain is a result of an exceptionally high level of cytK expression [12]. In earlier studies, in all other strains identified to carry cytK, the toxin existed as a different, less cytotoxic variant, named CytK-2. Recently, we identified two additional B. cereus strains carrying cytK-1: NVH 883/00 and INRA AF2 [13]. In a study performed to elucidate the genetic structure of the B. cereus group, these three strains appear to constitute a cluster genetically remote from all other tested strains (M-H. Guinebretière and C. Nguyen-The, unpublished results). While NVH 391/98 and INRA INRA AF2 were highly cytotoxic, NVH 883/00 was in initial experiments shown to be non-toxic towards Vero cells. The aim of this study was to investigate and compare the strains of this rare genetic group, to potentially gain insight into mechanisms responsible for the dramatic differences in cytotoxicity between strains.

Results

Strains carrying cytK-1 have varying levels of toxicity towards Vero cells

Supernatants collected from late log phase cultures of strains NVH 391/98 and INRA AF2 grown at 32°C and 37°C, as well as strain NVH 391/98 grown anaerobically at 32°C, gave 100% inhibition of protein synthesis in the Vero cell assay, showing that these strains were highly cytotoxic. In contrast, the supernatants tested from NVH 883/00, obtained from cultures grown at 37°C, 32°C, and 25°C, the latter concentrated by a factor of 100, as well as cultures grown anaerobically at 32°C, were shown to have undetectable toxicity in this assay. To determine whether differential CytK expression could be responsible for the varying levels of toxicity, Western immunoblotting of supernatants from all three strains grown at 32°C were performed using CytK antiserum. The results presented in Figure 1 show that NVH 883/00 expressed substantially less CytK than did NVH 391/98 and INRA AF2.

Figure 1
figure 1

Detection of CytK in culture supernatants. Western immunoblot probed with antiserum against CytK. The samples are supernatants from B. cereus strains INRA AF2, NVH 883/00 and NVH 391/98, collected from late log phase cultures grown at 32°C.

A novel variant of Nhe was identified in all three strains

Both strains NVH 391/98 and NVH 883/00 were negative in the Tecra and the Oxoid assays, which are commercial kits that employ monoclonal antibodies directed against NheA and Hbl component L2, respectively, to detect the presence of Nhe and Hbl in B. cereus culture supernatants. Furthermore, all three strains were negative in Western immunoblots using monoclonal antibodies directed against NheA and Hbl component B. However, strains NVH 391/98 and INRA AF2, but not NVH 883/00, were positive in a Western immunoblot using an antibody that is reactive towards both NheB and Hbl component L1, giving a band of the same size as NheB (Figure 2). This was quite unexpected as strain NVH 391/98 had previously been shown to not contain the genes encoding Nhe [4, 9]. PCR experiments using several sets of primers designed on the basis of published sequences of nhe were positive for all three strains with a few of the primer pairs used, thus providing us with a starting point for obtaining the complete sequences of nhe in these strains (see Additional file 1). DNA sequencing of the nhe operons in strains NVH 391/98 and NVH 883/00 revealed a novel variant of nhe, 99.6% identical in DNA sequence between the two strains. The deduced sequences of the three proteins comprising the Nhe toxin, NheA, NheB and NheC, from NVH 391/98 and NVH 883/00 were 77–81%, 87–88%, and 72–74% identical, respectively, to the corresponding protein sequences in B. cereus E33L, ATCC 14579, ATCC 10987, G9241, Bacillus thuringiensis serovar konkukian str. 97–27, serovar israelensis ATCC 35646, and Bacillus weihenstephanensis KBAB4. In comparison, the identities between the Nhe proteins in this set of strains were 96–99%, 97–100%, and 91–99%, respectively.

Figure 2
figure 2

Detection of NheB in culture supernatants. Western immunoblot of culture supernatants from B. cereus strains INRA AF2, NVH 883/00, NVH 391/98, NVH 0075/95 and ATCC 14579 detected using the 1C2 antibody, reactive against both NheB and Hbl component L1. Samples were collected from late log phase cultures grown at 32°C. NVH 0075/95 and ATCC 14579 were used as controls; NVH 0075/95 does not contain hbl, while ATCC 14579 produces both Nhe and Hbl. The results show that strains NVH 391/98 and INRA AF2 produce NheB.

