Effect of phage infection on toxin production by Clostridium difficile

doi:10.1099/jmm.0.45821-0

HOME

HELP

FEEDBACK

SUBSCRIPTIONS

Effect of phage infection on toxin production by Clostridium difficile

Shan Goh¹, Barbara J Chang¹ and Thomas V Riley^1,2

Microbiology, School of Biomedical & Chemical Sciences, The University of Western Australia, Queen Elizabeth II Medical Centre¹, and Division of Microbiology and Infectious Diseases, The Western Australian Centre for Pathology and Medical Research², Nedlands, Australia 6009

Correspondence Thomas V. Riley triley{at}cyllene.uwa.edu.au

Received July 13, 2004
Accepted September 9, 2004

Infection with Clostridium difficile and subsequent productionof toxins A and B may result in C. difficile-associated diarrhoeaand pseudomembranous colitis in hospital patients. The effectof four temperate phages, obtained by induction of clinicalC. difficile isolates, on toxin production by C. difficile wasdetermined. None of these phages converted a lysogenized non-toxigenicC. difficile strain to toxin production. One of the accessorytoxin genes, tcdE, was detected in three phages, ${phi}$ C2, ${phi}$ C6 and ${phi}$ C8; however, the non-repeating regions of tcdA and tcdB encodingthe enzymic domains were not carried on phage DNA. Phage infectionof toxigenic strains increased toxin B production in four ofsix lysogens, although the level of tcdB transcription as determinedby real-time RT-PCR was not significantly altered. However,levels of toxin A transcription in two lysogens were significantlyaltered without any corresponding differences in toxin A production.

This paper was presented at the First International Clostridiumdifficile Symposium, Kranjska Gora, Slovenia, 5–7 May2004.

${dagger}$ Present address: Department of Microbiology, Faculty of Medicine,National University of Singapore, MD4 #05-08, 5 Science Drive2, Singapore 117597.

Abbreviation: PaLoc, pathogenicity locus.

INTRODUCTION

TOP
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
REFERENCES

Clostridium difficile is a spore-forming anaerobe and the causativeagent of pseudomembranous colitis and many cases of antibiotic-associateddiarrhoea in hospital patients (Bartlett et al., 1978). ToxinsA and B are major virulence factors causing enterotoxicity andcytotoxicity, respectively, to cells (Lyerly et al., 1985).The secretory mechanism of both toxins is unknown; the toxinslack signal peptides, suggesting that an alternative to thetype II pathway of the general secretory pathway is present(Mukherjee et al., 2002). A toxin-associated gene, tcdE, whichlies in the pathogenicity locus (PaLoc) between tcdA and tcdB,was shown to possess a phage holin-like function when expressedin Escherichia coli. As phage holins are involved in cell membranedisruption (Wang et al., 2003), TcdE was speculated to playa role in toxin release through formation of membrane lesions(Tan et al., 2001). We wished to investigate whether the presenceof prophage would enhance toxin production in C. difficile.To date, production of C. difficile toxins has not been shownto be regulated or encoded by temperate phages, although thePaLoc possesses characteristics of a mobile genetic element(Braun et al., 1996; Hammond & Johnson, 1995).

Previous studies of the potential effects of phages on C. difficiletoxin production are limited to the description of two phagesthat did not convert non-toxigenic strains to toxin production(Mahony et al., 1985). In our study, four temperate phages thatwere induced from three clinical C. difficile isolates weretested for toxin conversion without success, although tcdE wasdetected in phage DNA. Toxin levels of phage-infected strains(stable lysogens) were also examined, followed by an investigationof tcdA and tcdB transcription in lysogens.

METHODS

TOP
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
REFERENCES

Bacteria and bacteriophages.

Fifty-six C. difficile isolates were isolated from stool samplesof diarrhoeal patients at Sir Charles Gairdner Hospital (SCGH),Western Australia, as previously described (Riley et al., 1994).Overnight broth cultures were induced with 3 µg mitomycinC ml^–1 for phage, as previously described (Nagy & Foldes, 1991).Three of the 56 isolates harboured temperatephages as determined by plaque assay: ${phi}$ C2 from CD242, ${phi}$ C5 fromCD578, and ${phi}$ C6 and ${phi}$ C8 from CD371 (Table 1). Isolates that produceda high number of plaques for each phage were determined throughphage assay (see below) and used as propagating strains. AllC. difficile isolates used in this study are shown in Table 1.Phages were purified as described by Sambrook et al. (1989)and determined to be Myoviridae ( ${phi}$ C2, ${phi}$ C5 and ${phi}$ C8) and Siphoviridae( ${phi}$ C6) phages (unpublished data).

