Multidrug-Resistant Streptococcus pneumoniae in Poland: Identification of Emerging Clones

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Journal of Clinical Microbiology, June 1999, p. 1739-1745, Vol. 37, No. 6
0095-1137/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Multidrug-Resistant Streptococcus pneumoniae in Poland: Identification of Emerging Clones

Karin Overweg,¹ Peter W. M. Hermans,¹^,^* Krzysztof Trzcinski,² Marcel Sluijter,¹ Ronald de Groot,¹ and Waleria Hryniewicz²

Department of Pediatrics, Sophia Children's Hospital, Erasmus University Rotterdam, 3000 DR Rotterdam, The Netherlands,¹ and Department of Epidemiology and Clinical Microbiology, Sera and Vaccines Central Research Laboratory, 00-725 Warsaw, Poland²

Received 17 September 1998/Returned for modification 8 December 1998/Accepted 22 February 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Penicillin resistance among Streptococcus pneumoniae isolates has rapidly emerged in Poland during the last decade and hasreached prevalence levels of up to 14.4% in 1997. In order toinvestigate the nature of this increase, a molecular epidemiologicalanalysis of non-penicillin-susceptible multidrug-resistant pneumococciisolated in 1995 and 1996 was conducted. Thirty-seven patientswho suffered mainly from upper respiratory tract infections andpneumococcal pneumonia were enrolled in this study. The medicalcenters to which the patients were admitted were located in 16Polish towns across the country. Eight distinct BOX PCR typeswere observed, representing 14 subtypes. Restriction fragmentend labeling (RFEL) analysis divided the pneumococcal strainsinto 16 distinct types. By combining the BOX PCR and RFEL data,four genetically distinct clusters of strains were identified.Two clusters represented the genetic clones 23F and 9V, whichhave recently emerged all over the world. The two other geneticclusters, which represented serotypes 23F and 6B, clearly predominatedin the analyzed collection of Polish non-penicillin-susceptiblepneumococcal strains. Since the latter clusters did not matchany of the 133 RFEL types of non-penicillin-susceptible pneumococcicollected in 15 other countries, their Polish clonal origin ismostlikely.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Streptococcus pneumoniae (pneumococcus) continues to be a common cause of serious and life-threatening infections, such aspneumonia, bacteremia, and meningitis, and of noninvasive infections,such as otitis media and sinusitis (3). In addition, pneumococciare often part of the normal nasopharyngeal flora. Especiallyin young children, pneumococcal colonization often occurs. Colonizationis an important risk factor: children colonized with S. pneumoniaemore often develop acute otitis media than children who are notcolonized (9, 18, 33, 43).

Until the 1960s, pneumococci were considered uniformly susceptible to penicillin, and sensitivity tests were hardly ever performed.In 1967, the first isolation of penicillin-resistant pneumococciwas reported in Australia (12). Subsequently, penicillin-resistantpneumococci have been isolated in Papua New Guinea and South Africa(20, 22, 31). In the late 1970s and 1980s, rates of resistance,including multiple resistance, have increased in Western countries,particularly in Spain, with resistance levels of up to 50% (11,20, 22, 31). A recent epidemiological study performed inthe United States has demonstrated that 25% of invasive pneumococciare non-penicillin susceptible (17). The emergence of high-levelresistance to penicillin, particularly in combination with otherresistance determinants, is a serious threat for current treatmentstrategies.

Several investigators have reported the international spread of multiply resistant pneumococcal clones. Soares and coworkershave reported the spread of a drug-resistant clone of serotype6B from Spain to Iceland in the late 1980s (37). This has resultedin an epidemic of this clone, which was isolated with frequenciesof up to 12% in 1992 (21). In 1991, Munoz and colleagues reportedevidence for the intercontinental spread of a multiply resistantclone of S. pneumoniae serotype 23F from Spain to the United States(24). This clone has subsequently disseminated through the UnitedStates (23). Finally, in 1995 Gasc and colleagues reported thespread of a multiply resistant pneumococcal clone of serogroup9 from Spain to France (10). The international clones 23F and9V have been identified in many countries in different parts ofthe world (14, 28). Besides the international spread of theclones 6B, 23F, and 9V, novel penicillin-resistant and multiplyresistant clones that tend to spread in an epidemic manner havebeen observed in the former Czechoslovakia, Spain, Japan, andSouth Africa (4, 30, 34, 42).

