Department of Microbiology, UCC, National University of Ireland-Cork, Cork, Ireland
Correspondence
E. Fidelma Boyd
f.boyd{at}ucc.ie
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ABSTRACT |
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INTRODUCTION |
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VPI-2 is a 57·3 kb chromosomal region encoding ORFs VC1758 to VC1809 which has all the characteristics of a pathogenicity island (Jermyn & Boyd, 2002). All toxigenic V. cholerae O1 and O139 serogroup isolates contained VPI-2, whereas non-O1/nonO139 non-toxigenic isolates lacked the region. VPI-2 encodes several gene clusters: a type-1 restriction modification system, which may protect the bacteria from viral infection (Bickle & Kruger, 1993
); a nannag gene cluster homologous to genes involved in sialic acid metabolism, which may act as a carbon and nitrogen source (Vimr et al., 2004
); neuraminidase, which acts on higher-order gangliosides in the intestine converting them to GM1 gangliosides, with the subsequent release of sialic acids (Galen et al., 1992
); and a region with homology to Mu phage. Among most V. cholerae O139 serogroup isolates, only a 20 kb region of VPI-2 was present, as ORFs VC1761 to VC1788 had been deleted, indicating the instability of the region (Jermyn & Boyd, 2002
).
The species V. mimicus is closely related to V. cholerae; however, V. mimicus is phenotypically and genotypically distinct from V. cholerae and can be readily differentiated from V. cholerae (Boyd et al., 2000a; Byun et al., 1999
; Davis et al., 1981
; O'Shea et al., 2004a
; Reen & Boyd, 2004
). V. mimicus, unlike V. cholerae, is negative in sucrose, VogesProskauer, corn oil and Jordan tartrate reactions (Davis et al., 1981
). Comparative sequence analysis of the housekeeping gene malate dehydrogenase (mdh) from V. mimicus isolates showed the mean pairwise divergence between V. cholerae and V. mimicus was approximately 10 %, which is equivalent to the divergence between Salmonella enterica LT2 and E. coli K-12 (Boyd et al., 1994
, 2000a
; Byun et al., 1999
; O'Shea et al., 2004a
). In addition, analysis of groE-I and groEL-II on chromosomes 1 and 2, respectively, of V. cholerae and V. mimicus also demonstrated the divergence of both species from one another (Reen & Boyd, 2004
). The natural habitat of V. mimicus, similar to V. cholerae, is the aquatic ecosystem, where it has been found both as a free-living bacterium and in association with phytoplankton and crustaceans (Acuna et al., 1999
; Campos et al., 1996
). Consumption of V. mimicus-contaminated shellfish has been linked to the development of gastroenteritis (Acuna et al., 1999
). The virulence determinants of V. mimicus have not been well characterized. Recently, it was demonstrated that some V. mimicus isolates also harbour VPI-1 (TCP) and CTX
(CT) (Boyd et al., 2000b
). Several V. mimicus strains isolated from clinical and environmental sources were shown to produce multiple toxins, including a haemolysin, zonula occludens toxin, a heat-stable enterotoxin, as well as a CT-like toxin (Campos et al., 1996
; Chowdhury et al., 1994
; Ramamurthy et al., 1994
; Shi et al., 1998
; Spira & Fedorka-Cray, 1983
, 1984
).
In this paper, we examined 17 V. mimicus clinical and environmental isolates of various serogroups for the presence of the 57·3 kb VPI-2 region. ORFs VC1773 to VC1787 were found to be present in all 17 V. mimicus stains examined. In addition, 11 V. mimicus isolates contained ORFs VC1758 (integrase) and VC1804 to VC1809. We reconstructed the phylogenetic relationship of the nanH (VC1784) gene among a range of V. cholerae and V. mimicus isolates and compared it to the species tree, as deduced from the housekeeping gene mdh. On the mdh gene tree, V. mimicus isolates formed a separate divergent lineage from V. cholerae. On the nanH gene tree, however, V. mimicus isolates clustered with V. cholerae non-O1/non-O139 isolates, indicating that the nanH gene from these species is closely related. Analysis of additional genes spanning VPI-2 among a subset of V. cholerae and V. mimicus were in agreement with the nanH data, suggesting that VPI-2 was horizontally transferred between these species.