View this table:
[in this window]
[in a new window]

Table 1. C. difficile isolates used for phage induction, propagation and infection, and in toxin assays

Culture media, bacterial growth and bacteriophage propagation.

C. difficile isolates were cultured in brain heart infusionbroth (BHIB; Oxoid) for overnight or 2.5–3 h (exponentialphase) at 37 °C in 80 % N₂, 10 % CO₂ and 10 % H₂ (Don WhitleyD3161). Cultures for toxin assays were incubated for 48 h. Anaerobebasal agar (ABA; Oxoid), either as base (1 % ABA) or overlay(0.74 % ABA, 0.01 M Ca²⁺ and 0.4 M Mg²⁺), was used for phageassays, culture of lysogens and viable counts. Phage was propagatedand assayed on solid media as described previously (Adams, 1959).Briefly, a phage suspension (500 µl of 10⁶–10⁷ p.f.u.ml^–1) was mixed with an indicator culture (4 ml of 10⁸c.f.u. ml^–1) and overlaid onto 1 % ABA for phage propagation,or 10 µl phage was spotted onto plates seeded with 600µl indicator for phage assay.

Isolation of stable lysogens of ${phi}$ C2, ${phi}$ C6 and ${phi}$ C8.

Five C. difficile isolates were infected with the four phages,producing six stable lysogens of ${phi}$ C2, ${phi}$ C6 and ${phi}$ C8 (Table 1). ${phi}$ C5did not lysogenize these isolates. Centres of turbid plaqueswere stabbed with a sterile wire and cultured on blood agar(BA) for 48 h. Single colonies arising from phage-resistantcells within the plaque, due either to mutation or to resistanceconferred by prophage, were induced with mitomycin C and assayedwith the uninfected strain to determine the presence of prophage.Stability of lysogens after –70 °C storage was testedby mitomycin C induction and colony blots using phage genomeprobes labelled with digoxigenin (Roche), as previously described(Karcher, 1995). Stable lysogens were named by the parentalisolate number followed by the phage type, e.g. lysogen CD382C2was host strain CD382 lysogenized by ${phi}$ C2.

DNA extraction from C. difficile and phages.

An overnight broth culture (10 ml) of C. difficile was concentratedin 1 ml TE buffer, treated with 2 µg lysozyme ml^–1at 37 °C for 30 min followed by 1 % (v/v) SDS, 40 mM EDTAand 500 µg proteinase K ml^–1 at 55 °C for 1–2h, and 100 µg RNase A ml^–1 at 37 °C for 30 min.DNA was extracted twice with equal volumes of phenol : chloroform: isoamyl alcohol (25 : 24 : 1) followed by chloroform, precipitatedwith 0.3 M sodium acetate (pH 5.2) and ethanol, and purified(Wizard Clean-up system by Promega). Extraction of phage DNAwas carried out as previously described (Sambrook et al., 1989).

Detection of toxin A and B levels in uninfected hosts and lysogens.

Broth cultures of C. difficile were standardized to obtain 1–9x10⁵c.f.u. ml^–1 and filtered (0.22 µm; Acrodisc). Crudetoxin in the filtrate was serially diluted twofold and toxinA and B were assayed by ELISA (Techlab) and cell culture, respectively.One toxin A unit was defined as the reciprocal of the ELISAend point dilution to logarithmic base 2. Toxin A assays wereperformed once only due to reagent costs. Toxin B was assayedby inoculating 20 µl crude toxin onto Vero cells witha seeding concentration of 50 000 cells per well (Mahony et al., 1989).Cells were observed after 48 h and the minimum cytotoxictitre (MCT), defined as the reciprocal of the dilution thatresulted in 50 % of cell death, was determined by neutral redassay (Mahony et al., 1989). MCTs were compared by mean andvariance of cytotoxic titre units, which was defined as thelogarithmic base 2 of the MCT (Freeman & Wilcox, 2003; Ketley et al., 1984).Assays were done in triplicate and repeated twice.

Detection of toxin genes in phage DNA by PCR.

