Molecular Infectious Diseases Group, University of Oxford, Department of Paediatrics, Weatherall Institute of Molecular Medicine, John Radcliffe Hospital, Oxford OX3 9DS, UK
Correspondence
Patricia Martin
patricia.martin{at}paediatrics.ox.ac.uk
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ABSTRACT |
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INTRODUCTION |
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The frequency of phase variation is a major factor controlling the genetic diversity and consequently the fitness of bacterial populations. Therefore, the study of cis- and trans-acting factors regulating the instability of simple sequence repeats is essential to understand the relevance of simple sequence tracts in the biology of the bacterium. The sequence and the length of a repeat tract are major cis-acting factors known to regulate repeat instability in human (Rolfsmeier et al., 2001), yeast (Tran et al., 1997
; Wierdl et al., 1997
) and bacterial organisms (de Bolle et al., 2000
). In N. meningitidis, a linear relationship between the length of the hmbR polyguanine (polyG) tract and phase variation frequency was reported in serogroup A strains (Richardson et al., 2002
).
Replication and post-replicative repair systems are also involved in the control of the plasticity of repeat tracts. In yeast, DNA polymerase proofreading and methyl-directed mismatch repair (MMR) correct frameshifts preferentially in short and long homonucleotide runs, respectively (Tran et al., 1997). In Escherichia coli, the overexpression of dinB, which encodes the error-prone DNA polymerase IV, results in an increased frequency of frameshifts in short homopolymeric tracts (Kim et al., 1997
). In Haemophilus influenzae, inactivation of mutS, a key component of MMR, and polI destabilize dinucleotide and tetranucleotide repeat tracts, respectively (Bayliss et al., 2002
). In N. meningitidis, investigation of two contingency loci revealed that the mismatch repair genes mutS and mutL have a role in controlling phase variation frequencies (Richardson & Stojiljkovic, 2001
; Richardson et al., 2002
).
Finally, the involvement of Dam (DNA adenine methylase) methylation in the regulation of phase variation is unclear. Dam methylation was shown to have no effect upon phase variation of tetranucleotides in H. influenzae (Bayliss et al., 2002) and of polyG tracts in N. meningitidis (Richardson & Stojiljkovic, 2001
). In contrast, Bucci et al. (1999)
proposed that the absence of Dam activity was responsible for the high frequency of N. meningitidis capsule phase variation and for the heightened virulence of some strains.
The effect of trans-acting factors on phase variation rates cannot be assumed to be similar for different genes. Indeed, in H. influenzae, mutations in mutS were not found to alter switching rates of dinucleotide repeats of the pilus locus but did alter switching rates of a similar dinucleotide repeat tract in another location in the chromosome (Bayliss et al., 2004). Therefore, the aim of the present study was to investigate the role of genes likely to influence phase variation in N. meningitidis in the regulation of switching frequencies for different types of repeat tracts. The mutS and dinB but not the dam or drg genes influenced the frequency of phase variation of genes associated with homopolymeric tracts. Contrary to this observation, the stability of tetranucleotide repeat tracts did not depend on the genetic factors investigated in the study.
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METHODS |
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Recombinant DNA techniques and nucleotide sequence analysis.
Restriction endonucleases were obtained from Roche or New England Biolabs and used according to the manufacturers' instructions.
PCR amplification was performed using Taq polymerase from Gibco-BRL. Reactions consisted of 30 cycles including 1 min of denaturation at 94 °C, 1 min of annealing at the appropriate temperature and 1 min of extension at 72 °C. The primers used in the study were purchased from Genosys and are listed in Table 2. Pairs of primers siaDF/siaDR, lacZB1/sprhind, porA1/porA2, lgtGC/lgtGD and nadAF/nadAR were used to PCR amplify DNA fragments containing the repeat tract associated with genes siaD, spr, porA, lgtG and nadA, respectively. The DNA sequences of both strands of these amplicons were obtained in a sequencing reaction with fluorescent dye-labelled dideoxynucleotide terminators using Ampli Taq DNA Polymerase FS (Perkin Elmer), according to the instructions supplied by Applied Biosystems. Primers used in sequencing reactions were siaDF and siaDR for siaD, sprF2, sprF3 and lacZB1 for spr, porA1 and porA2 for porA, and nadAF and nadAR for nadA (Table 2
). Clear sequence of the repeat tract could not be obtained from lgtG PCR products, an inherent trait of long homopolymeric tracts. lgtG PCR products were cloned into pT7 Blue vector (Novagen) and sequenced using primers lgtGC, lgtGD and the plasmid-specific primers M13 For and M13 Rev. The sequences were analysed on an automatic sequencer (model 377, Applied Biosystems). Nucleotide sequence data were analysed using the GCG program (Wisconsin package, version 10.2-Unix, Genetics Corporation Group).