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METHODS |
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Molecular analysis.
To assay for the presence of VPI-2 among V. mimicus isolates, 17 primer pairs that span the entire 57·3 kb VPI-2 region and two primer pairs that flank the island were used for PCR analysis (Jermyn & Boyd, 2002). PCR was performed in volumes of 20 µl containing 100 ng genomic DNA, 200 µM primer, 1·25 mM dNTPs, 50 mM MgCl2, and 1U Taq DNA polymerase (Bioline). The amplification conditions were pre-incubation at 96 °C for 60 s, followed by 30 cycles of 94 °C for 30 s, 4855 °C (depending on the primer pair) for 30 s and 72 °C for a time chosen based on the size of the expected fragment (60 s kb1). All PCRs were carried out in a PTC-200 Peltier Thermal Cycler (MJ Research). PCR products were resolved by electrophoresis on a 0·8 % agarose gel made with 1x TAE (consisting of 40 mM Tris/acetate and 1 mM EDTA) and containing ethidium bromide. PCR amplification products were visualized by UV transillumination.
Southern hybridization was carried out with DNA probes generated from PCR products from the reference V. cholerae strain N16961 as a template (Heidelberg et al., 2000). PCR products were purified using the ConceRT-PCR purification kit (Gibco, BRL). For Southern hybridization analysis, DNA from each strain was digested with the restriction enzyme EcoRI (Roche Molecular Biochemicals), and the fragments were separated by electrophoresis in 0·6 % TAE agarose. The gel was depurinated with 0·25 M HCl, denatured with a solution of 5 M NaCl and 10 N NaOH, and neutralized with 1 M Tris and 20x SSC. The fragments were transferred to nitrocellulose membranes by a posiblotter (Stratagene). DNA was fixed to the membrane by UV cross-linking. Approximately 100 ng probe DNA was conjugated to horseradish peroxidase using the ECL direct nucleic acid labelling system (Amersham Pharmacia Biotech), and after hybridization overnight, was detected by the ECL chemiluminescent substrate. Hybridization membranes were washed according to manufacturer's instructions.
Pulsed-field gel electrophoresis.
To determine whether the ORF VC1758 encoding an integrase was located in the proximity of VC1773VC1787, we carried out pulsed-field gel electrophoresis (PFGE). Genomic DNA was prepared from the V. mimicus strains PT5 and 523-80 as follows. The bacteria were grown in LB broth overnight at 37 °C. The cells were centrifuged and resuspended in SE buffer (consisting of 75 mM NaCl and 25mM EDTA) to an OD620 of 1·0. An equal volume of the cell suspension and 2 % agarose was mixed and cast in a mould. The individual agarose inserts were treated with PEN buffer (0·5 M EDTA, 1 %, w/v, N-lauroylsarcosine, 1 mg Pronase ml1) and washed with TE buffer (100 mM Tris/Cl, 10 mM EDTA). After processing, the inserts were incubated for at least 6 h with SfiI at 50 °C. Electrophoresis was performed with a CHEF-DR II electrophoresis system (Bio-Rad) in 1x TBE buffer (45 mM Tris, 45 mM boric acid, 1 mM EDTA) at 13 °C. Pulse ramps were 3 to 80 s for 21 h at 160 V in 1·0 % agarose. After electrophoresis, the gel was stained with ethidium bromide, washed and treated for Southern hybridization analysis.
DNA sequencing.