Primers for amplification of tcdA (NK 2/3) and tcdB (NK 104/105)were described previously (Kato et al., 1991). A PCR reactionof 30 µl consisted of 1 µl template DNA, 0.18 µMof each primer, 200 µM dNTP, 2.5 mM MgCl₂, 1x reactionbuffer and 0.75 U Taq gold polymerase (Perkin Elmer). Cyclingconditions were 94 °C for 9 min, 35 cycles of 95 °Cfor 20 s and 55 °C for 120 s, then 74 °C for 5 min.Primers for tcdE (KST 1/2) were also described previously (Tan et al., 2001).The 20 µl PCR reaction consisted of 7 µltemplate DNA, 0.2 µM of each primer, 200 µM dNTP,2 mM MgCl₂, 1x reaction buffer and 0.75 U Taq gold polymerase(Perkin Elmer). Cycling conditions were 94 °C for 10 min,45 cycles of 94 °C for 30 s, 55 °C for 30 s and 72 °Cfor 1 min, and 72 °C for 7 min. Primer sequences are shownin Table 2. Chromosomal DNA from four toxigenic and non-toxigenicisolates served as control for amplification of toxin genes.

View this table:
[in this window]
[in a new window]

Table 2. Oligonucleotides used in this study

Detection of toxin genes by Southern hybridization.

Phage and bacterial DNA was digested by HindIII and/or XbaI(Promega), separated in 1 % agarose, transferred to a nylonmembrane (Amersham Pharmacia Biotech) (Sambrook et al., 1989)and fixed by heating in a microwave for 2.5 min (Angeletti et al., 1995).Southern hybridization was carried out with theDIG High Prime DNA Labelling and Detection Starter Kit I (Roche),according to the manufacturer's instructions. Purified (WizardClean-up system; Promega) undigested phage DNA was DIG-labelledfor use as probes (Roche). Probes for tcdA, tcdB and tcdE wereprepared from PCR-amplified products of C. difficile VPI 10463.Optimal hybridization temperatures were determined from dotblots using appropriate DNA controls. Southern hybridizationswere repeated three times.

Colony hybridization.

Lysogens grown on BA in a matrix were transferred onto a nylonmembrane and lysed as previously described (Karcher, 1995).DNA was fixed and hybridized to phage probes as described above.

Extraction of bacterial RNA and real-time RT-PCR.

RNA extraction from a 10 ml overnight culture of C. difficilewas carried out using reagents supplied in Totally RNA (Ambion)according to the manufacturer's instructions. Relative quantitativereal-time RT-PCR was performed using the ABI Prism 7000 SequenceDetection System (Applied Biosystems) on RNA extracted fromuninfected (parental) and infected (lysogenic) C. difficileisolates. ToxA-283/360 and ToxB-23/101 primers were designedto flank their TaqMan probes TOXA-315 and TOXB-48 (Table 2),respectively. TaqMan probes were labelled 5' with the reporterdye 6-carboxyfluorescein, and 3' with minor groove binder groupsfor increased sequence specificity (Kutyavin et al., 2000).The reaction volume was 20 µl, which consisted of 1x Superscriptreaction mix (Invitrogen), 2.8 mM MgCl₂, 10 mM DTT, 0.3 U SuperscriptIII RT/Platinum Taq Mix (Invitrogen), 10 U RNaseOUT (Invitrogen),0.3 µM of each primer, 0.2 µM TaqMan probe and 40ng template RNA. RT-PCR reactions were carried out at 50 °Cfor 30 min, 94 °C for 5 min, and for 45 cycles of 94 °Cfor 10 s, 55 °C for 10 s, and 68 °C for 30 s. A samplewas used as calibrator RNA, where serial dilutions resultingin 2.44, 9.77, 39 and 156.25 ng RNA per reaction were amplified.The C_T values were used in generating a standard curve for relativequantification of samples (ABI PRISM 7000 Sequence DetectionSystem User Guide). All reactions were carried out in triplicate.

RESULTS AND DISCUSSION

TOP
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
REFERENCES

Phage did not convert non-toxigenic strain to toxin production

C. difficile strain CD382 was toxin B negative by cell cultureand a common host to all four phages. CD382 was infected withphages for isolation of stable lysogens, which were tested fortoxin B production through cell culture. The presence of tcdAand tcdB in DNA was also determined through PCR. CD382C2, CD382C5,CD382C6 and CD382C8 did not have a cytotoxic effect on Verocells. DNA of three single colonies of each lysogen was extractedfor PCR amplification with NK 2/3 (tcdA) and NK 104/105 (tcdB)primers. All samples were negative for tcdA and tcdB.