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Construction of MC58 strain harbouring the dinB gene under the control of the opa promoter.
Plasmid pCR2-Popa-dinB was derived from pCR2-Popa-gfp, which presents a gfp gene under the control of the N. meningitidis opa promoter (unpublished data). The gfp gene was excised as a NdeINsiI fragment from pCR2-Popa-gfp and replaced by the 5' portion of the N. meningitidis strain MC58 dinB gene amplified by PCR with primers Din-NdeI and Din2-Nsi (Table 2), which respectively contain a NdeI and a NsiI restriction site. The NdeI site of the primer Din-NdeI contains the translational start codon of the gene. A 610 bp DNA fragment resulting from the PCR amplification of the 5' region of the dinB gene of strain MC58 with primers Din-down and Din-down-Bam (Table 2
) was ligated with the 1·25 kb kanamycin resistance cassette, obtained by digestion of pUC4K vector (Pharmacia), in pT7 Blue vector (Novagen). The 1·86 kb fragment was released by digesting the resulting plasmid with EcoRI and SpeI and cloned upstream of the opa promoter in the plasmid digested with the same enzymes. This construct was transformed into strain MC58. By PCR amplification using primers Din-down2/Din2-Nsi and Din2-Nsi/Kan 5' (Table 2
), the transformant MC58PopadinB was shown to present a copy of the wild-type dinB gene and a copy of the gene under the control of the opa promoter. Although additional secondary DNA rearrangements also occurred, the resulting construct allowed the overexpression of the dinB gene.
Construction of mutS, dinB, dam, drg and galE knock-out mutants.
The plasmid pT7-mutS contains a 670 bp DNA fragment amplified by PCR from the 5' region of the mutS gene of strain MC58 with primers MutS-up-Kpn and MutS-up-Bam (Table 2), then the 1·25 kb kanamycin resistance cassette followed by a 500 bp DNA fragment PCR amplified from the 3' region of the mutS gene with primers MutS-down-Bam and MutS-down (Table 2
). This plasmid was linearized with ScaI and transformed into strain MC58. The transformant MC58mutS presented a 800 bp deletion of the mutS gene and an insertion of the kanamycin resistance cassette, confirmed by PCR using primers MutS-up2/MutS-down2, MutS-up-Kpn/Kan 5' and MutS-down/Kan 3' (Table 2
).
The plasmid pT7-dinB contains a 610 bp DNA fragment amplified by PCR from the 5' region of the dinB gene of strain MC58 with primers Din-down/Din-down-Bam, then the 1·25 kb kanamycin resistance cassette followed by a 630 bp DNA fragment PCR amplified from the 3' region of the dinB gene with primers Din-up-Kpn and Din-up-Bam. This plasmid was linearized by ScaI and transformed into strain MC58. The transformant MC58dinB presented a 800 bp deletion of the dinB gene and an insertion of the kanamycin resistance cassette, confirmed by PCR using primers Din-down2/Din-up2, Din-down/Kan 5' and Din-up-Kpn/Kan 3'.
Plasmid pADK1 contains a 540 bp internal fragment of the N. meningitidis strain BZ10 dam gene, which was amplified by PCR with primers DamF1/DamB2 (Table 2, Fig. 1
), then interrupted by the insertion of a kanamycin resistance cassette. This plasmid was linearized and transformed into the dam+ strains AK22, 94/155 and NGH38. The disruption of the dam gene in strains AK22dam1, AK22dam2, 94/155dam1 and NGH38dam1 was confirmed by PCR using primers DamF1/DamB2 (Table 2
, Fig. 1
). This was corroborated by Southern hybridization using the kanamycin resistance gene as a hybridization probe.