The primer pairs used for PCR amplification and subsequent sequencing are listed in Table 2. The nucleotide sequence of an internal fragment of six genes spanning the VPI-2 region was obtained: VC1764, encoding a methyl accepting subunit; nanE (VC1781), encoding N-acetylmannosamine-6-phosphate 2-epimerase; nagC (VC1783), encoding N-acetylglucosamine-6-phosphate deacetylase; nanH (VC1784), encoding neuraminidase; VC1799, encoding an integrase; and VC1806, encoding a replicase. For the nanH gene, fragments were amplified from the chromosomal DNA of 22 V. cholerae strains and three V. mimicus strains, whereas for the remaining five genes, five V. cholerae strains were examined, which included a classical strain O395, an O139 serogroup strain MO2, and three non-O1/non-O139 strains V46, V47 and V52, and a V. mimicus strain PT5. PCR was performed in a 20 µl reaction mixture using conditions as described earlier. PCR amplicons were purified using the ConceRT-PCR purification kit (Gibco-BRL) in accordance with manufacturer's instructions. Following purification, an aliquot of 10 µl was used as a sequencing template. All sequencing was carried out by MWG-Biotech.
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RESULTS |
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Genomic mapping of the VPI-2 in V. mimicus
To determine whether the 19·4 kb VPI-2 in V. mimicus was inserted in the same insertion site as that in V. cholerae, we carried out PCR analysis using primers designed from the insertion site of the VPI-2 in V. cholerae. Using the primer pair tRNAF (located within the serine tRNA) and int4 (located within ORF VC1758), a PCR product of 1·3 kb was identified in 11 isolates containing the 19·4 kb VPI-2 region. Nucleotide sequencing of the 1·3 kb product from V. mimicus strain PT5 showed that VPI-2 was located adjacent to a serine tRNA. Sequencing revealed that there was an intergenic region of 313 bp between the serine tRNA and VC1758, the first ORF of VPI-2 in V. mimicus.
PFGE was used to determine if VC1758 was located in close proximity to the ORFs VC1773VC1787, since PCR analysis failed to amplify any product using a primer pair designed between these regions. Using the probes nint3/nint4 (encompassing VC1758) and 148F/146B (encompassing VC1773VC1776), an identical hybridization fragment of approximately 200 kb was obtained from V. mimicus strain PT5. Similarly for V. mimicus strain 523-80, an identical hybridization fragment of approximately 120 kb was obtained from each probe. This indicated that the ORFs VC1758 and VC1773VC1776 were located in proximity to each other, on the same hybridization fragment, on the V. mimicus chromosome.
Genetic variation at the nanH locus
To determine the evolutionary history of the VPI-2 region among V. cholerae and V. mimicus, we sequenced a 611 bp (nucleotides 177788) fragment of the nanH gene from 22 V. cholerae strains and three V. mimicus isolates. Sequencing revealed variation at 49 nucleotide sites among the 22 V. cholerae nanH sequences examined, 41 of which were synonymous substitutions (silent sites) and eight of which were non-synonymous substitutions (amino acid replacement sites) (Table 3, Fig. 4
). No nucleotide differences were found between the epidemic V. cholerae O1 and O139 isolates examined. Of the 49 polymorphic sites identified, there were 14 singleton sites found among V. cholerae non-O1/non-O139 serogroup isolates. For example, V. cholerae O141 serogroup strain V46 contained seven singleton sites, O54 serogroup strain SG14 contained three singleton sites and O37 serogroup strain 151 contained two singleton sites. The maximum nanH sequence difference between V. cholerae strains was 5·23 % between strains 151 and V46.
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Of the 203 NanH amino acid sites examined, nine polymorphic amino acid sites were found among the V. cholerae and V. mimicus strains (Fig. 4). Eight amino acid polymorphisms were found among V. cholerae isolates and three among V. mimicus isolates, with one amino acid polymorphic site unique to V. mimicus. Six of the nine amino acid replacement polymorphisms were conservative and involved substitution of amino acids with similar properties. The remaining three amino acid polymorphisms all involved substitution of a hydrophobic residue with a hydrophilic one.