Detection of toxin genes in phage DNA

tcdA and tcdB were not detected in phage DNA by PCR or Southernhybridization (not shown). Probes were chosen for the non-repeatingregion of tcdA and tcdB in the interest of detecting them separately.The non-repeating nucleotide regions in tcdA and tcdB encodethe enzymic domain (Barroso et al., 1994; Faust et al., 1998).Although the phages did not harbour these sections of the toxingenes, it is possible that sequences related to the repeatingunits were present. Nucleotide repeating sequences at the 3'-endof both genes (Barroso et al., 1994; Dove et al., 1990) encoderepeating units responsible for carbohydrate binding in TcdAand receptor binding and translocation in TcdB (Pfeifer et al., 2003).

Despite a lack of association between the toxin genes and phageDNA in the above experiments, there are two intriguing reportsof homology between tcdA and genomes of phages belonging toother species. The toxin A gene was reported to be homologousto an unknown gene in phage ${phi}$ CT2 of Clostridium tetani (Canchaya et al., 2002).Lactobacillus casei phage A2 ORF22 was hypothesizedto have a sie function (Proux et al., 2002). Homology betweenORF22 and toxin A has been reported although no details of itsextent were provided (Proux et al., 2002). Alignment of ORF22(GenBank accession no. NC_004112) to TcdA of VPI 10463 (GenBankaccession no. X9298) and variant strains (GenBank accessionnos AJ011301, AF279457, AF217291, AJ132669 and Y10689) did notshow significant similarity. However, alignment of ORF22 toTcdC of VPI 10463 showed 55 % identity over the last 103 aaof TcdC with an e-value of 2e–22, but no significant similarityto the truncated TcdC of the variant strain 8864 (GenBank accessionno. Y10689). Such homology between TcdA and TcdC to phage proteinssuggests phage origins of toxin genes. It is interesting tonote that ORF22 was absent in the variant strain with a truncatedTcdC. Homology of phage genes to tcdB has not been described;however, part of the ${phi}$ C2 genome, sequence 584 (GenBank accessionno. AY522336), had low homology to tcdB (unpublished data).Matching bases were distributed between nucleotide positions227 and 630 of tcdB, which is the enzymic domain or the non-repeatingsection of the gene, but outside of the region amplified bythe PCR primers. No significant similarities or alignments wereidentified between a putative ORF in sequence 584 and TcdB tosuggest any phage function in toxin B production. This may explainthe lack of hybridization between the tcdB probe and ${phi}$ C2 DNA.

The tcdE gene was detected in ${phi}$ C2, ${phi}$ C5 and weakly in ${phi}$ C8 by PCR(not shown). To verify these results, Southern hybridizationsof tcdA, tcdB and tcdE probes to phage genomes were performed.The tcdE probe hybridized to a band of expected size (5.1 kb)in VPI 10463, as well as to three other bands (18.6, 12.6 and7 kb) not predicted to lie within the PaLoc (Fig. 1). Thesecould be prophage sequences with homology to tcdE, as phagesequences have been shown to be present in VPI 10463 (unpublisheddata). The tcdE gene was detected in ${phi}$ C2, ${phi}$ C5 and weakly in ${phi}$ C8.Four bands were common to ${phi}$ C2 and ${phi}$ C5, while the two bands in ${phi}$ C8 were unique (Fig. 1). Interestingly, tcdE was present onlyin the Myoviridae phages ( ${phi}$ C2, ${phi}$ C5 and ${phi}$ C8) and may encode an essentialprotein such as holin. In this regard, ${phi}$ C6 of the Siphoviridaefamily may possess a different holin that is dissimilar to thetcdE product. ${phi}$ C2 and ${phi}$ C5 were closely related, and both weremoderately related to ${phi}$ C8 but not to ${phi}$ C6, as determined by phageimmunity assays and Southern hybridization (Goh et al., 2005).This level of relatedness was reflected in the patterns of hybridizationof tcdE to phage DNA. The presence of tcdE in ${phi}$ C2, ${phi}$ C5 and ${phi}$ C8is interesting because it supports the idea that phage may havesome role in toxin secretion through a holin-like pathway, assuggested in two studies (Mukherjee et al., 2002; Tan et al., 2001).Holins are small membrane proteins that disrupt the bacterialmembrane together with endolysins (Wang et al., 2000). To date,little is known about C. difficile toxin secretion, and althoughthe type II pathway of the general secretory pathway is presentin clostridia it is unlikely to be involved (Bruggemann et al., 2003;Mukherjee et al., 2002). Phage-infected toxigenic strainsof C. difficile may be able to release toxins through a fullyfunctional holin pathway resulting in cell lysis. Alternatively,the existing tcdE-associated holin pathway may be complementedin lysogens by phage holin genes and function at a higher efficiencyto cause membrane disruption compared to uninfected toxigenicstrains that rely only on the tcdE-associated holin pathway.It is also possible that the presence of a holin-like tcdE inthe PaLoc is a coincidence. Putative holin sequences have beenfound in bacterial chromosomes, probably as remnants of crypticphages (Wang et al., 2000).