The plasmid pT7-drg contains a 640 bp DNA fragment amplified by PCR from the 5' region of the drg gene (or dpnC gene) of strain MC58 with primers Drg-up-Bam/Drg-up, then the 1·25 kb kanamycin resistance cassette followed by a 660 bp DNA fragment PCR amplified from the 3' region of the drg gene with primers Drg-down-Bam and Drg-down-Kpn. This plasmid was linearized by ScaI and transformed into strain MC58. The transformant MC58drg presented a 650 bp deletion of the drg gene and an insertion of the kanamycin resistance cassette, confirmed by PCR using primers Drg-down and Drg-up2.
galE knock-out mutants of strains MC58, MC58mutS, MC58dinB, MC58PopadinB, AK22, AK22dam1 and AK22dam2 were constructed using plasmid containing the galE gene disrupted by the erythromycin cassette (unpublished data). The erythromycin cassette was originally from the Bacillus subtilis plasmid pIM13 (Monod et al., 1986).
In each case, no polar effect was expected as a consequence of the disruption of each of the genes.
Detection of siaD, porA, lgtG and nadA phase variation by colony immunoblots.
Bacteria were grown overnight on solid media, transferred to a nitrocellulose filter (45 µm, pore size, Schleicher and Schuell) and allowed to air-dry. Non-specific binding sites were blocked for 1 h with 5 % (w/v) milk/0·1 % (w/v) azide/PBS-T [phosphate buffered salineTween 20, 0·05 % (v/v)]. Filters were washed three times with PBS-T, then incubated for 2 h 30 min with an appropriate dilution of antibody in PBS-T-bovine serum albumin [BSA, 2 % (w/v)]. Monoclonal antibodies (mAb) 735 (Frosch et al., 1985), P1.7 and B5 were used to detect siaD, porA and lgtG phase variation, respectively, and the antiserum containing antibodies raised against NadA (Pizza et al., 2000
) was used to detect the switching of nadA expression. The dilutions of antibodies used were 1/10 000, 1/500, 1/3500 and 1/10 000, respectively. Filters were then washed three times in PBS-T. Primary antibody was detected with anti-mouse IgG-Alkaline Phosphatase antibody (Sigma and Cedarlane Laboratories) by incubation for 1 h in PBS-T-BSA. Filters were washed three times in PBS-T and antibody was detected with 5-bromo-4-chloro-3-indolyl phosphatenitro blue tetrazolium (Perkin Elmer Life Sciences). The colour reaction was stopped after 30 min by several washes with water and the blots were air-dried.
Construction of translational fusion between the lacZ gene and the spr gene in N. meningitidis and detection of spr phase variation.
Chromosomal DNA of strain H44/76spr/lacZ, which contains a promoterless lacZ gene inserted in-frame downstream of the spr gene (Martin et al., 2003), was used to transform strains MC58, MC58mutS, MC58PopadinB, AK22, AK22dam1, AK22dam2 and MC58drg. The same chromosomal DNA was used to transform all the strains. Any additional mutations potentially introduced beside the desired one are most likely present in all the strains transformed. Moreover, there remains a very small possibility of co-transformation events. Transformants were streaked on BHI plates containing X-Gal (80 µg ml1). Blue transformants expressing
-galactosidase were analysed by PCR amplification and DNA sequencing to confirm the presence of the fusion.
To detect phase variation of the spr gene, the strains were grown overnight on BHI plates. Single colonies were then picked, plated on X-Gal-containing BHI plates and grown overnight. The coexistence of LacZ+ and LacZ variants, i.e. of blue colonies expressing -galactosidase and white colonies not expressing the enzyme, reflected the switching of the gene.
Determination of phase variation frequencies.
The frequencies of phase variation given are frequencies of mutants and were determined by dividing variant c.f.u. ml1 by the total viable c.f.u. ml1, all c.f.u. deriving from the same colony, as defined by Richardson & Stojiljkovic (2001). Our method to estimate mutation frequencies follows the same procedure (median frequency) as Richardson & Stojiljkovic (2001)
, thus allowing some valid comparison with their results. The relative fitness of the ON and OFF variants in the wild-type and mutant strains is assumed to be identical, since there is no reason to assume that the ON and OFF variants of the wild-type strain when compared to those of the mutant strains have different relative fitnesses when they are being investigated under similar in vitro conditions.
Determination of frequencies of spontaneous mutants resistant to rifampicin.
Frequencies of spontaneous mutants resistant to rifampicin were measured by two different methods. Cells from an overnight culture on plate were harvested in 1 ml PBS; 1010 cells were plated on BHI agar containing 30 µg rifampicin ml1. Alternatively, 1000 colonies deriving from a single dispersed colony were grown overnight and harvested in 1 ml PBS; 1010 bacteria were plated from this suspension on BHI agar containing 3 µg rifampicin ml1. Frequencies were determined by dividing resistant c.f.u. ml1 by the total viable c.f.u. ml1. Both methods gave similar results for a given strain.