Penicillin resistance among pneumococcal isolates has rapidly emerged in Poland during the last decade. The percentage ofnon-penicillin-susceptible strains has increased from 0 to 3%in 1990 to 1993 (1, 19) to 14.3% in 1996 (39) and 14.4%in 1997 (38). In order to identify the nature of the increasein the prevalence of non-penicillin-susceptible pneumococci inPoland, a molecular epidemiological study was conducted. To thisend, strains were isolated in 1995 and 1996 from 37 patients whosuffered mainly from upper respiratory tract infections and pneumococcalpneumonia and who were diagnosed in 19 different clinical centerslocated in 16 towns across the country. The pneumococcal isolateswere characterized by BOX PCR typing, restriction fragment endlabeling (RFEL) analysis, penicillin-binding protein (PBP) genotyping,serotyping, and drug susceptibilitytesting.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial isolates. Non-penicillin-susceptible S. pneumoniae strains were isolated from 37 Polish patients in 1995 and 1996. A single pneumococcalisolate per patient per infection was analyzed. Bacteriologicaldiagnosis was carried out in 19 distinct medical centers. Thesecenters were located in 16 Polish towns across the country (Fig.1). The clinical, bacteriological, and demographic parametersare listed in Table 1.

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FIG. 1. Map of Poland. The medical centers collaborating in this study are as follows: 1, Mother and Child Institute, Warsaw; 2, Health Care Center Praga-Polnoc, Warsaw; 3, Nieklanska Street Hospital, Warsaw; 4, Sienna Street Hospital, Warsaw; 5, Health Care Center, Kolobrzeg; 6, Regional Hospital, Gdansk; 7, Health Care Center, Tczew; 8, Health Care Center, Braniewo; 9, Regional Children's Hospital Olsztyn; 10, Regional Hospital, Suwalki; 11, Medical University, Bydgoszcz; 12, Health Care Center, Gorzow Wielkopolski; 13, Health Care Center, Czestochowa; 14, Health Care Center, Kedzierzyn Kozle; 15, Jan Bober Center for Microbiology and Autovaccines, Krakow; 16, Health Care Center, Myslenice; 17, Health Care Center, Mielec; 18, Health Care Center, Sanok; and 19, Regional Hospital, Lomza.

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TABLE 1. Microbiological parameters of 37 penicillin-resistant pneumococcal isolates and clinical and demographic data for the patients

Biochemical characterization, serotyping, and susceptibility testing. The isolates were determined to be S. pneumoniae by investigating their optochin susceptibility and bile solubility (25).All pneumococci were serotyped in the Sera and Vaccines CentralResearch Laboratory in Warsaw on the basis of capsular swelling(Quellung reaction) observed microscopically after suspensionin antisera prepared at Statens Seruminstitut, Copenhagen, Denmark(8).

The susceptibilities of pneumococcal strains were determined in the Sera and Vaccines Central Research Laboratory in Warsawaccording to the guidelines of the National Committee for ClinicalLaboratory Standards (26) by the broth microdilution methodin cation-adjusted Mueller-Hinton II broth (Beckton Dickinson,Oxford, United Kingdom) supplemented with 5% lysed horse blood.The following panel of antimicrobial agents was tested: penicillin(Polfa, Poznan, Poland), amoxicillin (SmithKline Beecham, Brentford,United Kingdom), cefotaxime (Roussel, Paris, France), doxycycline(Polfa), chloramphenicol (Polfa), erythromycin (Polfa), lincomycin(Upjohn, Kalamazoo, Mich.), vancomycin (Eli Lilly, Indianapolis,Ind.), rifampin (Polfa), ofloxacin (Hoechst-Roussel, Kansas City,Kans.), sparfloxacin (Rhone-Poulenc, Courbevoie cedex, France),and co-trimoxazole (trimethoprim with sulfamethoxazole) (Polfa).For doxycycline, lincomycin, and sparfloxacin susceptibility testing,French interpretative criteria were applied (6). The microdilutionpanels were prepared by a single senior technician. The qualitycontrol strains S. pneumoniae ATCC 49619 and Staphylococcus aureusATCC 29213 were included in eachrun.

RFEL analysis and BOX PCR typing. Typing of pneumococcal strains by RFEL analysis was performed as described by Van Steenbergen et al. (41) and adapted byHermans et al. (16). Briefly, purified pneumococcal DNA wasdigested with the restriction enzyme EcoRI. The DNA restrictionfragments were end labeled at 72°C with [ $alpha$ -³²P]dATP by using DNA polymerase (Goldstar; Eurogentec, Seraing,Belgium). The radiolabeled fragments were denatured and separatedelectrophoretically on a 6% polyacrylamide sequencing gel containing8 M urea. Subsequently, the gel was transferred onto filter paper,vacuum dried (HBI, Saddlebrook, N.Y.), and exposed for variablelengths of time at room temperature to ECL Hyperfilms (Amersham,Bucks, UnitedKingdom).