Sequence analysis of the 22 V. cholerae mdh sequences revealed variation at 24 nucleotide sites, of which 23 were synonymous substitutions and one was a non-synonymous substitution (Table 3). All three V. mimicus strains exhibited identical mdh sequences to one another, and contained 58 unique polymorphic sites compared to V. cholerae mdh sequences, two of which resulted in amino acid changes (Table 3
). The mean pairwise percentage difference among the V. cholerae and V. mimicus mdh sequences was 3·73 % and the maximum difference was 12·03 %.
The variability observed at the nanH locus was greater than that observed at the mdh locus for the same set of isolates. To determine whether the selective constraints at these loci are different, that is, whether nanH is under positive selection or not, we examined the synonymous (kS) and non-synonymous (kN) substitution rates and calculated the kN/kS ratio for each gene (Table 3). Amino acid replacements in a protein that incur an advantage to the cell are fixed at a higher rate than silent site substitutions resulting in a kN/kS ratio greater than 1. Amino acid replacements in a protein that are deleterious to the cell are fixed at a lower rate by purifying selection, with a kN/kS ratio less than 1. Substitutions in a protein that are neither selectively advantageous nor deleterious are neutral, with a kN/kS ratio equal to 1. The nanH gene kN/kS ratio was not high, indicating that this gene is not under positive selection (Table 3
).
Evolutionary genetic relationships of VPI-2 among V. cholerae and V. mimicus
To reconstruct the evolutionary history of the VPI-2 region from V. cholerae and V. mimicus, a phylogenetic tree based on the nanH gene was constructed. The nanH sequences from 25 isolates were analysed using the JukesCantor distance method and a neighbour-joining gene tree was constructed based on synonymous polymorphic sites only (Fig. 5). From Fig. 5
it can be seen that all V. cholerae O1 and O139 serogroup strains clustered together on the nanH gene tree. This cluster also included two V. cholerae non-O1/non-O139 serogroup strains: V52, a toxigenic O37 serogroup strain; and V45, a rough isolate, which gave an identical nanH sequence to the O1 and O139 serogroup isolates. The other V. cholerae non-O1/non-O139 serogroup strains were grouped into two divergent clusters on the nanH gene tree. The first cluster contained V. cholerae strains V46, V47, V51 and SG14. The second cluster contained the strains V54, 9581, 9582, 151 and E714 in addition to V. mimicus strains PT5, PT48 and 9583.
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To further determine the evolutionary history of the entire VPI-2 region among V. cholerae and V. mimicus isolates, we sequenced gene fragments from five additional ORFs, VC1764, VC1781, VC1783, VC1799 and VC1806, which spanned VPI-2. Nucleotide analysis of the five ORFs, for six V. cholerae strains, N16961, O395, MO2, V46, V47 and V52, provided similar findings to the nanH (VC1784) gene sequence analysis (Table 4). Strains N16961, O395, MO2 and V52 exhibited identical nucleotide sequences for the five ORFs VC1764, VC1781, VC1783, VC1799 and VC1806. Four ORFs, VC1781, VC1783, VC1799 and VC1806, of strains V46 and V47 exhibited different nucleotide sequences when compared to the consensus sequence in strain N16961. In contrast, the nucleotide sequence of the ORF VC1764 was identical between V46, V47 and N16961. Comparison of the nucleotide sequence of three ORFs, VC1781, VC1783 and VC1806, between V. mimicus strain PT5 and V. cholerae strain N16961 revealed similar findings to the nanH (VC1784) nucleotide comparison.
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DISCUSSION |
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The deletion of the type 1 restriction modification gene cluster and the nannag gene cluster from the V. cholerae O139 serogroup isolates may be the reason why this serogroup is no longer a dominant cause of epidemic cholera on the Indian subcontinent. The retention of VPI-2 in toxigenic V. cholerae O1 serogroup isolates suggests that this region may provide a competitive advantage in vivo, whereas the presence of the nannag region in all V. mimicus isolates examined suggests that it may be an essential region for survival in the environment. Interestingly, the nannag gene cluster is also present in the genomes of Vibrio vulnificus strains CMCP6 and YJ016 as well as Vibrio fischeri strain ES114, but is absent from the genome of Vibrio parahaemolyticus strain RIMD2210633 (W. S. Jermyn, unpublished data). Among Vibrio species sequenced to date, only V. cholerae and V. mimicus have been shown to encode neuraminidase (nanH), which cleaves sialic acid from sialoglycoconjugates (Corfield, 1990). V. vulnificus, V. parahaemolyticus and V. fischeri, however, encode N-acetylneuraminic acid synthase, which can synthesize sialic acid de novo, whereas V. cholerae and V. mimicus must acquire sialic acid from an external source.