RT-PCR.
Following 12 h growth, total RNA was prepared using the SV total RNA isolation system (Promega) from N. meningitidis strains MC58 and MC58PopadinB, the strain presenting the dinB gene under the control of the opa promoter. Five hundred and fifty nanograms of total RNA was reverse transcribed to produce cDNA using Moloney murine leukaemia virus (MMLV) reverse transcriptase (RT) and random primers (Promega). Co-amplification of the dinB transcript with an internal control allowed comparison of the levels of dinB gene expression between the RNA samples. PCR amplification of the dinB cDNA was performed with oligonucleotides Din-up2 and Din-NdeI. Primers specific for the constitutively expressed housekeeping gene gdh (glucose-6-phosphate dehydrogenase), gdh-P1 and gdh-P2 (Table 2), were also included in each PCR amplification to provide an internal control. To control for chromosomal DNA contamination, RNA was directly used for PCR amplification. The relative intensities of the dinB-specific and gdh-specific products were measured by densitometry (ImageQuant, Amersham Biosciences) for three independent experiments.
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RESULTS |
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An 11-fold increase of the frequency of spontaneous acquisition of rifampicin resistance was observed in the MC58mutS background (3·0x108) compared to wild-type (2·7x109) (Table 3).
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To estimate the frequency of siaD phase variation (on to off switching), 105 colonies of the wild-type strain MC58 were plated. However, we could not detect any non-reactive colonies using mAb 735. This finding was in agreement with the low frequency of capsule switching already reported in N. meningitidis (Hammerschmidt et al., 1996). It was therefore not possible to determine the frequency of capsule phase variation in the wild-type strain MC58 (Table 3
). In contrast, in MC58mutS, on to off switching was observed. Amplification by PCR and sequencing of the siaD polyC tract in 22 capsule-negative variants revealed that five displayed eight cytosine residues, three exhibited six residues and 14 had seven residues in the repeat tract. mAb 735 reactive colonies are typically associated with seven cytosines. Interestingly, capsule-negative variants presenting a frameshift in the polyC tract as well as variants displaying seven cytosine residues in the repeat tract were obtained in distinct experiments. Although the quoted frequencies may be underestimated due to the possibility of overlooking non-reactive colonies, in strain MC58mutS, capsule-negative variants resulting from a frameshift in the repeat tract located in siaD arose at a frequency of 3·7x104 (Table 3
) and capsule-negative mutants resulting from a different mutational event were obtained at a similar frequency (2·5x104).
We measured the frequency of off to on spr phase variation by enumerating blue colonies expressing (on) and white colonies not expressing (off) -galactosidase. The frequency was increased at least 700-fold in the MC58mutS background (8·3x103) when compared to the wild-type frequency (1·2x105) (Table 3
).
To detect lgtG phase variation, we used mAb B5. Part of the epitope recognized by mAb B5 comprises the phosphoethanolamine (PEA) at the 3 position of heptose II in the LPS. In the on state, lgtG encodes a glucosyltransferase which adds a glucose to the 3 position of heptose II, precluding the addition of PEA (Mackinnon et al., 2002). This LPS structure therefore impedes the recognition and the binding of mAb B5 (Plested et al., 1999
). In the lgtG off state, glucose is not added; therefore PEA can be added and consequently mAb B5 can recognize the relevant epitope. Thus, a mAb B5-positive phenotype implies the existence of an off state and a mAb B5-negative phenotype an on state of lgtG gene expression. We showed that strains MC58 and MC58mutS both presented 12 cytosine residues in the repeat tract located in lgtG. This number of bases makes the ORF out of frame, preventing the synthesis of a mature protein. The frequency of lgtG phase variation measured was therefore the off to on frequency. lgtG phase variation was increased by about 120-fold in the MC58mutS background (2·0x103) as compared to the wild-type (2·6x105) (Table 3
).
Preliminary data obtained from a single experiment revealed an increase in the frequency of frameshifts in the porA gene in the MC58mutS background (3·8x104) compared to the wild-type frequency (3·3x105). Sequencing of the repeat tract associated with porA in 13 colonies that reacted with mAb P1.7 and in five colonies that did not react with mAb P1.7 revealed that the polyG tract contained 11 and 10 guanine residues, respectively.
