Development of a Rapid PCR Method Using the Insertion Sequence IS1203 for Genotyping Shiga Toxin-Producing Escherichia coli O157

We developed a rapid PCR method utilizing the diversity of theinsertion site IS1203 for genotyping Shiga toxin-producing Escherichiacoli (STEC) O157 (IS1203 PCR typing). DNA fragments digestedby PvuII, which cut IS1203 at one site, were ligated with themselvesand detected by PCR with outward-facing primer pairs for IS1203.To minimize nonspecific bands, nested PCR was also performed.Two fingerprinting patterns produced from the upstream or downstreamregions of IS1203 were obtained within 1 or 2 days. By combiningthe two patterns, 79 STEC O157 isolates were classified into39 types, which were then classified into 36 subtypes by pulsed-fieldgel electrophoresis (PFGE). The discriminatory power of IS1203PCR typing (D = 0.974) is similar to that of PFGE (D = 0.981).This method can be used for rapid and simplified genotyping.

INTRODUCTION

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Introduction

Shiga toxin-producing Escherichia coli (STEC) O157 is associatedwith outbreaks and sporadic cases of diarrhea, hemorrhagic colitis,and hemolytic-uremic syndrome. Genotyping is a useful way toidentify strains with the same genetic background. Pulsed-fieldgel electrophoresis (PFGE) is a standard and effective methodfor genotyping STEC O157 (11, 16). Many studies have reportedthat STEC O157 can be classified into numerous genotypes byPFGE (1, 5, 7). However, PFGE is time-consuming and technicallydemanding and requires a special electrophoresis system.

The genomes of most bacteria contain distinct classes of insertionsequences (IS). IS typing involves utilizing the diversity ofinsertion sites. For some bacterial species, IS typing can beutilized for genotyping methods other than PFGE. For Mycobacteriumtuberculosis, restriction fragment length polymorphism (RFLP)analysis using the sequence IS6110 is a standard genotypingmethod (12, 18). This method is time-consuming because it isa standard Southern blotting-based technique. Several studieshave investigated genotyping methods using PCR with insertionsequence primers. Otal et al. (13) reported on an IS6110-basedPCR method using single outward-facing primers for IS6110 thatis comparable to standardized IS6110 RFLP analysis methods.IS typing by PCR has also been developed for STEC O157. Thompsonet al. (17) reported that the band patterns yielded by IS3 typingfor E. coli using outward-facing primers are not as variableas those produced by PFGE.

STEC O157 contains the IS1203 sequence in addition to IS3. IS1203was reported by Paton and Paton (14) for the E. coli O111:H^–strain PH. IS1203 is a 1,312-nucleotide sequence with imperfect26-bp terminal inverted repeats and is closely related to theIS629 sequence of Shigella sonnei (10) and IS3411 of E. coli(4). At least 12 copies of IS1203 have been found in the genomeof the E. coli O111:H^– strain PH (14). IS1203 sequenceswere found in the genome sequence data of STEC O157 EDL933 (accessionno. NC_002655) (12 copies) and of the Sakai strain (accessionno. NC_002695) (19 copies). IS1203 was also found in the stx₁and stx₂ genes of STEC O157 (8, 15) and in phage carrying stx₂(6).

In this study, we developed a genotyping method using IS1203(referred to here as IS1203 PCR typing) which is similar tothe IS6110-inverse-PCR method developed by Otal et al. (13).We attempted to create a rapid and reproducible PCR genotypingprotocol using ligation and nested PCR.

MATERIALS AND METHODS

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Materials and Methods

Strains. Seventy-nine STEC O157 strains derived from patients (n = 64)and cattle (n = 15) were used. They were isolated in Aichi Prefecture,Japan, from 1999 to 2002 except for one strain, which was derivedfrom the Sakai outbreak in 1996 (2, 9). The origins of strainsobtained from patients were as follows: 29 strains from 9 outbreakcases, 1 strain from the Sakai outbreak, and 34 strains fromsporadic cases.