BOX PCR typing was carried out in a single laboratory as described before (40). Briefly, 50 ng of pneumococcal DNA was amplifiedby PCR (4 min at 94°C [predenaturation]; 40 cycles of 1 min at94°C, 1 min at 60°C, and 2 min at 74°C; and 2 min at 74°C [extension]),using primer BOX-A (5'ATACTCTTCGAAAATCTCTTCAAAC), which was designedfrom the primary structure of the BOX repeat motif. The amplifiedproducts were separated on a 1.5% agarose gel. Gels were stainedwith ethidium bromide, after which the banding patterns were evaluatedvisually. BOX PCR patterns showing a single band difference weredefined as nonidentical types (e.g., 1, 2, and 3). Identical bandingpatterns varying in the intensity of one or more bands were definedas subtypes (e.g., 7, 7.1, and 7.2).

PBP genotyping. Genetic polymorphism of the penicillin resistance genes pbp1a, pbp2b, and pbp2x was investigated by restriction fragment lengthpolymorphism (RFLP) analysis. To this end, we amplified the genesby PCR and analyzed the digested DNA products by agarose gel electrophoresis.PCR amplification of the PBP-encoding genes was performed in a50-µl PCR buffer system containing 75 mM Tris-HCl (pH 9.0), 20mM (NH₄)₂SO₄, 0.01% (wt/vol) Tween 20, 1.5 mM MgCl₂, 0.2 mM deoxynucleosidetriphosphates, 10 pmol of the individual primers, 0.5 U of DNApolymerase (Eurogentec), and 10 ng of purified chromosomal DNA.Cycling was performed in a PTC-100 Programmable Thermal Controller(MJ Research, Watertown, Mass.) and consisted of the followingsteps: predenaturation at 94°C for 1 min; 30 cycles of 1 min at94°C, 1 min at 52°C, and 2 min at 72°C; and a final extensionat 72°C for 3 min. The primers used to amplify the genes pbp1a,pbp2b, and pbp2x were described previously (5, 7, 24).

The amplification products (5 µl) were digested with the restriction endonuclease HinfI and separated by electrophoresis in2.5% agarose gels containing 0.5× Tris-borate-EDTA and 0.1 µgof ethidium bromide per ml (5 mm thick) (Agarose MP; BoehringerMannheim, Almere, The Netherlands). Gels were run in 0.5× Tris-borate-EDTAcontaining 0.1 µg of ethidium bromide per ml at 20 mA for 4 h.Prior to electrophoresis, samples were mixed with a 5×-concentratedlayer mix consisting of 50% glycerol in water and 0.8 mg of bromophenolblue per ml. Gels were photographed with a Polaroid MP4 Landcameraand Polaroid 667 films. The different PBP genotypes are representedby a three-number code (e.g., 6-14-43, referring to the RFLP patternsof the genes pbp1a [pattern 6], pbp2b [pattern 14], and pbp2x[pattern 43],respectively.

Computer-assisted analysis of the DNA banding patterns. The RFEL types were analyzed by using the Windows version of the Gelcompar software version 4 (Applied Maths, Kortrijk, Belgium)after imaging the RFEL autoradiograms with the Image Master DTS(Pharmacia Biotech, Uppsala, Sweden). To this end, the DNA fragmentsin the molecular size range of 160 to 400 bp were explored. TheDNA banding patterns were normalized by using pneumococcus-specificbands present in the RFEL banding patterns of all strains. Comparisonof the banding patterns was performed by the unweighted pair groupmethod with arithmetic averages (29) and with the Jaccard similaritycoefficient applied to peaks (36). Computer-assisted analysisand the methods and algorithms used in this study were accordingto the instructions of the manufacturer of Gelcompar. A toleranceof 1.5% in band positions was applied during comparison of theDNA patterns. Identical DNA types were arbitrarily defined asthose with RFEL homologies higher than 95%. Cluster codes I toIV refer to clusters of pneumococcal strains displaying RFEL typeswith homologies higher than 80% that were confirmed to be geneticallyrelated by using BOX PCR typing (identical BOX PCR types orsubtypes).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

The molecular epidemiology of non-penicillin-susceptible multidrug-resistant pneumococci in Poland was investigated. Thirty-sevenpatients who suffered mainly from upper and lower respiratorytract infections (n = 20 and 13, respectively) were enrolled inthis study. In addition, three patients suffered from otitis media,a brain abscess, and conjunctivitis, respectively. The clinicaldiagnosis of one patient was unknown. The medical centers to whichthe patients were referred were located in 16 Polish towns acrossthe country (Fig. 1). The clinical and demographic parametersare listed in Table 1.