The tetranucleotide (TAAA) repeat tract associated with nadA is located in the promoter region of the gene. In strain MC58, nine repeated motifs constitute the repeat tract, a number of repeats associated with a low level of nadA transcription and a weak reactivity with the specific polyclonal antibody (Martin et al., 2003). Loss or gain of one tetranucleotide repeat, leading to eight or ten reiterated motifs, was shown to result in increased expression of nadA, as evidenced by strong antibody reactivity. No differences in switching between strong and weak antibody reactivities were detected between strains MC58 (4·4x104) and MC58mutS (3·0x104) (Table 3
).
In conclusion, we showed that mutS was involved in the control of the instability of homopolymeric tracts (C7 in siaD, C10 in spr, G11 in porA and C12 in lgtG) but not of tetranucleotide repeat tracts [(TAAA)9 in nadA].
dinB influences the stability of the siaD homopolymeric tract
To investigate the involvement of dinB in the regulation of phase variation, we constructed a dinB knock-out mutant of strain MC58 (MC58dinB) and a MC58 mutant strain in which the dinB gene was placed under the control of the opa promoter (MC58PopadinB). Using RT-PCR we found that, under the growth conditions used, expression of dinB was increased by approximately 70 %, relative to strain MC58 (Fig. 2). Disruption or overexpression of dinB did not modify the global mutation frequency, as detected by spontaneous resistance to rifampicin, compared to the frequency determined in the wild-type background (1·8x109 and 2·9x109 vs 2·7x109, respectively) (Table 3
).
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We detected capsule-negative variants in strain MC58PopadinB. The siaD repeat tract was sequenced in seven capsule-negative colonies. Two variants displayed eight cytosines and five had six cytosines in the repeat tract. Thus, the siaD on to off phase variation frequency was augmented in the strain MC58PopadinB (1·4x104), when compared with the wild-type frequency (<1·0x105) (Table 3). Interestingly, overexpression of dinB did not affect the frequency of switching of the spr gene when compared to the wild-type (2·0x105 vs 1·2x105, respectively). Likewise, we showed that the frequency of lgtG phase variation was unchanged (Table 3
). Preliminary data also suggested that the porA switching frequency was not affected by the overexpression of the dinB gene (3·3x105 vs 1·4x105). Finally, overexpression of dinB did not alter the frequency of nadA phase variation when compared to wild-type (3·7x104 vs 4·4x104, respectively) (Table 3
).
Conservation of two distinct dam loci in Dam+ and Dam N. meningitidis strains
To investigate the consequences of dam inactivation on the bacterial phenotype, we constructed mutants in which the dam gene was disrupted. Contrary to what Richardson & Stojiljkovic (2001) reported, Bucci et al. (1999)
reported that the pathogenic strains they investigated presented a Dam phenotype. Therefore, we investigated the presence or absence of the dam gene in a global collection of 84 disease isolates representative of the genetic diversity of N. meningitidis. Phylogenetic profiles of these geographically and genetically distinct N. meningitidis strains were previously characterized (Maiden et al., 1998
). The chromosomal DNA of each of the 84 strains was extracted and digested with the restriction enzymes DpnI, DpnII and Sau3AI. Fig. 3(a)
shows an example of patterns obtained for a subset of N. meningitidis strains. DpnI recognizes and cuts its cognate targets only when GATC sites are methylated, DpnII cuts only unmethylated sites, and Sau3AI cuts both methylated and unmethylated target sequences. Since Dam directs the methylation of the deoxyadenosine site at the GATC sequence, hence rendering DNA resistant to cleavage by DpnII, but not by DpnI or Sau3AI, the functional integrity of the dam gene can be ascertained via a combination of these three enzymes.
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The genetic basis of the dam gene inactivation was investigated in the Dam strains. This revealed that all the Dam strains were the result of an ancestral inactivation event. We surveyed the presence of drg (dam replacing gene) in the Dam strains (Bucci et al., 1999). All the Dam strains yielded a PCR product of 705 bp with primers DrgF1 and DrgB2 (Fig. 1
), whereas all the Dam+ strains did not (data not shown). Southern analyses using the 705 bp PCR amplicon as a probe confirmed that only Dam strains possessed the drg gene (data not shown). The chromosomal location of drg was determined by analysing the immediate up- and down-stream sequences which flanked the drg gene. Each pair of primers (Drg5F/DrgB3 and Drg3F/DamB5, Fig. 1
) generated a PCR product of similar size from all the Dam strains (data not shown), indicating that drg gene insertion indeed occurred at the dam locus, at the same place. This suggests that the acquisition of drg most likely occurred once during the evolution of the bacterium and indicates that the two types of dam loci have been conserved in the dam+/drg and dam/drg+ strains, respectively.