PFGE. PFGE was performed as described elsewhere (1), with minor modifications.In brief, bacterial cells cultured in Luria-Bertani (LB) brothat 37°C overnight with shaking were directly embedded inlow-melting-temperature agarose (Nippon Gene, Tokyo, Japan).After appropriate preparations for restriction endonucleasedigestion were made, the DNA in each plug was digested with30 U of XbaI (Roche Diagnostics, Mannheim, Germany) at 37°Covernight. PFGE was performed on a 1% agarose gel by using aGene Navigator system (Pharmacia Biotech AB, Uppsala, Sweden)in 0.5x Tris-borate-EDTA buffer at 200 V. For whole-genome separation,linearly ramped switching times from 1 to 40 s were appliedfor 22 h. ${lambda}$ DNA concatemers (Bio-Rad Laboratories, Hercules,Calif.) were used as size markers, and the gels were visualizedby ethidium bromide staining and photographed under a transilluminator.The patterns were analyzed with FingerPrinting II software (version4.2; Bio-Rad Laboratories). A dendrogram was drawn from thisdata by the unweighted pair group method with arithmetic averages(UPGMA), and similarity coefficients were calculated by theJaccard method. PFGE patterns were sorted by FingerPrintingII and visually compared by using the criteria of Tenover etal. (16). Major strain types were designated by letters, withnumbers added for subtypes.

IS1203 PCR typing. A schematic drawing of IS1203 PCR typing is shown in Fig. 1.Strains were cultured in LB broth at 37°C overnight withshaking, and chromosomal DNA was purified by using a DNeasytissue kit (QIAGEN, Hilden, Germany) according to the manufacturer'sinstructions. Five hundred nanograms of purified DNA was digestedby 10 U of the PvuII restriction enzyme (Roche Diagnostics)for 1 h at 37°C. The digested DNA was purified by phenolextraction and ethanol precipitation and was then dissolvedin 500 µl of distilled water. As IS1203 was digested byPvuII at one site (Fig. 1a), each of the digested fragmentscontained an upstream or a downstream region of IS1203. To detectfragments containing IS1203, digested DNA fragments were self-ligatedby using a Rapid DNA Ligation kit (Roche Diagnostics). Ligationwas performed in a total volume of 10 µl containing 2to 4 ng of digested DNA for 30 min at 20°C. The self-ligatedDNA was detected by PCR using primer pair 1203-82 (5'-CAC GTTCCA GCT CTT TCA G-3') and 1203-11 (5'-GAC TGG CTG AAG AGA GAGAT-3') for fragments containing the upstream region of IS1203(upstream typing), and primer pair 1203-62 (5'-TAA ACG CCA CATAGA CGA AGC C-3') and 1203-31 (5'-GTA TGA CAA CGC GAT GGC T-3')for fragments containing the downstream region (downstream typing).PCR was performed in a volume of 25 µl containing 2.5µl of ligated DNA, EX-Taq buffer, deoxynucleoside triphosphates,0.2 µM each primer, and 1 U of EX-Taq (Takara Bio, Ohtsu,Japan). PCR cycles consisted of 94°C for 1 min, 55°Cfor 45 s, and 72°C for 1 min, and PCR was performed for20 cycles by using a GeneAmp PCR system 9600 (Applied BiosystemsJapan, Tokyo, Japan).

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FIG. 1. Schematic diagram of IS1203 PCR typing. (a) IS1203 sequences were divided into two fragments, the upstream (open box) and downstream (solid box) fragments, by PvuII digestion between nucleotides 1032 and 1033 (arrowhead). Arrows indicate the primer regions for upstream typing (1203-82 and 1203-11 for first PCR, and 1203-72 and 1203-21 for nested PCR) and downstream typing (1203-62 and 1203-31 for first PCR, and 1203-52 and 1203-41 for nested PCR). (b) Detection of PvuII-digested fragments containing IS1203. STEC O157 genomic DNA contains more than 10 copies of IS1203 (two copies of IS1203 are shown in the figure for simplicity). Open box, IS1203 upstream region; solid box, downstream region. STEC O157 genomic DNA was digested at the PvuII recognition sites (arrowheads). Digested fragments were then self-ligated. Ligated fragments containing IS1203 were amplified by PCR in the direction of the arrows. Fragments containing upstream or downstream regions of IS1203 were reacted. Nested PCR was performed for accuracy, and two electrophoresis patterns (upstream and downstream patterns) were obtained from one strain.

To minimize nonspecific bands, nested PCR was performed by usingprimer pair 1203-72 (5'-GCG TAC AGC CAA TCT TTG G-3') and 1203-21(5'-GTT ATG GGA CTT GCC GGT GTT-3') for upstream typing andprimer pair 1203-52 (5'-TGC CAT GTG CTG ACG TAA G-3') and 1203-41(5'-GAA AAA CCG TGC AGA AGT GG-3') for downstream typing. PCRwas performed as described above except that 1 µl of theproduct from the first PCR procedure was used as the DNA template.Five microliters of nested PCR products was separated by electrophoresisin a 2.0% DNA agar gel (Marine BioProducts, Delta, British Columbia,Canada) at a constant voltage of 50 V for 2.5 h by using a Mupid-2Mini Electrophoresis unit (Advancebio, Tokyo, Japan). Gels werevisualized by ethidium bromide staining and photographed undera UV transilluminator. A 100-bp molecular size marker ladder(Nippon Gene) was used as a reference. The patterns were analyzedwith FingerPrinting II software (version 4.2) as a compositedata set of upstream and downstream typing. A dendrogram wasdrawn from these data by use of UPGMA, with the weight betweenthe upstream and downstream typing set at 1:1.

