Typing by sequencing the slpA gene of Clostridium difficile strains causing multiple outbreaks in Japan

doi:10.1099/jmm.0.45807-0

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Typing by sequencing the slpA gene of Clostridium difficile strains causing multiple outbreaks in Japan

Haru Kato¹, Toshiyuki Yokoyama² and Yoshichika Arakawa¹

¹Department of Bacterial Pathogenesis and Infection Control, National Institute of Infectious Diseases, 4-7-1 Gakuen, Musashimurayama, Tokyo 208-0011, Japan ²Kumiai Hospital, 5-68 Ozinmachi, Takayama Gifu 506-8502, Japan

Correspondence Haru Kato cato{at}nih.go.jp

Received July 1, 2004
Accepted October 18, 2004

Previous reports have documented that a surface layer protein(SlpA) varies among Clostridium difficile isolates. The typingsystem by sequencing the variable region of the slpA gene wasapplied to typing C. difficile strains belonging to one PCRribotype, type smz, which has been identified as frequentlycausing outbreaks in Japan. The PCR ribotype smz strains recoveredfrom patients at different hospitals in Japan were examined.Among 10 type smz strains tested, three subtypes, smz-1, -2and -3, were identified that differed from each other by onenucleotide. slpA sequence typing was also applied to directtyping on DNA extracted from stool specimens. Of 22 stool specimensexamined, 17 were PCR positive for slpA; eight were typed asslpA sequence type smz-1 and nine as type smz-2. C. difficilewas cultured from 12 of these 17 stool specimens, and the sequenceresults of the recovered isolates were compared with those fromthe DNA extracted from the stool specimens. In all 12 of thesestool specimens, the sequence results of DNA from recoveredC. difficile isolates completely agreed with those of DNA extracteddirectly from stool specimens. The remaining five stool specimenswere culture-negative for C. difficile. Sequence typing hasthe advantage of enabling easy comparison of typing resultsamong multiple laboratories via the Internet without exchangingreference strains as is required in typing systems which dependon banding-pattern analyses. slpA sequence typing appears tobe a reproducible and reliable typing system for C. difficileas well as being useful for the typing of C. difficile whenstool specimens contain only small numbers of C. difficile orare inappropriate for culturing.

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

Abbreviations: AP-PCR, arbitrarily primed PCR; MLST, multilocussequence typing; REA, restriction enzyme analysis.

The GenBank/EMBL/DDBJ accession numbers for the sequences ofthe variable regions of the slpA gene of strain GAI 97660 (slpAsequence type smz-1), strain MRY 04-0409 (slpA sequence typesmz-2) and strain MRY 04-0410 (slpA sequence type smz-3) areAB180242, AB181350 and AB181351, respectively.

Introduction

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Introduction
Methods
ACKNOWLEDGEMENTS
References

It is well known that Clostridium difficile readily spreadsnosocomially (Brazier, 1998; Johnson et al., 1999; Kato et al., 2001).It has been documented that specific strains cause multiplenosocomial outbreaks over the world. In the USA (Samore et al., 1997;Johnson et al., 1999), a single strain or two highly relatedtypes, i.e. restriction enzyme analysis (REA) type J9 and J7/arbitrarilyprimed PCR (AP-PCR) type 01/AP-PCR type A, have been shown tobe involved in epidemics in a number of hospitals. The epidemicstrain that caused an outbreak in New York was typed as serogroupG (H. Kato et al., 1993) and PCR ribotype gr (Kato et al., 2001).Brazier and others have reported that PCR ribotype 1 (Stubbs et al., 1999),which corresponded to serogroup G (Brazier et al., 1997),was responsible for most of the published outbreaksin the UK (Brazier, 1998). In addition, they typed a USA outbreakstrain in Massachusetts as PCR ribotype 1 (Brazier, 1998). InJapan, one PCR ribotype, type smz, has been identified as frequentlycausing outbreaks (Kato et al., 2001). Interestingly, the epidemicstrains in both the UK and the USA as well as in Japan, i.e.the type smz strain, were non-typable by PFGE typing becauseof DNA degradation (Samore et al., 1997; Corkill et al., 2000;Kato et al., 2001).