The 37 non-penicillin-susceptible pneumococcal strains were characterized by RFEL analysis and BOX PCR typing. RFEL analysisdivided the 37 pneumococcal strains into 16 distinct types (Fig.2; Table 1). Eight distinct BOX PCR types were observed, representing14 subtypes (Fig. 3; Table 1). When RFEL and BOX PCR analyseswere combined, four genetically distinct clusters of strains (designatedI, II, III, and IV) were identified. Within these clusters, geneticrelatedness of the strains was demonstrated by both RFEL analysisand BOX PCR (sub)typing. Clusters I, II, III, and IV consistedof 12, 3, 11, and 7 strains, respectively. Each cluster was representedby strains that originated from different centers (Table 1).The remaining four strains did not fulfill the cluster criteria.

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FIG. 2. Genetic relatedness of 37 Polish non-penicillin-susceptible pneumococcal strains based on the RFEL banding patterns of the isolates. The RFEL fingerprints, their relatedness (dendrogram), strain numbers, and genetic cluster codes (Roman numerals) are depicted. Cluster codes I to IV refer to clusters of pneumococcal strains displaying RFEL types with homologies higher than 80% that are confirmed to be genetically related by BOX PCR typing (identical BOX PCR types or subtypes).

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FIG. 3. DNA fingerprint patterns of the 14 distinct BOX PCR (sub)types represented by the 37 Polish non-penicillin-susceptible pneumococcal strains. Lane numbers indicate BOX PCR type codes. Numbers at the left indicate the sizes of standard DNA fragments in base pairs.

Comparison of the Polish RFEL types with 133 genotypes present in the international RFEL data library representing 15 othercountries (13, 14) revealed that the genetic clusters II andIV matched the Spanish pandemic clone 23F (RFEL type 15) and theSpanish-French international clone 9V (RFEL type 23), respectively(data not shown). The remaining 14 Polish RFEL types did not matchany of the 133 non-Polish types present in the internationallibrary.

The 37 non-penicillin-susceptible pneumococci from Poland represented seven distinct serotypes (Table 1). The most predominantserotypes were 23F (n = 15), 6B (n = 12), and 9V (n = 6). Serotypes6A, 14, and 19A were all observed once in the Polish collection.Strain 31 displayed a rough phenotype and could not be serotyped.Serotypes 23F, 6B, and 9V included 6, 5, and 2 RFEL types, respectively,whereas the remaining three serotypes (6A, 14, and 19A) were restrictedto single RFEL types. The clusters I, II (pandemic clone 23F),and III displayed the serotypes 23F, 23F, and 6B, respectively.Genetic cluster IV (pandemic clone 9V) harbored both serotypes9V (n = 6) and 14 (n = 1), indicating horizontal transfer of capsulargenes within thiscluster.

The penicillin MICs of the pneumococcal strains varied from 0.12 to 8.0 µg/ml. Within the genetic clusters, various resistanceprofiles were observed, ranging from lack of susceptibility topenicillin and doxycycline only to multidrug resistance againstpenicillins, cefotaxime, co-trimoxazole, doxycycline, chloramphenicol,erythromycin, and lincomycin. Genetic cluster I had the highestpenicillin MICs (up to 8 µg/ml), as well as the greatest multidrugresistance (Table 1). The lowest penicillin MICs were observedfor isolates of genetic cluster III. The resistance patterns ofthese strains demonstrated their relative susceptibilities tothe antimicrobial agents tested. Nevertheless, all members ofcluster III were multidrug resistant, i.e., resistant to threeor more antibiotics. None of the isolates were resistant to vancomycin,rifampin, andfluoroquinolones.

The penicillin resistance profiles of the pneumococcal strains were investigated in further detail by PBP genotyping. To thisend, the penicillin resistance genes pbp1a, pbp2b, and pbp2x weresubjected to RFLP analysis (Fig. 4). The genetic clusters II (pandemicclone 23F) and IV (pandemic clone 9V) included two and three distinctPBP genotypes, respectively (Table 1). The polymorphism was restrictedto pbp2b. Similar results were observed for cluster III: therewere two distinct PBP genotypes that differed only in the pbp2bgene. For cluster I, seven distinct PBP genotypes were observed;in contrast to the case for the other three genetic clusters,genetic polymorphism was demonstrated in pbp1a (two types), pbp2b(five types), and pbp2x (four types). Except for clusters II andIV, representing pandemic clones 23F and 9V, respectively, nooverlap was observed between the PBP genotypes of the four clusters.Similarly, the four genotypes that were observed only once inthe Polish collection also displayed unique PBP genotypes. Thepolymorphism of the PBP-encoding genes within clusters II andIV was remarkable, as the majority of the pandemic 23F and 9Visolates that are now present in the international data library(51 23F strains from 10 countries [96%] and 31 9V strains from5 countries [97%]) display PBP genotype 1-1-1 (13, 14).