dam and drg do not influence the stability of homopolymeric and tetranucleotide repeat tracts
We constructed dam knock-out mutants in strains AK22, 94/155 and NGH38, arbitrarily chosen to represent the dam+/drg genotype. The inactivation of the Dam function in these mutant strains was subsequently verified by using the restriction enzymes DpnI, DpnII and Sau3A1. All the DNAs were susceptible to complete digestion by DpnII and Sau3A1, but resistant to DpnI (Fig. 3b), demonstrating the absence of Dam function in the strains.
We determined the spontaneous mutation frequency in the above three pairs of isogenic strains, nine natural dam+ strains and 12 natural dam strains randomly selected from the same meningococcal strain collection. In general, no marked difference was detected between dam+ and dam strains, regardless of the mechanism by which the Dam activity had been abolished (Table 4).
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We constructed a drg knock-out mutant in MC58, a strain representative of the dam/drg+ genotype. The spontaneous mutation frequency determined for the MC58drg mutant (0·9x109) was not significantly different from the frequency determined for the wild-type strain (2·7x109, Table 3). The frequency of phase variation was determined for the siaD, spr and nadA genes in the MC58drg background. This revealed that disruption of the drg gene did not affect the frequency of frameshifts occurring in homopolymeric and tetranucleotide repeat tracts (Table 3
). This therefore complements and extends the findings reported by Bucci et al. (1999)
.
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DISCUSSION |
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According to the classification established by Richardson & Stojiljkovic (2001), strain MC58 has a low overall mutation rate, as defined by spontaneous acquisition of rifampicin resistance. We have shown that the mutS mutant of N. meningitidis strain MC58 presented a spontaneous mutation frequency 11-fold higher than the wild-type rate. Thus, we confirm the weak mutator phenotype resulting from the inactivation of the mutS gene previously reported in N. meningitidis (Richardson & Stojiljkovic, 2001
). Likewise, in H. influenzae, mutS, mutL and mutH mutants exhibit a significant three- to fourfold higher global mutation frequency than wild-type strain Rd (Bayliss et al., 2002
). In addition, inactivation of dam did not result in a global mutator phenotype in N. meningitidis, in agreement with previous findings in this organism (Richardson & Stojiljkovic, 2001
) and in H. influenzae strain Rd (Bayliss et al., 2002
). Strain MC58 does not appear to have the mutH gene (Tettelin et al., 2000
), suggesting that mismatch repair in N. meningitidis may be different from the system characterized in E. coli.
We showed that disruption of mutS in N. meningitidis increased the frequency of frameshifts occurring in homonucleotide tracts of various lengths (C7 in siaD, C10 in spr, G11 in porA and C12 in lgtG). This extends the conclusions drawn previously from the analysis of two contingency loci associated with polyG tracts of similar length, 9 and 10 bases (Richardson & Stojiljkovic, 2001). The effect of mutS on phase variation rates could not be assumed a priori to be similar for different genes (Bayliss et al., 2004
). As most of the phase variable genes in N. meningitidis are associated with polyC or polyG tracts (Saunders et al., 2000
), bacterial cells contain many genes that appear to be hypermutable targets in mismatch-repair-deficient strains. Consistently, strains exhibiting a general mutator phenotype resulting from defects in mismatch-repair pathways were found amongst clinical isolates of N. meningitidis (Richardson & Stojiljkovic, 2001
; Richardson et al., 2002
). Pathogenic bacteria can face strong selective pressures when colonizing a new host or a new environment within the same host. Thus, mutator strains of N. meningitidis could be advantageous, at least in the short term, because of their adaptive capacities, resulting from an enhanced variability of their surface-exposed structures.
