Methicillin-resistant Staphylococcus aureus Clones, Western Australia.Community-associated methicillin-resistant Staphylococcus aureus methicillin-resistant Staphylococcus aureus Methicillin-aminoglycoside resistant Staphylococcus aureus, MRSA An organism with multiple antibiotic resistances–eg, aminoglycosides, chloramphenicol, clindamycin, erythromycin, rifampin, tetracycline, (MRSA MRSA Methicillin-resistant Staphylococcus aureus. See MARSA. ) was first reported in Western Australia Western Australia, state (1991 pop. 1,409,965), 975,920 sq mi (2,527,633 sq km), Australia, comprising the entire western part of the continent. It is bounded on the N, W, and S by the Indian Ocean. Perth is the capital. in the early 1990s from indigenous peoples The term indigenous peoples has no universal, standard or fixed definition, but can be used about any ethnic group who inhabit the geographic region with which they have the earliest historical connection. living in remote areas. Although a statewide policy of screening all hospital patients and staff who have lived outside the state for MRSA has prevented the establishment of multidrug-resistant epidemic MRSA, the policy has not prevented SCCmec type IV and type V MRSA clones from becoming established. Of the 4,099 MRSA isolates analyzed (referred to the Gram-positive Bacteria Typing and Research Unit) from July 2003 to December 2004, 77.5% were community-associated MRSA (CA-MRSA CA-MRSA Community Acquired Methicillin-Resistant Staphylococcus Aureus ). Using multilocus sequence/staphylococcal chromosome cassette mec typing, 22 CA-MRSA clones were characterized. Of these isolates, 55.5% were resistant to [greater than or equal to]1 non-[beta]-lactam antimicrobial drug. Five Panton-Valentine leukocidin Panton-Valentine leukocidin a nonhemolytic toxin produced by Staphylococcus aureus which kills segmented neutrophils and macrophages. (PVL PVL Periventricular Leukomalacia PVL Prevail PVL Parameter Value Language PVL Pade Via Lanczos (circuit modeling) PVL Physical Volume Library PVL Pascack Valley Line (New Jersey Transit commuter rail line) )-positive CA-MRSA clones were identified. The emergence of multidrug-resistant CA-MRSA clones and the detection of PVL toxin genes in clones previously reported as PVL negative is a major public health concern. ********** Staphylococcus aureus Staphylococcus au·re·us n. A bacterium that causes furunculosis, pyemia, osteomyelitis, suppuration of wounds, and food poisoning. Staphylococcus aureus Staphylococcus pyogenes successfully colonizes humans, contaminates the hospital environment, and has the genetic versatility to acquire resistance to multiple antimicrobial agents Antimicrobial agents Chemical compounds biosynthetically or synthetically produced which either destroy or usefully suppress the growth or metabolism of a variety of microscopic or submicroscopic forms of life. . Methicillin-resistant S. aureus The aureus (pl. aurei) was a gold coin of ancient Rome valued at 25 silver denarii. The aureus was regularly issued from the 1st century BC to the beginning of the 4th century AD, when it was replaced by the solidus. (MRSA) was first detected soon after the introduction of methicillin methicillin /meth·i·cil·lin/ (meth?i-sil´in) a semisynthetic penicillin highly resistant to inactivation by penicillinase; used as the sodium salt. meth·i·cil·lin n. in 1960, and isolation rates increased until the early 1970s (1). These earlier "classic" MRSA strains were genetically similar to each other and may have evolved from a single clone (2). In 1976, the first outbreak of gentamicin-resistant MRSA in Australia (3) was reported, and by 1981 extensive outbreaks occurred in several countries. In 1985, it became evident that these "modern" strains of MRSA carried epidemic potential not possessed NOT POSSESSED. A plea sometimes used in actions of trover, when the defendant was not possessed of the goods at the commencement of the action. 