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FIG. 4. DNA fingerprint patterns of the pbp1a (n = 5), pbp2b (n = 7), and pbp2x (n = 8) genotypes represented by the 37 Polish non-penicillin-susceptible pneumococcal strains. Lane numbers indicate PBP genotype codes. Numbers at the left indicate the sizes of standard DNA fragments in base pairs.

Comparison of the PBP genotypes of the individual genes pbp1a, pbp2b, and pbp2x between the Polish non-penicillin-susceptiblestrains and 185 Dutch penicillin-susceptible pneumococcal meningitisisolates (15, 32) revealed the exclusive presence of penicillin-susceptiblepbp1a and pbp2b genotypes among the Polish clusters I, III, andIV. Two strains of cluster IV (pandemic clone 9V; strains 37 and38 with penicillin MICs of 0.5 and 1.0 µg/ml, respectively) displayedthe predominant penicillin-susceptible pbp2b genotype 2 (Fig.4; Table 1). In addition, the majority of the strains belongingto cluster III displayed the predominant penicillin-susceptiblepbp1a-pbp2b genotype 2-2 (penicillin MIC of 0.12 µg/ml). Finally,the majority of cluster I displayed the penicillin-susceptiblepbp1a genotype 6 (penicillin MICs ranging from 2.0 to 8.0 µg/ml);this genotype was observed only once in the collection of 185Dutch penicillin-susceptiblepneumococci.

Among the pbp1a, pbp2b, and pbp2x genotypes that are restricted to non-penicillin-susceptible pneumococci (13, 14), thepresence of pbp1a genotype 1 was observed among clusters II (clone23F) and IV (clone 9V) (Table 1). In addition, the pbp2b genotypes1 and 18 and the pbp2x genotype 1 were observed in three geneticclusters. These data indicate horizontal exchange of penicillinresistance genes between pneumococcal strains of the differentPolishclusters.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Penicillin resistance among pneumococcal isolates has rapidly emerged in Poland during the last decade. The percentage ofnon-penicillin-susceptible strains has increased from 0 to 3%in 1990 to 1993 (1, 19) to 14.3% in 1996 (39) and 14.4%in 1997 (38). In order to identify the nature of the increasein the prevalence of non-penicillin-susceptible pneumococci inPoland, a molecular epidemiological study was conducted. The emergenceof four genetically distinct non-penicillin-susceptible multidrug-resistantpneumococcal clusters was clearly demonstrated. Clusters II andIV represented the genetic clones 23F (24) and 9V (11), respectively,which have recently emerged all over the world (13, 14). Inaddition, the two other clusters, I and III, predominated in thecollection of non-penicillin-susceptible pneumococci from Poland.Since these clusters did not match any of the 133 RFEL types ofnon-penicillin-susceptible pneumococci collected in 15 other countriesand present in the international data library of RFEL types (13,14), their Polish origin is mostlikely.

Various researchers have reported horizontal transfer of capsular genes (2, 13-15). The high frequency of capsular transfermay have consequences for the outcome of current vaccine strategies,which focus on the use of a restricted number of distinct capsularpolysaccharides. The use of multivalent conjugate vaccines mayshift the capsular distribution towards capsular types that arenot present in these vaccines. Such a shift might be enhancedby the frequent horizontal exchange of capsular genes. Geneticcluster IV (pandemic clone 9V) harbored both serotypes 9V (n =6) and 14 (n = 1). These serotypes are known to occur in thisinternational clone (13, 14). The Polish strains that weregenetically related to the pandemic clone 23F (cluster II), whichharbors serotypes 23F, 19F, 14, 9N, 19A, and 3 (13, 14, 27),displayed only the ancestral serotype23F.