The typing results of epidemic strains of outbreaks previouslydocumented are summarized in Table 1. To investigate the pathogenicityof these specific strains, it is necessary to compare the epidemicstrains that are responsible for outbreaks across the world.Since it is not easy to exchange reference strains or antiseraamong different laboratories in different countries, typingsystems in which results do not depend on banding-pattern analysisare required for a study of global epidemiology.

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Table 1. Isolates used and their typing designation in comparison with epidemic strains reported from the USA and UK HK, designated by Kato et al. (2001); JSB, designated by Brazier et al. (1998); GEK, designated by Killgore et al. (1994); MS, designated by Samore et al. (1997).

Previous reports have documented that a surface layer protein(SlpA) varies among C. difficile isolates (McCoubrey & Poxton, 2001;Calabi et al., 2001) and typing results by RFLP analysisof the slpA gene correlate well with those by serogrouping (Karjalainen et al., 2002).In this study, we preliminarily identified theslpA gene of PCR ribotype smz strains recovered at a numberof hospitals in Japan. One of our aims was to examine the variabilityof the slpA gene among smz strains; a second aim was to comparethe sequence results with those of C. difficile previously availablein databases as well as with that of the epidemic strain thatcaused an outbreak in the USA; a third aim was to apply slpAsequence typing to typing of C. difficile directly from stoolspecimens without culturing.

Methods

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Introduction
Methods
ACKNOWLEDGEMENTS
References

Bacterial strains and stool specimens.

Ten C. difficile isolates typed as PCR ribotype smz were obtainedfrom patients at 10 different hospitals in diverse areas ofJapan. The type smz strain was predominant at eight of these10 hospitals, suggesting a nosocomial outbreak of the strainat those eight hospitals; a strain of a type other than smzwas predominant at another hospital, but no dominant strainswere found at the remaining hospital.

Included in the present study were one epidemic strain, strain900233 (serogroup G/AP-PCR type 01/PCR ribotype gr), causingan outbreak in a hospital in upstate New York (H. Kato et al., 1993, 2001;Killgore & Kato, 1994), and a type smz strain,strain 900295, recovered during this New York outbreak (Kato et al., 2001).The epidemic strain from the same hospital inNew York was reported to be AP-PCR type A/REA type J9 (Samore et al., 1997;Johnson et al., 1999).

Stool specimens were obtained with the informed consent of patientsadmitted to Kumiai Hospital, Gifu, Japan who were given thediagnosis of antibiotic-associated diarrhoea. The isolationof C. difficile from stool specimens and the identificationof C. difficile were performed by methods described previously(Kato et al., 1998). Stool specimens were tested for toxin Ausing an immunoassay kit (Oxoid) and for toxin B using a Verocell cytotoxicity assay with a neutralization test by anti-C.difficile toxin B serum (TechLab).

Typing of recovered isolates.

The toxin-producing type of isolates was determined by a PCRmethod described previously (Kato et al., 1998, 1999). PCR ribotypingwas performed as described previously (Stubbs et al., 1999;Kato et al., 2001). The variable region of the slpA gene wasamplified by the primers slpAcom19 (sequence 5'-GTTGGGAGGAATTTAAGRAATG-3')and slpAcom22 (sequence 5'-GCWGTYTCTATTCTATCDTYWCC-3'). ThePCR assay was performed in the same manner as described forthe PCR detection of the toxin genes (Kato et al., 1998) witha modification of the thermal profile, i.e. 35 cycles comprising95 °C for 20 s and 55 °C for 180 s. The PCR productwas purified and sequenced directly with an ABI Prism dye-terminatorcycle sequencing ready reaction kit (PE Applied Biosystems)as described previously (Kato et al., 1999). Both strands ofthe amplified products were sequenced.

Direct typing on stool specimens.