View larger version (67K):
[in this window]
[in a new window]

Fig. 1. Detection of tcdE in phage DNA. (a) Separation of HindIII-digested C. difficile and phage DNA in 1 % agarose. Lanes: 1, ${lambda}$ /HindIII marker; 2, VPI 10463; 3, CD33; 4, ${phi}$ C2; 5, ${phi}$ C5; 6; ${phi}$ C6; 7, ${phi}$ C8. (b) Southern hybridization of (a) to DIG labelled tcdE probe carried out at 36 °C. There was strong hybridization of the tcdE probe to VPI 10463, ${phi}$ C2 and ${phi}$ C5, and weak signals from ${phi}$ C8.

Toxin A and B assays of lysogens and parents

Cytotoxicity assays were carried out on five toxigenic parentalisolates and six lysogens (Table 1). Since an absorbance standardfor quantification of toxin A was not provided with the ELISAkit (TechLab), the minimum end point titre was used as a measureof toxin A levels. A twofold increase in toxin A was measuredin CD1017C6, while the remaining lysogens were unaltered, suggestingphage had little effect on toxin A production (Fig. 2a). Significantincreases in toxin B were observed in all lysogens except forCD594C8 and CD727C6, which had unaltered levels (Fig. 2b). Thisapparent lack of coordination between toxin A and toxin B productionmay be due to methodology and should be confirmed by repeatingthe toxin A assays, and using an ELISA method for toxin B. Phagehad a positive effect on toxin B production in CD839C2, CD1017C6,CD1017C8 and CD6938C6 (Fig. 2b) despite the apparent absenceof tcdB in phage DNA. Hence increased toxin production was notthrough acquisition and transcription of an additional toxingene. However, as discussed earlier, toxin B levels may havebeen increased through a phage-mediated process of toxin secretion.Alternatively, toxin expression may have been up-regulated inthese lysogens.

View larger version (29K):
[in this window]
[in a new window]

Fig. 2. Toxin A and B of lysogens compared to parental strains. (a) Toxin A titres, expressed as absorbance units, were determined by ELISA. The end point dilution was the reciprocal of the minimum dilution that resulted in an A₄₅₀ $<=$ 0.09. (b) Minimum cytotoxic titre (MCT) of toxin B was determined by neutral red assay. Data are expressed as mean ± SEM. *, P values < 0.01; na, the strain was not a host of the phage, or a stable lysogen was not isolated.

Toxin A and B expression in lysogens and parents (real-time RT-PCR)

A relative quantitative method of real-time RT-PCR was employedto compare toxin transcripts in parental isolates and lysogens.Coordinated transcription of tcdA and tcdB after phage infectionwas observed in all lysogens except CD594C8 and CD6938C6, inwhich significant changes in the amounts of tcdA transcriptswere observed (Fig. 3). This is unusual as tcdA and tcdB transcriptionis co-regulated (Hammond et al., 1997; Hundsberger et al., 1997)through tcdD (Mani & Dupuy, 2001), which is responsive togrowth phase, constituents of medium, and temperature (Karlsson et al., 2003;Mani et al., 2002). Interestingly, phage infectionincreased tcdA transcription in CD594C8 but not TcdA production,while phage infection did not affect tcdB transcription butincreased TcdB production in four lysogens (Table 3). This suggeststhat phage infection has a greater effect on toxin productionor release than transcription of tcdA and tcdB, perhaps throughthe action of holins. In lysogens, functional holins may resultin channels that are only large enough for TcdB (266 kDa) topass through but not TcdA (308 kDa), hence extracellular TcdAlevels are unaltered. However, a recent study on the size ofmembrane lesions formed by the ${lambda}$ holin showed that a proteinof 480 kDa passed through the lesions. The authors suggestedthat holins may not form channels of a constant diameter, butrather cause general disruption of the cell membrane (Wang et al., 2003).