Within the four genetic clusters, RFLP of the PBP-encoding genes was often observed, in particular in pbp2b. This findingindicates frequent horizontal transfer of the penicillin resistancegenes. PBP genotype 1-1-1 was observed in clusters II (pandemicclone 23F) and IV (pandemic clone 9V). In a recent study by Hermansand coworkers (13), the vast majority of isolates of the pandemicclones 23F and 9V also displayed the PBP genotype 1-1-1. In thatstudy, PBP genotype 1-1-1 was displayed by 41% of the strainscollected in 15 other countries and represented 20 of the 133distinct RFEL types. In addition, genetic polymorphism in thepenicillin resistance genes of the pandemic clones 9V and 23Fwas rarely observed. However, in 5 of the 10 Polish strains thatwere related to the pandemic clones 9V and 23F, differences inthe PBP genotypes were observed, suggesting that in Poland horizontaltransfer of penicillin resistance genes, in particular pbp2b,occurs more frequently in these clones than in those present inthe other countries. The pbp2b genotypes 18 (observed only inPoland so far) and 1 and the pbp2x genotype 1 were observed inthree of the four genetic clusters. These data suggest that thesePBP genotypes have spread in the Polish population of non-penicillin-susceptiblepneumococci by horizontal genetransfer.

The strains belonging to cluster III invariably displayed low penicillin MICs of 0.12 µg/ml. In addition, the majority ofthese strains displayed the penicillin-susceptible pbp1a-pbp2bgenotype 2-2. Although the predictive value of PBP genotypingfor pneumococcal penicillin resistance can be debated for methodologicalreasons, this observation is in concordance with data from Smithand coworkers (35), who have demonstrated that in pneumococciwith low penicillin MICs, pbp2b is usually not affected bymutations.

In summary, penicillin resistance has rapidly emerged in Poland over the last decade. Although the pandemic clones 9V and23F are present in this country, the nationwide emergence of twonovel multidrug-resistant pneumococcal clones that are presumablyof Polish origin has clearly contributed to the increase in theprevalence of non-penicillin-susceptible pneumococci inPoland.

	ACKNOWLEDGMENTS

We thank Melanie Srodzinski and Daniëlle van Nispen for technicalassistance.

This study was sponsored by grants from the Sophia Foundation for Medical Research, Rotterdam, The Netherlands (to K.O.) andfrom the Polish Committee of Scientific Studies, Warsaw, Poland(Microbank Project) (to K.T. and W.H.).

P.W.M.H. and K.T. contributed equally to thisstudy.

	FOOTNOTES

^* Corresponding author. Mailing address: Laboratory of Pediatrics/Room Ee1500, Erasmus University Rotterdam, P.O. Box 1738,3000 DR Rotterdam, The Netherlands. Phone: 31-10-4088224. Fax:31-10-4089486. E-mail: hermans{at}kgk.fgg.eur.nl.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

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22. Lister, P. D. 1995. Multiply-resistant pneumococcus: therapeutic problems in the management of serious infection. Eur. J. Clin. Microbiol. Infect. Dis. 4(Suppl.):18-25.

23. McDougal, L. K., R. R. Facklam, M. Reeves, S. Hunter, J. M. Swenson, B. C. Hill, and F. C. Tenover. 1992. Analysis of multiply antimicrobial-resistant isolates of Streptococcus pneumoniae from the United States. Antimicrob. Agents Chemother. 36:2176-2184[Abstract/Free Full Text].

24. Munoz, R., T. R. Coffey, M. Daniels, C. G. Dowson, G. Laible, J. Casal, R. Hakenbeck, M. Jacobs, J. M. Musser, B. G. Spratt, and A. Tomasz. 1991. Intercontinental spread of a multiresistant clone of serotype 23F Streptococcus pneumoniae. J. Infect. Dis. 164:302-306[Medline].

25. Murray, P. R., E. J. Baron, M. A. Pfaller, F. C. Tenover, and R. H. Yolken (ed.). 1995. Manual of clinical microbiology, 6th ed. American Society for Microbiology, Washington, D.C.

26. National Committee for Clinical Laboratory Standards. 1997. Methods for dilution antimicrobial susceptibility tests for bacteria that grow aerobically, 4th ed. Approved standard M7-A4. National Committee for Clinical Laboratory Standards, Wayne, Pa.

27. Nesin, M., M. Ramirez, and A. Tomasz. 1998. Capsular transformation of a multidrug-resistant Streptococcus pneumoniae in vivo. J. Infect. Dis. 177:707-713[Medline].

28. Reichmann, P., E. Varon, E. Günther, R. R. Reinert, R. Lüttiken, A. Marton, P. Geslin, J. Wagner, and R. Hakenbeck. 1995. Penicillin-resistant Streptococcus pneumoniae in Germany: genetic relationship to clones from other European countries. J. Med. Microbiol. 43:377-385[Abstract/Free Full Text].