DNA was extracted from stool specimens using the QIAamp DNAstool mini kit (Qiagen). The primers used for a nested PCR detectingthe non-repeating region of the toxin A gene (tcdA) from DNAextracted from stool specimens were HK5 (sequence 5'-AACTTATCCTGGGAAGTTGC-3')and HK6 (sequence 5'-GTGAATTATATTTTTAACAGGCTC-3') for the outerprimer set, and NK3 (sequence 5'-GGAAGAAAAGAACTTCTGGCTCACTCAGGT-3') and NK2 (sequence 5'-CCCAATAGAAGATTCAATAT TAAGCTT-3')for the inner primer set (N. Kato et al., 1993).

The primers used for sequence typing of the slpA gene directlyon DNA extracted from stool specimens were slpAcom19-slpAcom22for the outer primer set, and slpAcom13 (sequence 5'-TAGGTGATGGARAWTAYGTWG-3') and slpAcom12 (sequence 5'-CATAWBBTT TAGCTAAATYTTBWGC-3')for the inner primer set. The primers slpAcom19, slpAcom22,slpAcom13 and slpAcom12 were selected from the conserved regionsof the slpA gene among five PCR ribotype strains frequentlyrecovered in Japan, including a type smz strain.

The PCR assay on DNA extracted from the specimens was performedin a reaction volume of 50 µl consisting of 2.5 mM MgCl₂,50 mM KCl, 10 mM Tris/HCl (pH 9.0), the four deoxynucleosidetriphosphates (200 µM each), 12.5 pM of each primer, 1.25U of Taq DNA polymerase (Promega), 5 µg of BSA and 5 µlof extracted DNA (or PCR product for the second PCR). The thermalprofile was 35 cycles comprising 95 °C for 20 s and 55 °Cfor 180 s for the primer pair slpAcom19-slpAcom22, and 35 cyclescomprising 95 °C for 20 s and 55 °C for 120 s for theother primer pairs. The PCR product from the second PCR withprimers slpAcom13-slpAcom12 was sequenced in the same manneras described for the slpA sequence typing of isolates.

Results and Discussion

The slpA gene of a type smz strain, GAI 97660 (Kato et al., 2001),recovered from a patient with pseudomembranous colitis,was amplified by primers slpAcom19 and slpAcom22, and the resultantPCR product was sequenced. The deduced amino acid sequence ofslpA in GAI 97660 showed the highest identity of 76 % with thatof strain 9354 (GenBank accession no. AF448120), which was characterizedas serogroup A, subgroup unknown (Karjalainen et al., 2002).

Among 10 type smz strains from different areas of Japan, subtypeswere identified (type smz-1, smz-2 and smz-3) that differedfrom each other by one nucleotide, involving a single deducedamino acid that differed for each one. The slpA gene of threestrains, GAI 97660 (type smz-1), MRY 04-0409 (type smz-2) andMRY 04-0410 (type smz-3), was sequenced after 10 subcultureson Brucella HK agar plates (Kyokuto Seiyaku). In each of thethree isolates, the sequence results following serial subculturesagreed with those before subculturing. The numbers of strainstyped as slpA sequence types smz-1, -2 and -3 were five, fourand one, respectively. Strains of all three slpA sequence typeswere detected from outbreaks, and strains of smz-1 and smz-2types from sporadic cases.

The slpA sequence of the New York outbreak strain, 900233, showed38 % homology to that of GAI 97660 and was 100 % identical tothat of strain R8366 (GenBank accession no. AJ300676), whichwas serogrouped as G by Delmee's group (Karjalainen et al., 2002)and typed as PCR ribotype 1 by Brazier's group (Stubbs et al., 1999).During the outbreak at the New York hospital,PCR ribotype smz strains were recovered from three patientsbut, unlike the PCR ribotype gr strain, they did not appearto be involved in the epidemic. One of the three smz isolates,900295, was typed as smz-2 by slpA sequence typing.