The present study has identified for the first time a role for dinB in the regulation of phase variation in a bacterial pathogen. DinB is the recently discovered DNA polymerase IV which belongs to the SOS regulon (Kim et al., 1997). Investigations are currently under way to elucidate its role in the bacterial cell (Wagner et al., 2002
; Tompkins et al., 2003
). It has been shown that N. gonorrhoeae does not possess an SOS-like system that is induced in response to DNA damage (Black et al., 1998
). Moreover, the lexA gene is missing in the N. meningitidis strain MC58 genome sequence (Tettelin et al., 2000
). One can therefore speculate that in N. meningitidis, dinB is not under the control of a DNA damage-inducible system. Consequently, the context in which the DNA polymerase IV is recruited could be different in E. coli and in N. meningitidis. In our study we showed that, contrary to what was observed in E. coli (Kim et al., 1997
), overexpression of dinB in N. meningitidis did not result in a global mutator phenotype. Although this absence of a mutator phenotype could be due to a quantitative difference of DinB molecules in both organisms, the amount of molecules of DNA polymerase IV in N. meningitidis was sufficient to increase the frequency of frameshifts in the siaD homopolymeric tract. We also showed that the frequencies of frameshifts in the other homonucleotide tracts we investigated were not affected by dinB overexpression. In yeast, the impact of proofreading in preventing frameshift mutations was shown to decrease when the length of a homonucleotide run increases (Tran et al., 1997
). In addition, in E. coli, the proofreading activity of DNA polymerase III recognizes frameshifts close to the 3' end of the nascent DNA strand (Strauss et al., 1997
). Bulged nucleotides resulting from replication slippage within a long run of simple repeats could locate at a distance from the 3' end of the growing DNA strand and thus escape from DNA proofreading. Thus, to explain the lack of effect of overexpression of dinB on the frequency of frameshifts in long homopolymeric tracts, we hypothesize that in N. meningitidis neither DNA polymerase III nor DNA polymerase IV mediates efficient proofreading on long repeat tracts. Construction of mutants containing increasing tract lengths incorporated into the siaD gene, and investigation of the influence of dinB overexpression on the instability of these various repeat tracts, would be required to test this hypothesis.
In this study we have shown that the instability of tetranucleotide repeats did not depend on genetic factors such as mutS, dinB, dam and drg. Similarly, in H. influenzae, where phase variation is almost exclusively mediated by tetranucleotide repeat tracts (Hood et al., 1996), mutation of polI but not of genes involved in MMR or other pathways of DNA repair or recombination was shown to increase phase variation rates mediated by tetranucleotide repeat tracts (Bayliss et al., 2002
). Thus, in N. meningitidis as in H. influenzae, tetranucleotide repeat tracts seem to be refractory to most of the mismatch correction systems.
We also demonstrated that 27 % of N. meningitidis strains possessed a dam gene and an active Dam function, 70 % of which belonged to either the A4 cluster or ET-37 lineage, which are classical hypervirulent lineages. Dam is associated with less than a third of virulent strains, findings not consistent with previous data suggesting an absence of Dam activity in pathogenic isolates (Bucci et al., 1999). The selection of strains from Italy and France investigated in this latter study is unlikely to be representative of the global meningococcal population. Bucci and colleagues also showed that dam-deficiency in N. meningitidis created a mutator phenotype, resulting in an increased frequency of phase variation in the siaD gene (Bucci et al., 1999
). However, we and others (Richardson & Stojiljkovic, 2001
) could not reproduce this finding, showing a lack of correlation between Dam methylation and the frequency of phase variation. In contrast, a multifactorial role of Dam methylation was involved in Salmonella virulence (Garcia-Del Portillo et al., 1999
). Mutants of Salmonella typhimurium lacking dam were shown to be attenuated for virulence and to present a distinct pattern of secreted proteins compared to dam+ strains (Garcia-Del Portillo et al., 1999
). The strict correlation between the presence of drg and the absence of dam evidenced in our study confirmed that the presence of dam and drg was mutually exclusive (Bucci et al., 1999
). We showed that the drg gene was located at an identical locus in all dam/drg+ strains. This suggests that the common ancestor of the N. meningitidis strains investigated was likely to be a dam-proficient strain. The drg gene shares significant homology with the Streptococcus pneumoniae type II restriction endonuclease gene dpnI (Cantalupo et al., 2001
), suggesting that drg has been horizontally acquired. Investigation of the involvement of drg in the regulation of the phase variation frequencies suggested that it did not have a role in the control of repeat tract stability. The function of the drg gene, which must be important for the bacteria since it has been widely conserved, remains to be elucidated.
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ACKNOWLEDGEMENTS |
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REFERENCES |
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Received 22 March 2004;
revised 8 June 2004;
accepted 8 June 2004.