29. Romesburg, H. C. 1990. Cluster analysis for researchers, p. 9-28. Krieger, Malabar, Fla.

30. Sa Figueiredo, A. M., R. Austrian, P. Urbaskova, L. A. Teixeira, and A. Tomasz. 1995. Novel penicillin-resistant clones of Streptococcus pneumoniae in the Czech Republic and in Slovakia. Microb. Drug Resist. 1:71-78. [Medline]

31. Schreiber, J., and M. Jacobs. 1995. Antibiotic-resistant pneumococci. Pediatr. Clin. N. Am. 42:519-537[Medline].

32. Sluijter, M. Unpublished observations.

33. Sluijter, M., H. Faden, R. de Groot, N. Lemmens, W. H. F. Goessens, A. van Belkum, and P. W. M. Hermans. 1998. Molecular characterization of pneumococcal nasopharynx isolates in children during the first two years of life. J. Clin. Microbiol. 36:2248-2253[Abstract/Free Full Text].

34. Smith, A. M., and K. P. Klugman. 1997. Three predominant clones identified within penicillin-resistant South-African isolates of Streptococcus pneumoniae. Microb. Drug Resist. 3:385-389. [Medline]

35. Smith, A. M., K. P. Klugman, T. J. Coffey, and B. G. Spratt. 1993. Genetic diversity of penicillin-binding protein 2B and 2X genes from Streptococcus pneumoniae in South Africa. Antimicrob. Agents Chemother. 37:1938-1944[Abstract/Free Full Text].

36. Sneath, P. H. A., and R. R. Sokal. Numerical taxonomy, p. 131-132. Freeman, San Francisco, Calif.

37. Soares, S., K. G. Kristinsson, J. M. Musser, and A. Tomasz. 1993. Evidence for the introduction of a multiresistant clone of serotype 6B Streptococcus pneumoniae from Spain to Iceland in the late 1980s. J. Infect. Dis. 168:158-163[Medline].

38. Trzcinski, K. Unpublished observations.

39. Trzcinski, K., and W. Hryniewicz. 1997. Antimicrobial susceptibility of common bacterial pathogens isolated from lower respiratory tract infections in Poland in 1996 $---$ The Alexander Project. Med. Sci. Monitor 3:714-722.

40. Van Belkum, A., M. Sluijter, R. de Groot, H. A. Verbrugh, and P. W. M. Hermans. 1996. A novel BOX-repeat PCR assay for high-resolution typing of Streptococcus pneumoniae strains. J. Clin. Microbiol. 34:1176-1179[Abstract].

41. Van Steenbergen, T. J. M., S. D. Colloms, P. W. M. Hermans, J. de Graaff, and R. H. A. Plasterk. 1995. Genomic DNA fingerprinting by restriction fragment end labeling (RFEL). Proc. Natl. Acad. Sci. USA 92:5572-5576[Abstract/Free Full Text].

42. Yoshida, R., Y. Hirakata, M. Kaku, H. Takemura, H. Tanaka, K. Tomono, H. Koga, S. Kohno, and S. Kamahira. 1997. Genetic relationship of penicillin resistant Streptococcus pneumoniae serotype 19B strains in Japan. Epidemiol. Infect. 118:105-110[Medline].

43. Zenni, M. K., S. H. Cheatham, J. M. Thompson, G. W. Reed, A. B. Batson, P. S. Palmer, K. L. Holland, and K. M. Edwards. 1995. Streptococcus pneumoniae colonization in the young child: association with otitis media and resistance to penicillin. J. Pediatr. 127:533-537[Medline].