The PlcR transcriptional regulator cannot account for varying levels of toxin expression

The PlcR/PapR quorum sensing system is presently the only established regulator of extracellular virulence factors in B. cereus group strains [7, 8]. Transcription of cytK from strain NVH 391/98 has previously been shown to be PlcR-dependent, even though the cytK promoter in this strain contains a PlcR recognition sequence with one base divergence from the currently defined PlcR recognition sequence [12]. However, as the cytK promoter regions of strains NVH 391/98 and NVH 883/00 are 100% identical, differences in the promoter regions cannot account for the differential expression of CytK in these two strains. Also, a perfect PlcR recognition sequence was found upstream of nheA in both strains NVH 391/98 and NVH 883/00.

To explore whether differences in the PlcR/PapR system itself could be responsible for the observed differential expression of CytK and Nhe, plcR and papR were sequenced in strains NVH 391/98, NVH 883/00, and INRA AF2. The deduced amino acid sequences of both PlcR and PapR were 100% identical in the three strains. Furthermore, the expression of PlcR was determined to be of comparable level in all three investigated strains using Western immunoblotting (results not shown).

YvrGH and YvfTU two-component systems are not responsible for the varying toxin levels

Regulation of virulence gene expression by two-component systems has been described in a wide range of pathogenic bacteria [14]. A partial sequence encoding a protein with homology towards the YvrG histidine kinase in ATCC 14579 was previously identified to be located upstream of cytK in NVH 391/98 [4], while in ATCC 14579, genes BC_5352 and BC_5353 encoding a putative two-component system (yvfTU) are located upstream from plcR [15]. As two-component systems sometimes control the expression of genes located in the same locus, we explored whether these two-component systems could have a regulatory function explaining the observed differential expression of toxins. yvrGH and yvfTU were DNA sequenced in both strains NVH 391/98 and NVH 883/00.

The deduced amino acid sequences of YvrH and YvrG each differed with only one amino acid between strains NVH 391/98 and NVH 883/00. A knockout mutant was obtained in B. cereus ATCC 14579. Unfortunately, the mutant could not be prepared in NVH 391/98, as all attempts to transform this strain failed despite various conditions used [12]. However, no difference between the B. cereus ATCC 14579 wild-type and the yvrGH null mutant could be observed in Western immunoblots where culture supernatants were probed using CytK antiserum, in the Vero cell cytotoxicity assay, or in transcriptional assays of cytK expression using lacZ fusions (results not shown).

Unpublished results (by J. Brillard) indicate that a knockout mutant of the yvfTU two-component system in B. cereus ATCC 14579 showed reduced expression of CytK using lacZ fusions, compared with the wild-type strain. However, the yvfTU locus located immediately upstream from plcR was 100% identical in strains NVH 391/98 and NVH 883/00. Reverse transcription (RT) PCR experiments were carried out to assess whether or not YvfTU was expressed in the low toxin-producing strain NVH 883/00. The results in Figure 3 show that yvfTU was expressed in all strains. Thus, neither the YvrGH nor the YvfTU two-component systems seemed to be responsible for the divergent expression of toxins in the presently investigated B. cereus strains.

Figure 3
figure 3

Detection of yvfTU expression by RT-PCR. Reverse transcriptase (RT) PCR experiments performed on the yvfTU operon of B. cereus strains ATCC 14579, INRA AF2, NVH 391/98, and NVH 883/00. The operon encodes the YvfTU two-component system. Lanes 1: RT-PCR on 500 ng RNA. Lanes 2: Negative control (RT-PCR on 500 ng RNA with a heat-inactivated reverse-transcriptase). Lanes 3: Positive control (PCR on 200 ng genomic DNA). The ~700 bp PCR product covered the 3'-region of yvfT running into the 5'region of yvfU, indicating that these two genes were expressed in a single operon.