These sequence results indicate that the type smz strain clearlydiffers from the strain causing the New York outbreak not onlyby PCR ribotyping (Kato et al., 2001) but also by slpA sequencetyping. The region of slpA examined was found to be conservedamong clinical smz isolates, including the type smz strain whichwas found at the New York hospital but not involved in the epidemicthere. Since strains typed as PCR ribotype smz are non-typableby PFGE because of a DNA degradation problem (Kato et al., 2001),the results of slpA sequence typing cannot be compared withthose by PFGE. While three slpA sequence types were found amongtype smz strains, no predominant subtype was detected in thisstudy.

slpA sequence typing was applied to direct typing on DNA extractedfrom stool specimens obtained from patients at a hospital. Atotal of 22 stool specimens were examined for toxins A and B,C. difficile, and direct PCR detection of tcdA. Of these specimens,17 were PCR-positive for tcdA (results of other tests on these17 are summarized in Table 2). The remaining five specimens,which were PCR-negative for tcdA, were also negative for thedetection of fecal toxins or C. difficile culture.

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Table 2. Detection of toxins A and B, culture for C. difficile, and typing results from direct PCR of 17 stool specimens where direct PCRs were positive for detection of tcdA SlpA S type, slpA sequence type; A⁺B⁺, toxin A-positive, toxin B-positive; ND, not done.

Nested PCR amplification of the slpA gene was performed on the17 stool specimens that were directly PCR-positive for tcdA.The second PCR for slpA generated a PCR product approximately550 bp in size in all 17, and the resultant PCR product wassequenced. Two slpA sequence types, smz-1 and smz-2, were identifiedamong the 17 specimens from the hospital patients, suggestinga nosocomial spread of two subtypes at that hospital. C. difficilewas recovered from 12 of these 17 specimens, and all 12 isolateswere typed as type smz by PCR ribotyping and slpA sequence typing,the results of which completely agreed with those of directsequence typing in all 12 specimens. The nested PCR led to successin the slpA sequence typing of C. difficile in five stool specimenswith negative results on culturing. It was suggested that bothof the nested PCRs detecting tcdA and slpA directly from stoolspecimens used in this study may be more sensitive than culturingC. difficile, although the number of stool specimens testedhere was limited.

The typing results of banding-pattern analyses, such as thoseby AP-PCR, PCR ribotyping, REA or PFGE, may be difficult tocompare in many isolates and to share among different laboratories.Typing by sequencing has the advantage that the typing resultscan be compared among numerous laboratories via the Internetwithout the need for exchanging reference strains or antisera.Recently, multilocus sequence typing (MLST) has been used fora long-term epidemiological study of a variety of bacteria,and its application to C. difficile has been reported (Lemee et al., 2004).Like MLST analysis, the use of slpA sequencetyping may be feasible for a global epidemiological study bysharing typing data from many clinical isolates identified ata number of laboratories. Moreover, this method can be appliedto direct typing from clinical materials. In the present study,five culture-negative specimens were PCR-positive for slpA followedby slpA sequence typing. Such typing is also useful for analysinga specimen containing small numbers of C. difficile or one thatis inappropriate for culturing, such as one stored at ambienttemperature for prolonged periods before laboratory testing.While this method needs to be further evaluated for its typingability on a large number of clinical isolates and stool specimensand for its specificity to the slpA gene of C. difficile, slpAsequence typing appears to be a reproducible, sensitive andreliable typing method for C. difficile.

ACKNOWLEDGEMENTS

TOP
Introduction
Methods
ACKNOWLEDGEMENTS
References

For their valuable help in the collection of strains and specimens,the authors would like to thank T. Yamamoto and K. Suzuki (NagoyashiKoseiin Geriatric Hospital), S. Ishigo (Ogaki Municipal Hospital),M. Kunihiro and I. Nakamura (Yamaguchi Prefectural Hospital),T. Oguri and S. Misawa (Juntendo University Hospital), K. Yoshimoto(Shirasagi Hospital), M. Komatsu and M. Aihara (Tenri Hospital),H. Kato (Toyokawa City Hospital), H. Sato and C. Sakai (ChibaCancer Center Hospital), and G. E. Killgore (Centers for DiseaseControl and Prevention). The technical assistance of Y. Yoshimurais also gratefully acknowledged. This work was supported bya grant-in-aid for Scientific Research (C) from the Ministryof Education, Culture, Sports, Science and Technology, Japan.

References

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