There were 49 polymorphic substitutions among the nanH sequences examined in V. cholerae, which was approximately twice as many polymorphic sites compared to mdh in the same set of strains (Table 3). This could indicate that nanH is under some selective pressure for change or that there is relax pressure at this locus. Analysis of the nanH sequence demonstrated that most of the polymorphic sites were silent site substitutions that do not result in amino acid changes, and the kN/kS ratio at this locus was much lower than 1, indicating that mutations in this gene are probably deleterious to the host (Table 3
). In fact, there was a limited number of replacement polymorphisms at this locus, indicating functional constraints on this protein. Analysis of the sequenced nanH fragment revealed that a number of key features and motifs, which are essential for enzyme function, were conserved. For example, in the active site of NanH, two arginines that stabilize the carboxylic acid group of sialic acid were conserved. Also the FRIP region, which is involved in substrate affinity, was conserved. This indicated that the enzyme function was maintained between Vibrio isolates.
In order to elucidate the evolutionary history of VPI-2 among V. cholerae and V. mimicus, comparative sequence analysis of the nanH gene tree with the species tree, deduced from the housekeeping gene mdh, was carried out. In a number of studies, the mdh locus has been shown to be an excellent indicator of the overall genetic diversity of a species, since it is not under selective pressure and is present in all isolates of a species (Boyd et al., 1994, 1996
; Byun et al., 1999
; O'Shea et al., 2004a
; Reen & Boyd, 2004
). Clustering of V. cholerae isolates on the nanH gene tree was similar to the clustering of isolates on the mdh gene tree; however, the congruence between the trees did not extend to nanH from V. mimicus. On the nanH gene tree, V. mimicus did not form a separate divergent branch from V. cholerae as it does on the mdh tree, but instead clustered with V. cholerae non-O1/non-O139 isolates (Fig. 5
). We examined five additional loci on the VPI-2 among six V. cholerae isolates and one V. mimicus isolate (Table 4
). These five loci, which span the nannag gene cluster and regions in the 5' and 3' of VPI-2, overall gave a similar pattern of divergence and clustering as nanH. This indicates that nanH, and by extension the nannag genes, were horizontally transferred between V. mimicus and V. cholerae. We favour an evolutionary scenario in which VPI-2 was present in the most recent common ancestor of V. mimicus and horizontally transferred to V. cholerae soon after these species diverged. Horizontal transfer between V. cholerae and V. mimicus has previously been documented (Boyd et al., 2000b
; Faruque et al., 1999
). The presence of both CTX
and VPI in V. mimicus natural isolates has been demonstrated (Boyd et al., 2000b
). Nucleotide sequence identity of genes from both CTX
and VPI derived from V. mimicus and V. cholerae has been reported, which strongly suggests that contemporary horizontal transfer of DNA between these species has occurred (Boyd et al., 2000b
). Both V. cholerae and V. mimicus occupy similar environmental niches and it is possible that V. mimicus acts as an environmental reservoir of novel DNA for V. cholerae. Horizontal gene transfer between Vibrio species appears to be an emerging theme in the evolution of this genus, since transfer of a 8·5 kb region encoded on the Vibrio seventh pandemic island-II (VSP-II) between V. cholerae and V. vulnificus has also recently been described (O'Shea et al., 2004b
).
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ACKNOWLEDGEMENTS |
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Received 13 September 2004;
revised 30 September 2004;
accepted 30 September 2004.
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