The three investigated strains are genetically remote from other strains of the B. cereus group

During the course of this study, 13 genes were DNA sequenced in strains NVH 391/98 and NVH 883/00. It became apparent that while all examined genes were of high identity (> 99%) in NVH 391/98 and NVH 883/00, their identity towards other B. cereus strains from which DNA sequences are publicly available was typically around 70–80%. Using PCR experiments, INRA AF2 was confirmed to contain the same gene variants as NVH 391/98 and NVH 883/00. A total of 47 PCR reactions were performed, covering all 13 investigated genes, using a combination of 62 primers specific to strains NVH 391/98 and NVH 883/00 (see Additional file 1). To further study the genetic relatedness of these three strains towards other strains of the B. cereus group, multilocus sequence typing (MLST) was performed, using partial sequences of the seven housekeeping genes adk, ccpA, glpF, glpT, panC, pta, and pycA. The MLST scheme used is from the University of Oslo's Bacillus cereus group MultiLocus Sequence Typing website [16], which is adapted from three previously published schemes [10, 17, 18]. The obtained sequences from strains NVH 391/98 and INRA AF2 were 100% identical, while the only difference between the sequences of these two strains and NVH 883/00 were one nucleotide change in each of panC and pta. Figure 4 shows the phylogenetic tree prepared from the sequences obtained from the three examined strains and the corresponding sequences from other B. cereus group strains. The results clearly show that strains NVH 391/98, NVH 883/00, and INRA AF2 comprise a genetically remote cluster of strains within the B. cereus group.

Figure 4
figure 4

Phylogenetic analysis. Neighbour-joining phylogenetic tree prepared from the concatenated housekeeping gene sequences of different strains of the B. cereus group. The tree was based on the MLST scheme described at the University of Oslo's Bacillus cereus group MultiLocus Sequence Typing website [16]. Bootstrap support values (in %) are shown next to the appropriate nodes. Abbreviations: Bc: B. cereus, Bt: B. thuringiensis, Bw: B. weihenstephanensis.

Discussion

In the present study, we have investigated aspects of cytotoxicity, toxin production and regulation in a genetically remote and rare collection of strains within the B. cereus group. The original strain of this type, B. cereus NVH 391/98, was highly pathogenic and the strain in which CytK was first discovered [4], while the closely related B. cereus NVH 883/00 and INRA AF2 are the only two other identified strains of this group.

We have identified a novel variant of the genes encoding Nhe in all three investigated strains. Nhe was previously undetected in NVH 391/98 [4, 9], most likely due to the high sequence divergence of the novel Nhe-variant as compared with previously identified Nhe proteins. This would result in lack of detection by PCR and by assays employing monoclonal antibodies lacking cross-reactivity towards epitopes on the novel Nhe variant. This is supported by the discovery by Dietrich et al. [19] that when monoclonal antibodies were raised against NheB purified from B. cereus B-4ac, 20 out of 25 of the obtained antibodies showed reactivity towards an exoprotein from NVH 391/98 of the same size as NheB.

While strains NVH 391/98 and INRA AF2 were shown to be highly cytotoxic towards Vero cells and expressed high levels of the toxins CytK and NheB, strain NVH 883/00 was shown to be non-toxic under all conditions tested, with low or absent toxin expression. To date, these are the only three strains that have been identified to carry the cytK-1 variant [13]. The presence of CytK-1 was implicated as the primary reason for the high pathogenicity of NVH 391/98, due to the greater cytotoxic activity of CytK-1 compared with the CytK-2 variant [11], and a particularly high level of cytK-1 expression [12]. Although these factors certainly still seem valid, the identification of the non-toxic NVH 883/00 carrying cytK-1 indicates that the presence of this gene variant is not a sufficient criterion for identification of highly cytotoxic strains.

It has been proposed that gene content plays a small role in the diversity of phenotype and pathogenicity observed between B. cereus group strains, and that subtle changes to regulatory networks are of much greater importance [20]. Selected regulatory genes were investigated and compared, to potentially identify mechanisms responsible for the differential expression of toxins in NVH 391/98 and NVH 883/00. The PlcR/PapR quorum sensing system is presently the only established regulator of expression of extracellular virulence factors in B. cereus group strains [7, 8]. However, as the deduced PlcR and PapR proteins were 100% identical between strains NVH 391/98 and NVH 883/00, and the expression of PlcR was determined to be of comparable level, we propose that additional regulatory factors are involved.