IS1203 PCR type names were assigned as follows. Clusters withmore than 30% similarity were given Greek letters, from ${alpha}$ to ${eta}$ ; subclusters with more than 60% similarity were designatedby Roman numerals within the same cluster; and IS1203 PCR patternswith 1 or 2 differences in the bands had Arabic numerals added.Clusters or subclusters without subdivisions were not givena lower class name. Seven randomly selected strains, includingtwo strains with the same PFGE pattern, were used to test forreproducibility. The reproducibility tests were performed underthe same conditions three times.

Statistical analysis. The numerical index of discrimination (D index) for IS1203 PCRtyping and PFGE, defined as the average probability that differentgenotyping was assigned to two unrelated strains in a populationof a given genus, was calculated by the method of Hunter andGaston (3).

RESULTS

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Results

PFGE analysis. Seventy-nine strains were classified into 24 types (A to Y;to avoid confusion with the number zero, the letter O was notassigned) by PFGE. Strains within the same type had similaritycoefficients of >70% (Fig. 2). Five types were further subdividedinto 17 subtypes: A1 to A7, B1 and B2, J1 and J2, U1 to U4,and X1 and X2. From the results of PFGE subtyping, 79 strainswere classified into 36 PFGE subtypes. Strains obtained froman outbreak were classified as belonging to the same PFGE type,and the D index was 0.981 for PFGE.

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FIG. 2. A dendrogram based on PFGE patterns was drawn by using UPGMA. PFGE patterns are also shown. Shiga toxin-producing types and PFGE types are shown in the Stx and PFGE type columns. Superscript numbers or letters following strain designations indicate origins, as follows: #1 through #9, strains isolated from outbreaks; S, strain isolated from the Sakai outbreak; C, strains isolated from cattle stool.

IS1203 PCR typing. We repeated IS1203 PCR typing three times for seven strains(Fig. 3). For these tests, the same electrophoresis patternswere obtained in the 1.2-kbp region. Bands above 1.2 kbp fordownstream typing of strains 2-051 and 0-536 were not stablein the repeated test.

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FIG. 3. Electrophoresis patterns of IS1203 PCR typing repeated three times. Electrophoresis patterns under 1.2 kbp were the same for all strains. Large fragments had a tendency to be unstable (downstream typing, strains 2-051 and 0-536).

Three to nine bands under 1.2 kbp were detected by upstreamtyping for each strain, and the strains were classified into29 upstream types. Thirty of 79 strains were classified into18 types with one-to-one correspondence to PFGE, and the other49 strains, classified into 11 upstream types, were dividedinto 18 subtypes by PFGE. The D index was 0.921 for upstreamtyping.

One to nine bands under 1.2 kbp were detected by downstreamtyping, but two strains exhibited no band. Seventy-seven strainswhich exhibited more than one band were classified into 27 downstreamtypes. Seventeen of these 77 strains were classified into 10types with one-to-one correspondence to PFGE. The other 60 strains,which were classified into 17 downstream types, were dividedinto 24 subtypes by PFGE. The D index was 0.952 for downstreamtyping.

Based on the composite data set that combined the fingerprintingpatterns of upstream and downstream typing, 79 strains wereclassified into 39 types (Fig. 4). IS1203 PCR types were dividedinto four major clusters (clusters ${alpha}$ to ${delta}$ ) and three independenttypes ( ${varepsilon}$ , ${zeta}$ , and ${eta}$ ). Forty-one strains exhibited 25 patterns withone-to-one correspondence to PFGE (Fig. 4). Another 17 strainswere classified into 12 types by IS1203 PCR typing and into6 types by PFGE (Table 1). Some strains with the same PFGE typehad IS1203 PCR types in different clusters: two strains withPFGE type U2 were classified as ${alpha}$ -II-2 and ${zeta}$ , respectively, andtwo strains with PFGE type D were classified as ${gamma}$ -I-1 and ${delta}$ -II,respectively. Finally, 21 strains were classified into two typesby IS1203 PCR typing and into six subtypes by PFGE (Table 2).Seven strains of one IS1203 PCR type (ß-I-5) wereclassified into four major PFGE types. Strains collected fromthe same outbreak had the same IS1203 PCR type. The D indexwas 0.974 for IS1203 PCR typing with composite data sets.