View larger version (35K):
[in this window]
[in a new window]

Fig. 3. Level of tcdA and tcdB transcripts in lysogens compared to parental strains by real-time RT-PCR. Coordinated transcription of tcdA and tcdB was observed in all lysogens except CD594C8 and CD6938C6. (a) Toxin A transcription was significantly increased in CD594C8 but significantly decreased in CD6938C8 compared to the corresponding parental strain. (b) The overall trend of toxin B transcription in lysogens is similar to that in (a). *, P values < 0.01. Data are expressed as mean ± SEM. Input RNA was determined using a calibrator sample from which a standard curve was constructed.

View this table:
[in this window]
[in a new window]

Table 3. Summary of toxin levels and toxin gene transcription in lysogens of ${phi}$ C2, ${phi}$ C5 and ${phi}$ C8 +, Toxin level in lysogen is significantly higher than parental strain; 0, no change or insignificant change in toxin level of lysogen compared to parental strain; –, toxin level in lysogen is significantly lower than parental strain.

The PaLoc of C. difficile has characteristics of a mobile element;non-toxigenic strains lack this virulence element (Braun et al., 1996).Perhaps the homology of tcdE, tcdA and tcdB to phagesequences discussed so far indicates that the PaLoc was carriedby phages that integrated at a specific site and conferred toxigenicityto ancestral C. difficile strains. However, functional prophagegenes have disintegrated severely and the present PaLoc is aremnant of cryptic phage genes. The inability of contemporaryphages to convert contemporary non-toxigenic C. difficile strainsto toxin production could be due to phage genomes having evolvedto play some other role in the biology of C. difficile. In summary,toxin production was not always directly correlated with toxintranscription in lysogens. Differences in toxin levels appearedto be dependent on the parental strains rather than the infectingphage, since these changes were not associated with a specificphage, and occurred in some, but not all, lysogens of ${phi}$ C2, ${phi}$ C6and ${phi}$ C8. Variable toxin levels may be related to the toxinotypeof parental strains, given the putative relationship of PaLocand phage genes. Certain toxinotypes might also be more readilylysogenized and/or exhibit greater stability of lysogenic phages.Identification and sequencing of the holin genes in the phages,as well as site-directed mutagenesis of tcdE, will be necessaryfor determining the role of phages in toxin production or secretionin C. difficile.

REFERENCES

TOP
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
REFERENCES

Adams, M. (1959). Bacteriophages: New York: Interscience.

Angeletti, B., Battiloro, E., Pascale, E. & D'Ambrosio, E. (1995). Southern and Northern blot fixing by microwave oven. Nucleic Acids Res 23, 879–880.[Free Full Text]

Barroso, L. A., Moncrief, J. S., Lyerly, D. M. & Wilkins, T. D. (1994). Mutagenesis of the Clostridium difficile toxin B gene and effect on cytotoxic activity. Microb Pathog 16, 297–303.[CrossRef][Medline]

Bartlett, J. G., Moon, N., Chang, T. W., Taylor, N. & Onderdonk, A. B. (1978). Role of Clostridium difficile in antibiotic-associated pseudomembranous colitis. Gastroenterology 75, 778–782.[Medline]

Braun, V., Hundsberger, T., Leukel, P., Sauerborn, M. & von Eichel-Streiber, C. (1996). Definition of the single integration site of the pathogenicity locus in Clostridium difficile. Gene 181, 29–38.[CrossRef][Medline]

Bruggemann, H., Baumer, S., Fricke, W. F. & 8 other authors (2003). The genome sequence of Clostridium tetani, the causative agent of tetanus disease. Proc Natl Acad Sci U S A 100, 1316–1321.[Abstract/Free Full Text]

Canchaya, C., Desiere, F., McShan, W. M., Ferretti, J. J., Parkhill, J. & Brussow, H. (2002). Genome analysis of an inducible prophage and prophage remnants integrated in the Streptococcus pyogenes strain SF370. Virology 302, 245–258.[CrossRef][Medline]

Dove, C. H., Wang, S. Z., Price, S. B., Phelps, C. J., Lyerly, D. M., Wilkins, T. D. & Johnson, J. L. (1990). Molecular characterization of the Clostridium difficile toxin A gene. Infect Immun 58, 480–488.[Abstract/Free Full Text]

Faust, C., Ye, B. & Song, K. P. (1998). The enzymatic domain of Clostridium difficile toxin A is located within its N-terminal region. Biochem Biophys Res Commun 251, 100–105.[CrossRef][Medline]

Freeman, J. & Wilcox, M. H. (2003). The effects of storage conditions on viability of Clostridium difficile vegetative cells and spores and toxin activity in human faeces. J Clin Pathol 56, 126–128.[Abstract/Free Full Text]

Goh, S., Riley, T. & Chang, B. (2005). Isolation and characterization of temperate bacteriophages of Clostridium difficile. Appl Environ Microbiol (in press).