Two-component systems have often been shown to play key roles in regulation of virulence in bacteria [14, 21]. In the current study, the possibility that two selected two-component systems, YvrGH and YvfTU, had a regulatory function related to toxin production was explored. Both were initially chosen for investigation based on their proximity to cytK-1 and plcR, respectively, as genes under the control of a two-component system often map in the vicinity of the regulatory genes [22]. However, neither the YvrGH nor the YvfTU two-component systems seemed to be responsible for the divergent expression of toxins in the presently investigated B. cereus strains, even though YvfTU has been implicated in positive regulation of CytK expression in B. cereus ATCC 14579 (J. Brillard, unpublished results).

Phylogenetic analysis (MLST) of strains NVH 391/98, NVH 883/00, and INRA AF2 compared to other B. cereus group strains showed that these three strains comprise a genetically remote cluster of strains within the B. cereus group. Thus, the presence of the novel nhe operon and the cytK-1 gene variant in these strains are intrinsic to the distant phylogenetic relationship towards other strains of the B. cereus group. Previous phylogenetic studies by Sorokin et al. [10] places strain NVH 391/98 rather far from main B. cereus group strain clusters. Based on these data, one could propose that the presently studied B. cereus strains should comprise a novel species. The assignment of a new species has probably been hampered by the fact that prior to the current report, only one single strain of this cluster (NVH 391/98) has been described, and perhaps that these strains do not seem to be distinguishable from other B. cereus strains based on traditional criteria such as morphology and phenotype.

Conclusion

We have discovered a novel Nhe variant in a rare group of B. cereus strains, which has previously been undetected in culture supernatants using PCR and methods based on monoclonal antibodies, due to its divergent sequence as compared with previously identified Nhe proteins. Despite cytK-1 expression having been shown to be exceptionally high in strain NVH 391/98 [12], the presence of a cytK-1 gene alone does not imply that the organism has high pathogenic potential, since strain NVH 883/00 carries cytK-1 but is non-cytotoxic. However, the presence of the novel nhe operon and the cytK-1 gene variant in strains NVH 391/98, NVH 883/00 and INRA AF2 seems to be a characteristic that is linked to their distant genetic relationship towards other B. cereus group strains. Furthermore, we found no evidence that the PlcR/PapR system or the YvrGH and YvfTU two-component systems are responsible for the differing levels of Nhe and CytK toxin expression between these strains. We therefore postulate that there must be additional unidentified regulatory mechanisms that are of significant importance for regulation of toxin expression in B. cereus.

Methods

Strains and growth conditions

B. cereus NVH 391/98 is a clinical isolate [4]. B. cereus NVH 883/00 is an isolate from spices and B. cereus NVH 0075/95 is a food-poisoning strain, both submitted to the Norwegian School of Veterinary Science, Oslo, Norway. B. cereus INRA AF2 is an isolate connected to a food poisoning case, submitted to the Institut National de la Recherche Agronomique, Avignon, France. B. cereus ATCC 14579 was used for construction of the yvrGH knockout mutant. XL10-Gold E. coli (Stratagene) was used for recombinant expression of CytK-1. B. cereus was grown in BHIG (brain heart infusion supplemented with 1 % w/v glucose) at 32°C or 37°C and 200 rpm, from overnight cultures diluted 1:100. Supernatants were collected by centrifugation. Supernatant from cultures grown at 25°C was concentrated 100 times by precipitation with 70% saturated (NH4)2SO4. Anaerobic growth was performed as follows: 5 ml of BHIG was boiled in glass tubes to remove oxygen, cooled, and inoculated with 50 μl of an overnight culture. The tubes were incubated at 32°C under anaerobic conditions, and samples of supernatants were obtained after 6, 24 and 48 hours.

Cytotoxicity assays

Cytotoxicity was determined using a Vero cell test [23]. The assay monitors the inhibition of protein synthesis in the cells by measuring the reduction of incorporated 14C-leucine in the Vero cells upon addition of toxin proteins. 100 μl samples of late log phase culture supernatants were applied to the assay in duplicate. The B. cereus Enterotoxin Reverse Passive Latex Agglutination test kit (Oxoid, Bassingstoke, England) and the Bacillus Diarrheal Enterotoxin visual immunoassay (Tecra Diagnostics, Roseville, Australia) were used according to the manufacturers' instructions.