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FIG. 4. A dendrogram was drawn by using a composite data set of upstream and downstream patterns obtained from IS1203 PCR typing by UPGMA. The electrophoresis patterns of upstream anddownstream typing are also shown. The patterns were divided into four major clusters (clusters ${alpha}$ to ${delta}$ ) and three independent types. Pattern designations obtained from composite IS1203 PCR typing data and from PFGE are shown in the respective columns. IS1203 PCR types exhibiting one-to-one correspondence with the PFGE subtypes are asterisked. Superscript numbers or letters following strain designations indicate origins, as follows: #1 through #9, strains isolated from outbreaks; S, strain isolated from the Sakai outbreak; C, strains isolated from cattle stool.

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TABLE 1. IS1203 PCR types with the same PFGE pattern

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TABLE 2. IS1203 PCR types with different PFGE patterns

DISCUSSION

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Discussion

This is the first report of PCR typing of STEC O157 strainsby use of IS1203. To easily carry out IS typing, several researchershave developed IS-typing PCR methods. Most of these use singleprimers for the IS3 sequence of E. coli (17) or the IS6110 sequenceof M. tuberculosis (13).

In this study, we developed an IS-typing PCR method that utilizesand is similar to the IS6110-inverse-PCR method developed byOtal et al. (13), which involves IS typing using digestion withthe restriction endonuclease PstI, ligation, and PCR. AlthoughOtal et al. expected more bands by IS6110-inverse PCR, the numberof bands was not higher than that obtained by IS6110 PCR typingwithout the ligation step. The fragment size produced in standardRFLP analysis with IS6110 by PstI digestion is greater than1 kbp (12). We hypothesized that the fragments should be shortenough to be amplified by PCR. Prolonging the PCR extensionstep was not effective for amplifying large fragments (datanot shown). The advantages of this protocol are as follows.First, to increase the discriminatory power of IS1203 PCR typing,PvuII digestion and ligation were performed. As IS1203 was cutat one site by PvuII, we obtained two fingerprint patterns containingthe upstream and downstream regions of IS1203, respectively.This produced characteristic patterns for each strain, and thecombination of these patterns increases the discriminatory powerof IS1203 PCR typing. In addition, the fragments were shortenough to facilitate PCR amplification (the expected lengthwas less than 1 kbp in about one-third of the bands generatedfrom the Sakai strain), and we could obtain stable bands. Second,we acquired reproducible results, because ligation and nestedPCR minimized nonspecific bands under 1.2 kbp. We observed thatsome amplicons in the first PCR disappeared from nested-PCRproducts (data not shown). This suggested that some nonspecificreaction(s) occurred in the first PCR and that such nonspecificbands could be removed by the second PCR. We expected that minimizationof nonspecific bands would improve reproducibility. Therefore,we performed nested PCR to obtain reproducible results. Althoughwe could obtain reproducible results for most strains, furtherinterlaboratory reproducibility studies are required.

Concerning the discriminatory power of IS1203 PCR typing, PFGEidentified 36 different subtypes and IS1203 PCR typing identified39. Thompson et al. (17) developed a subtyping method basedon PCR amplification of variable DNA sequences between the repetitiveIS3 elements of STEC O157 and reported that PFGE identified25 different subtypes and IS3-based PCR identified 15. IS1203PCR typing allows for higher discriminatory power than IS3-basedPCR. The D index (0.974) for IS1203 PCR typing was slightlylower than that for PFGE (0.981) in this study, suggesting thatthe discriminatory power of our method is slightly lower thanthat of PFGE. However, the D index (0.974) indicates that iftwo strains from a population are randomly sampled, 97.4% ofthe time they will belong to different types (3). We believethat most strains can be identified by IS1203 PCR typing.

IS1203 PCR typing is an easy and rapid genotyping method witha sensitivity similar to that of PFGE. This method can be usedto screen STEC O157 isolates.

ACKNOWLEDGMENTS

This work was supported by grants from the Ministry of Health,Labor, and Welfare of Japan.

FOOTNOTES

* Corresponding author. Mailing address: 7-6 Nagare Tsuji-machi Kita-ku, Nagoya 462-8576, Aichi, Japan. Phone: 81-52-910-5669. Fax: 81-52-913-3641. E-mail: masahiro_4_suzuki{at}pref.aichi.lg.jp.

REFERENCES

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