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20.	Klugman, K. P. 1990. Pneumococcal resistance to antibiotics. Clin. Microbiol. Rev. 3:171-196[Abstract/Free Full Text].
21.	Kristinsson, K. G., M. A. Hjalmarsdottir, and O. Steingrimsson. 1992. Increasing penicillin resistance in pneumococci in Iceland. Lancet 339:1606-1607[Medline].
22.	Lister, P. D. 1995. Multiply-resistant pneumococcus: therapeutic problems in the management of serious infection. Eur. J. Clin. Microbiol. Infect. Dis. 4(Suppl.):18-25.
23.	McDougal, L. K., R. R. Facklam, M. Reeves, S. Hunter, J. M. Swenson, B. C. Hill, and F. C. Tenover. 1992. Analysis of multiply antimicrobial-resistant isolates of Streptococcus pneumoniae from the United States. Antimicrob. Agents Chemother. 36:2176-2184[Abstract/Free Full Text].
24.	Munoz, R., T. R. Coffey, M. Daniels, C. G. Dowson, G. Laible, J. Casal, R. Hakenbeck, M. Jacobs, J. M. Musser, B. G. Spratt, and A. Tomasz. 1991. Intercontinental spread of a multiresistant clone of serotype 23F Streptococcus pneumoniae. J. Infect. Dis. 164:302-306[Medline].
25.	Murray, P. R., E. J. Baron, M. A. Pfaller, F. C. Tenover, and R. H. Yolken (ed.). 1995. Manual of clinical microbiology, 6th ed. American Society for Microbiology, Washington, D.C.
26.	National Committee for Clinical Laboratory Standards. 1997. Methods for dilution antimicrobial susceptibility tests for bacteria that grow aerobically, 4th ed. Approved standard M7-A4. National Committee for Clinical Laboratory Standards, Wayne, Pa.
27.	Nesin, M., M. Ramirez, and A. Tomasz. 1998. Capsular transformation of a multidrug-resistant Streptococcus pneumoniae in vivo. J. Infect. Dis. 177:707-713[Medline].
28.	Reichmann, P., E. Varon, E. Günther, R. R. Reinert, R. Lüttiken, A. Marton, P. Geslin, J. Wagner, and R. Hakenbeck. 1995. Penicillin-resistant Streptococcus pneumoniae in Germany: genetic relationship to clones from other European countries. J. Med. Microbiol. 43:377-385[Abstract/Free Full Text].
29.	Romesburg, H. C. 1990. Cluster analysis for researchers, p. 9-28. Krieger, Malabar, Fla.
30.	Sa Figueiredo, A. M., R. Austrian, P. Urbaskova, L. A. Teixeira, and A. Tomasz. 1995. Novel penicillin-resistant clones of Streptococcus pneumoniae in the Czech Republic and in Slovakia. Microb. Drug Resist. 1:71-78. [Medline]
31.	Schreiber, J., and M. Jacobs. 1995. Antibiotic-resistant pneumococci. Pediatr. Clin. N. Am. 42:519-537[Medline].
32.	Sluijter, M. Unpublished observations.
33.	Sluijter, M., H. Faden, R. de Groot, N. Lemmens, W. H. F. Goessens, A. van Belkum, and P. W. M. Hermans. 1998. Molecular characterization of pneumococcal nasopharynx isolates in children during the first two years of life. J. Clin. Microbiol. 36:2248-2253[Abstract/Free Full Text].
34.	Smith, A. M., and K. P. Klugman. 1997. Three predominant clones identified within penicillin-resistant South-African isolates of Streptococcus pneumoniae. Microb. Drug Resist. 3:385-389. [Medline]
35.	Smith, A. M., K. P. Klugman, T. J. Coffey, and B. G. Spratt. 1993. Genetic diversity of penicillin-binding protein 2B and 2X genes from Streptococcus pneumoniae in South Africa. Antimicrob. Agents Chemother. 37:1938-1944[Abstract/Free Full Text].
36.	Sneath, P. H. A., and R. R. Sokal. Numerical taxonomy, p. 131-132. Freeman, San Francisco, Calif.
37.	Soares, S., K. G. Kristinsson, J. M. Musser, and A. Tomasz. 1993. Evidence for the introduction of a multiresistant clone of serotype 6B Streptococcus pneumoniae from Spain to Iceland in the late 1980s. J. Infect. Dis. 168:158-163[Medline].
38.	Trzcinski, K. Unpublished observations.
39.	Trzcinski, K., and W. Hryniewicz. 1997. Antimicrobial susceptibility of common bacterial pathogens isolated from lower respiratory tract infections in Poland in 1996 $---$ The Alexander Project. Med. Sci. Monitor 3:714-722.
40.	Van Belkum, A., M. Sluijter, R. de Groot, H. A. Verbrugh, and P. W. M. Hermans. 1996. A novel BOX-repeat PCR assay for high-resolution typing of Streptococcus pneumoniae strains. J. Clin. Microbiol. 34:1176-1179[Abstract].
41.	Van Steenbergen, T. J. M., S. D. Colloms, P. W. M. Hermans, J. de Graaff, and R. H. A. Plasterk. 1995. Genomic DNA fingerprinting by restriction fragment end labeling (RFEL). Proc. Natl. Acad. Sci. USA 92:5572-5576[Abstract/Free Full Text].
42.	Yoshida, R., Y. Hirakata, M. Kaku, H. Takemura, H. Tanaka, K. Tomono, H. Koga, S. Kohno, and S. Kamahira. 1997. Genetic relationship of penicillin resistant Streptococcus pneumoniae serotype 19B strains in Japan. Epidemiol. Infect. 118:105-110[Medline].
43.	Zenni, M. K., S. H. Cheatham, J. M. Thompson, G. W. Reed, A. B. Batson, P. S. Palmer, K. L. Holland, and K. M. Edwards. 1995. Streptococcus pneumoniae colonization in the young child: association with otitis media and resistance to penicillin. J. Pediatr. 127:533-537[Medline].