PCR and DNA sequencing of toxin and regulatory genes

Genomic DNA from B. cereus used as template in PCRs was isolated using the method of Pospiech and Neumann [24]. PCR products subjected to DNA sequencing were obtained either by conventional PCR, inverse PCR, or using the DNA Walking SpeedUp premix kit (Seegene). DNA sequencing was performed on both strands and sequences were submitted to GenBank, with the following accessions for the NVH 883/00 sequences: [GenBank:DQ885233] for the locus containing yvrG, yvrH, the orf2 upstream of cytK-1 and cytK-1, [GenBank:DQ885234] for the locus containing the gene encoding an ABC transporter permease protein, yvfT, yvfU, plcR, and papR, and [GenBank:DQ885235] for nheA, nheB, nheC, and the downstream gene encoding a deoxyribonucleotide regulator. The corresponding DNA sequences obtained from strain NVH 391/98 in this study were identical to the corresponding sequences of the NVH 391/98 shotgun genome sequence [GenBank:AALL00000000], except in the case of the nhe operon, in which the complete sequence was obtained in the current report [GenBank:DQ885236]. The plcR and papR genes from strain INRA AF2 has the following accession: [GenBank:EF108376].

Sequence and phylogenetic analysis

The positions of coding sequences were predicted using EasyGene [25]. The following genomic sequences were used as reference strains: B. cereus ATCC 14579 [GenBank:AE016877], B. cereus ATCC 10987 [GenBank:AE017194], B. cereus G9241 [GenBank:AAEK01000000], B. cereus E33L [GenBank:CP000001], B. thuringiensis serovar konkukian str. 97–27 [GenBank:AE017355], B. thuringiensis serovar israelensis ATCC 35646 [GenBank:AAJM01000000], and B. weihenstephanensis KBAB4 [GenBank:AAOY00000000]. Pairwise alignments were calculated using the Smith-Waterman algorithm [26].

MLST was performed using partial sequences of the genes adk, ccpA, glpF, glpT, panC, pta, and pycA, ranging in length from 330 to 444 nucleotides, according to the scheme given at the University of Oslo's Bacillus cereus group MultiLocus Sequence Typing website [16]. PCR and DNA sequencing was performed as described, with the exception that primer aagtaagggctaagaaga was used as the forward primer for amplification of glpT, and primers ccaagggatataaagcgagatg and aatcaactataccgtttgtatttgc was used for panC. The GenBank accessions for the sequences from NVH 883/00 are adk; [GenBank:EF108377], ccpA; [GenBank:EF108378], glpF; [GenBank:EF108379], glpT; [GenBank:EF108380], panC; [GenBank:EF108381], pta; [GenBank:EF108382], and pycA; [GenBank:EF108383]. The GenBank accessions for the sequences from INRA AF2 are adk; [GenBank:EF108384], ccpA; [GenBank:EF108385], glpF; [GenBank:EF108386], glpT; [GenBank:EF108387], panC; [GenBank:EF108388], pta; [GenBank:EF108389], and pycA; [GenBank:EF108390]. The sequences for strain NVH 391/98 were obtained from the NVH 391/98 shotgun genome sequence [GenBank:AALL00000000], except in case of the adk locus, for which the sequence was obtained in the current report [GenBank:EF108391]. The reference strains listed above were used for all loci, with the exception of glpF, which was absent from the available shotgun genome sequences of B. weihenstephaniensis KBAB4 and B. thuringiensis serovar israelensis ATCC 35646, and tuncated in B. cereus G9241. The DNA sequences of all seven genes were concatenated, giving a sequence 2700 nucleotides in length, and aligned using ClustalW. A phylogenetic tree was calculated using the neighbour-joining method, where genetic distances were estimated using the Kimura model and bootstrap confidence values were generated using 1000 permutations. The tree was printed using TreeView [27].