Hammond, G. A. & Johnson, J. L. (1995). The toxigenic element of Clostridium difficile strain VPI 10463. Microb Pathog 19, 203–213.[CrossRef][Medline]

Hammond, G. A., Lyerly, D. M. & Johnson, J. L. (1997). Transcriptional analysis of the toxigenic element of Clostridium difficile. Microb Pathog 22, 143–154.[CrossRef][Medline]

Hundsberger, T., Braun, V., Weidmann, M., Leukel, P., Sauerborn, M. & von Eichel-Streiber, C. (1997). Transcription analysis of the genes tcdA-E of the pathogenicity locus of Clostridium difficile. Eur J Biochem 244, 735–742.[Medline]

Karcher, S. J. (1995). Molecular Biology: a Project Approach. San Diego: Academic Press.

Karlsson, S., Dupuy, B., Mukherjee, K., Norin, E., Burman, L. G. & Akerlund, T. (2003). Expression of Clostridium difficile toxins A and B and their sigma factor TcdD is controlled by temperature. Infect Immun 71, 1784–1793.[Abstract/Free Full Text]

Kato, N., Ou, C. Y., Kato, H., Bartley, S. L., Brown, V. K., Dowell, V. R. & Ueno, K. (1991). Identification of toxigenic Clostridium difficile by the polymerase chain reaction. J Clin Microbiol 29, 33–37.[Abstract/Free Full Text]

Kato, H., Kato, N., Watanbe, K. & 7 other authors (1998). Identification of toxin A-negative, toxin B-positive Clostridium difficile by PCR. J Clin Microbiol 36, 2178–2182.[Abstract/Free Full Text]

Ketley, J. M., Haslam, S. C., Mitchell, T. J., Stephen, J., Candy, D. C. & Burdon, D. W. (1984). Production and release of toxins A and B by Clostridium difficile. J Med Microbiol 18, 385–391.[Abstract/Free Full Text]

Kutyavin, I. V., Afonina, I. A., Mills, A. & 11 other authors (2000). 3'-minor groove binder-DNA probes increase sequence specificity at PCR extension temperatures. Nucleic Acids Res 28, 655–661.[Abstract/Free Full Text]

Lyerly, D. M., Lockwood, D. E., Richardson, S. H. & Wilkins, T. D. (1982). Biological activities of toxins A and B of Clostridium difficile. Infect Immun 35, 1147–1150.[Abstract/Free Full Text]

Lyerly, D. M., Saum, K. E., MacDonald, D. K. & Wilkins, T. D. (1985). Effects of Clostridium difficile toxins given intragastrically to animals. Infect Immun 47, 349–352.[Abstract/Free Full Text]

Mahony, D. E., Bell, P. D. & Easterbrook, K. B. (1985). Two bacteriophages of Clostridium difficile. J Clin Microbiol 21, 251–254.[Abstract/Free Full Text]

Mahony, D. E., Gilliatt, E., Dawson, S., Stockdale, E. & Lee, S. H. (1989). Vero cell assay for rapid detection of Clostridium perfringens enterotoxin. Appl Environ Microbiol 55, 2141–2143.[Abstract/Free Full Text]

Mani, N. & Dupuy, B. (2001). Regulation of toxin synthesis in Clostridium difficile by an alternative RNA polymerase sigma factor. Proc Natl Acad Sci U S A 98, 5844–5849.[Abstract/Free Full Text]

Mani, N., Lyras, D., Barroso, L., Howarth, P., Wilkins, T., Rood, J. I., Sonenshein, A. L. & Dupuy, B. (2002). Environmental response and autoregulation of Clostridium difficile TxeR, a sigma factor for toxin gene expression. J Bacteriol 184, 5971–5978.[Abstract/Free Full Text]

Mukherjee, K., Karlsson, S., Burman, L. G. & Akerlund, T. (2002). Proteins released during high toxin production in Clostridium difficile. Microbiology 148, 2245–2253.[Abstract/Free Full Text]

Nagy, E. & Foldes, J. (1991). Electron microscopic investigation of lysogeny of Clostridium difficile strains isolated from antibiotic-associated diarrhea cases and from healthy carriers. APMIS 99, 321–326.[Medline]