Preparation of CytK antiserum

Recombinant CytK-1 for use in antiserum production was expressed from the vector construct pMS20-cytK-1 previously described [11]. Cultures were grown in 2 litres of modified CGY medium [28] containing 0.4 % glucose and 50 μg ml-1 kanamycin, and incubated at 37°C for 5 hours. The harvested pellet was resuspended in 20 ml lysis buffer (50 mM NaH2PO4, 300 mM NaCl, pH 8.0, 1 mg ml-1 lysozyme). Incubated on ice 30 minutes, and lysed by sonication. 0.25 mg RNase A and 10 U DNase (Promega) was added, followed by incubation on ice for 20 minutes. Purification of CytK-1 protein from the supernatant was performed as previously described [4]. A N2W rabbit was immunized using four ~1 ml doses, administered in two-week intervals, with a final bleeding six days after the fourth immunization. Fresh protein samples were used for each immunization.

SDS-PAGE and Western immunoblotting

SDS-PAGE (12% acrylamide) and Western immunoblotting was carried out according to standard protocols [29]. For detection of enterotoxins by Western immunoblotting, 12 μl culture supernatant from late log phase cultures grown at 32°C was applied. CytK antiserum was used at a dilution of 1:500. For detection of PlcR, bacterial pellet from 100 μl culture was suspended in SDS-PAGE sample buffer and applied. The PlcR rabbit antiserum [30], diluted 1:2000, was kindly supplied by Dr. Stephen Leppla, Maryland, USA. The secondary antibody biotin-goat-anti-rabbit IgG (Bio-Rad) was used at a 1:1000 dilution. Monoclonal antibodies 1A8 against NheA [19], 2A3 against Hbl component B, and 1C2 against both NheB and Hbl component L1 [31], used at dilutions of 1:15, were obtained as a gift from Dr. Erwin Märtlbauer, University of Munich, Germany. For these blots, the secondary antibody biotin-goat-anti-mouse IgG (Amersham Biosciences) was used at a 1:500 dilution. All blots were incubated with a complex of streptavidin and biotinylated alkaline phosphatase used at a dilution of 1:3000, prior to development with a NBT/BCIP solution.

Construction of the yvrGH mutant

The yvrGH operon was interrupted by allelic exchange with a kanamycin resistance gene (KmR) in B. cereus ATCC 14579 as follows: The regions upstream of yvrH and downstream of yvrG were PCR amplified using tgcaggatcc gttagcaaatcgccactact/tgcagtcgac atacgtagttcggattctcg and tgcactgcag agaatggattaccggtctaac/tgcaccatgg agggaagcaggttagtattgt, respectively. PCR products were digested with Bam HI/Sal I and Pst I/Nco I using primer-incorporated restriction sites (underlined). KmR was PCR-amplified from pDG783 [32] using primers tctggtcgac catttgaggtgatagg and gctactgcag atcgatacaaattcctcgtaggcg, and digested with Sal I/Pst I. The three digested DNA fragments were purified, and ligated into Nco I/Bam HI digested pMAD [33]. The recombinant plasmid pMADΔyvrGH was transformed into B. cereus ATCC 14579, transformants were subjected to allelic exchange as previously described [33], and the yvrGH mutant was confirmed by DNA sequencing.

cytK transcriptional activity

The cytK-promoter of B. cereus ATCC 14579 has previously been cloned in pHT304-18'Z, giving a cytK'-lacZ transcriptional fusion [12]. The plasmid was transformed into B. cereus ATCC 14579 wild-type and ΔyvrGH, and cells were grown in LB medium at 37°C with shaking. β-galactosidase specific activities were measured in triplicate samples from each culture as described previously [34]. Experiments were repeated twice.

RT-PCR of yvfTU

RNA extraction was performed using the FastRNA ProBlue kit (Qbiogen) on strains grown at 37°C in LB medium and harvested in stationary phase (OD600 = 1.4). RT-PCR experiments were performed with the Titan One Tube RT-PCR System (Roche), using 500 ng RNA in each reaction. The primers used were either ttgtGaaAaatccagagcgtgc (for ATCC 14579) or ttgtAaaGaatccagagcgtgc (for the three clinical strains), and atccaatccactttgaatcggc. Diverging nucleotides in the forward primer sequences are indicated in uppercase.