Pfeifer, G., Schirmer, J., Leemhuis, J., Busch, C., Meyer, D. K., Aktories, K. & Barth, H. (2003). Cellular uptake of Clostridium difficile toxin B: translocation of the N-terminal catalytic domain into the cytosol of eukaryotic cells. J Biol Chem 278, 44535–44541.[Abstract/Free Full Text]

Proux, C., van Sinderen, D., Suarez, J., Garcia, P., Ladero, V., Fitzgerald, G. F., Desiere, F. & Brussow, H. (2002). The dilemma of phage taxonomy illustrated by comparative genomics of Sfi21-like Siphoviridae in lactic acid bacteria. J Bacteriol 184, 6026–6036.[Abstract/Free Full Text]

Riley, T. V., O'Neill, G. L., Bowman, R. A. & Golledge, C. L. (1994). Clostridium difficile-associated diarrhoea: epidemiological data from Western Australia. Epidemiol Infect 113, 13–20.[Medline]

Sambrook, J., Fritsch, E. F. & Maniatis, T. (1989). Molecular Cloning: a Laboratory Manual, 2nd edn. Cold Spring Harbor, NY: Cold Spring Harbor Laboratory.

Tan, K. S., Wee, B. Y. & Song, K. P. (2001). Evidence for holin function of tcdE gene in the pathogenicity of Clostridium difficile. J Med Microbiol 50, 613–619.[Abstract/Free Full Text]

Wang, I. N., Smith, D. L. & Young, R. (2000). Holins: the protein clocks of bacteriophage infections. Annu Rev Microbiol 54, 799–825.[CrossRef][Medline]

Wang, I. N., Deaton, J. & Young, R. (2003). Sizing the holin lesion with an endolysin-beta-galactosidase fusion. J Bacteriol 185, 779–787.[Abstract/Free Full Text]

This article has been cited by other articles:

R. Govind, G. Vediyappan, R. D. Rolfe, B. Dupuy, and J. A. Fralick
Bacteriophage-Mediated Toxin Gene Regulation in Clostridium difficile
J. Virol., December 1, 2009; 83(23): 12037 - 12045.
[Abstract] [Full Text] [PDF]

L.-C. Fortier and S. Moineau
Morphological and Genetic Diversity of Temperate Phages in Clostridium difficile
Appl. Envir. Microbiol., November 15, 2007; 73(22): 7358 - 7366.
[Abstract] [Full Text] [PDF]

S. Goh, P. F. Ong, K. P. Song, T. V. Riley, and B. J. Chang
The complete genome sequence of Clostridium difficile phage {phi}C2 and comparisons to {phi}CD119 and inducible prophages of CD630
Microbiology, March 1, 2007; 153(3): 676 - 685.
[Abstract] [Full Text] [PDF]

R. Govind, J. A. Fralick, and R. D. Rolfe
Genomic Organization and Molecular Characterization of Clostridium difficile Bacteriophage {Phi}CD119.
J. Bacteriol., April 1, 2006; 188(7): 2568 - 2577.
[Abstract] [Full Text] [PDF]

I. R Poxton
Clostridium difficile
J. Med. Microbiol., February 1, 2005; 54(2): 97 - 100.
[Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Alert me when this article is cited

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via CrossRef

Citing Articles via Google Scholar

Google Scholar

Articles by Goh, S.

Articles by Riley, T. V

Search for Related Content

PubMed

PubMed Citation

Articles by Goh, S.

Articles by Riley, T. V

Agricola

Articles by Goh, S.

Articles by Riley, T. V

				L.-C. Fortier and S. Moineau Morphological and Genetic Diversity of Temperate Phages in Clostridium difficile Appl. Envir. Microbiol., November 15, 2007; 73(22): 7358 - 7366. [Abstract] [Full Text] [PDF]

				S. Goh, P. F. Ong, K. P. Song, T. V. Riley, and B. J. Chang The complete genome sequence of Clostridium difficile phage {phi}C2 and comparisons to {phi}CD119 and inducible prophages of CD630 Microbiology, March 1, 2007; 153(3): 676 - 685. [Abstract] [Full Text] [PDF]

				R. Govind, J. A. Fralick, and R. D. Rolfe Genomic Organization and Molecular Characterization of Clostridium difficile Bacteriophage {Phi}CD119. J. Bacteriol., April 1, 2006; 188(7): 2568 - 2577. [Abstract] [Full Text] [PDF]

				I. R Poxton Clostridium difficile J. Med. Microbiol., February 1, 2005; 54(2): 97 - 100. [Full Text] [PDF]