3 Mann. & Gr. 101, 103. by MRSA isolated in the 1960s and early 1970s and that they were genetically different from the earlier classic MRSA (4). Since 1990, international and intercontinental spread of MRSA (known as epidemic MRSA or EMRSA) has increased. In 2002, Enright et al., using multilocus sequence typing Multilocus sequence typing (MLST) is a technique in molecular biology for the typing of multiple loci. The procedure characterizes isolates of bacterial species using the DNA sequences of internal fragments of multiple (usually seven) housekeeping genes. (MLST MLST Multi Locus Sequence Typing MLST Medical Logistics Support Team MLST Mini Losi Super Truck (1/18th scale radio control vehicle) ) combined with staphylococcal staphylococcal pertaining to Staphylococcus spp. staphylococcal clumping test used as a means of measuring the quantity of fibrinogen-split products in a sample of blood. chromosome cassette mec (SCCmec) typing, established that relatively few major EMRSA clones existed (5). These clones emerged either as descendants of preexisting pre·ex·ist or pre-ex·ist v. pre·ex·ist·ed, pre·ex·ist·ing, pre·ex·ists v.tr. To exist before (something); precede: Dinosaurs preexisted humans. v.intr. EMRSA clones or by horizontal transfer of the mec determinants into methicillin-susceptible S. aureus. EMRSA became endemic in hospitals in eastern Australian states (New South Wales New South Wales, state (1991 pop. 5,164,549), 309,443 sq mi (801,457 sq km), SE Australia. It is bounded on the E by the Pacific Ocean. Sydney is the capital. The other principal urban centers are Newcastle, Wagga Wagga, Lismore, Wollongong, and Broken Hill. , Victoria, and Queensland) in the late 1980s and 1990s, with some spread to hospitals in South Australia South Australia, state (1991 pop. 1,236,623), 380,070 sq mi (984,381 sq km), S central Australia. It is bounded on the S by the Indian Ocean. Kangaroo Island and many smaller islands off the south coast are included in the state. , the Northern Territory, and Tasmania (6). However, a statewide MRSA policy, introduced in 1982, prevented these strains from becoming established in Western Australia (WA) hospitals. This policy required MRSA screening of anyone who had been hospitalized or had been a healthcare worker in a hospital outside of WA in the previous 12 months. MRSA-positive patients were isolated in the hospital, and staff with MRSA-positive test results received decolonization decolonization Process by which colonies become independent of the colonizing country. Decolonization was gradual and peaceful for some British colonies largely settled by expatriates but violent for others, where native rebellions were energized by nationalism. treatment. Imported MRSA still occasionally caused single-strain outbreaks in hospitals; however, infection control interventions contained them. In the early 1990s, nonmultidrug-resistant MRSA (nmMRSA) were observed in WA, initially from indigenous people in remote communities (7) but subsequently in Perth, the state capital. These strains became known as "WA-MRSA." Although WA-MRSA did not readily spread in WA hospitals, 1 strain was responsible for an outbreak of hospital-acquired infection (8). Strains of nmMRSA have recently been reported in the eastern Australian states, and studies in Queensland and New South Wales showed a strong association between community-acquired infection with nmMRSA and Polynesian ethnicity. Isolates causing these infections were indistinguishable by phage phage: see bacteriophage. phage - A program that modifies other programs or databases in unauthorised ways; especially one that propagates a virus or Trojan horse. See also worm, mockingbird. The analogy, of course, is with phage viruses in biology. typing and pulsed-field gel electrophoresis gel electrophoresis n. Electrophoresis performed in a gel composed of agarose, polyacrylamide, or starch. from those previously reported in New Zealand New Zealand (zē`lənd), island country (2005 est. pop. 4,035,000), 104,454 sq mi (270,534 sq km), in the S Pacific Ocean, over 1,000 mi (1,600 km) SE of Australia. The capital is Wellington; the largest city and leading port is Auckland. (9,10). Subsequently, a second strain (WAMRSA-7 or Qld MRSA) has been associated with community-acquired infections in Caucasians in Queensland (11). The emergence of nmMRSA has also been reported in other parts of the world, including North America North America, third largest continent (1990 est. pop. 365,000,000), c.9,400,000 sq mi (24,346,000 sq km), the northern of the two continents of the Western Hemisphere. (12) and Europe (13). Although nmMRSA strains appear to have originated in the community, they may include nmEMRSA strains that have been associated with healthcare facilities (e.g., EMRSA-15, EMRSA-16, and the New York/Japan EMRSA) or nonmultidrug-resistant sporadic hospital MRSA strains that have been taken into the community. In 1997, the Department of Health WA, in collaboration with the Department of Microbiology and Infectious Diseases infectious diseases: see communicable diseases. at Royal Perth Hospital Royal Perth Hospital (RPH) is an 855-bed teaching hospital located on north eastern edge of the CBD of Perth, Western Australia (). Royal Perth Hospital also has specialised rehabilitation facilities at Shenton Park. , PathWest Laboratory Medicine WA, and the School of Biomedical Sciences at Curtin University of Technology established the Gram-positive Bacteria Typing and Research Unit to assist in controlling MRSA in WA. Since then, all MRSA isolated in WA have been referred to the unit for epidemiologic typing. This study describes the different epidemic and CAMRSA clones isolated in WA and establishes their genetic relatedness. Materials and Methods MRSA Isolates All MRSA isolated in WA between July l, 2003, and December 31, 2004, were included in this study. Isolates were recovered from clinical and infection control screening specimens. For the purpose of this study, duplicate isolates from the same patient (as determined by their antimicrobial drug susceptibility phenotype) were excluded. Antimicrobial Susceptibility Testing A test for oxacillin oxacillin /ox·a·cil·lin/ (ok?sah-sil´in) a semisynthetic penicillinase-resistant penicillin used as the sodium salt in infections due to penicillin-resistant, gram-positive organisms. susceptibility was performed on Mueller-Hinton agar by the disk diffusion method according to according to prep. 1. As stated or indicated by; on the authority of: according to historians. 2. In keeping with: according to instructions. 3. Clinical Laboratory Standards Institute (CLSI CLSI Clinical and Laboratory Standards Institute (Wayne, PA) CLSI Cisco Link Services Interface ) recommendations by using a 1-[micro]g oxacillin disk (14). Oxacillin susceptibility results discrepant dis·crep·ant adj. Marked by discrepancy; disagreeing. [Middle English discrepaunt, from Latin discrep with those of the referring laboratory were confirmed by the detection of the mecA gene by polymerase chain reaction polymerase chain reaction (pŏl`ĭmərās') (PCR), laboratory process in which a particular DNA segment from a mixture of DNA chains is rapidly replicated, producing a large, readily analyzed sample of a piece of DNA; the process is (PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) ) (15). An antibiogram was performed on Mueller-Hinton agar by the disk diffusion method according to CLSI recommendations, against a panel of 8 antimicrobial drugs (14): erythromycin erythromycin (ĭrĭth'rōmī`sĭn), any of several related antibiotic drugs produced by bacteria of the genus Streptomyces (see antibiotic). (15 [micro]g), tetracycline tetracycline (tĕ'trəsī`klēn), any of a group of antibiotics produced by bacteria of the genus Streptomyces. They are effective against a wide range of Gram positive and Gram negative bacteria, interfering with protein (30 [micro]g), trimethoprim trimethoprim /tri·meth·o·prim/ (-meth´o-prim) an antibacterial closely related to pyrimethamine; almost always used in combination with a sulfonamide, primarily for the treatment of urinary tract infections. (5 [micro]g), ciprofloxacin ciprofloxacin /cip·ro·flox·a·cin/ (sip?ro-flok´sah-sin) a synthetic antibacterial effective against many gram-positive and gram-negative bacteria; used as the hydrochloride salt. cip·ro·flox·a·cin n. (5 [micro]g), gentamicin gentamicin /gen·ta·mi·cin/ (jen?tah-mi´sin) an aminoglycoside antibiotic complex isolated from bacteria of the genus Micromonospora, (10 [micro]g), rifampin rifampin (rĭfăm`pĭn), antibiotic used in the treatment of tuberculosis. It is also used to eliminate the meningococcus microorganism from carriers and to treat leprosy, or Hansen's disease. (5 [micro]g), fusidic acid fusidic acid a lipophilic steroid antibioitic, the product of Fusidium coccineum; mainly active against gram-positive bacteria. (10 [micro]g), and mupirocin (5 [micro]g). The French CA-SFM susceptibility testing interpretive criterion was used for fusidic acid (16), and the suggested interpretive criterion by Finlay et al. was used for mupirocin (17). CLSI interpretive criteria were used for the remaining antimicrobial drugs (18). MRSA that were resistant to [greater than or equal to] 3 of the 8 antimicrobial drugs listed were defined as mMRSA and those resistant to <3 drugs were defined as nmMRSA (8). Urease urease /ure·ase/ (u´re-as) an enzyme that catalyzes the hydrolysis of urea to ammonia and carbon dioxide; it is a nickel protein of microorganisms and plants that is used in clinical assays of plasma urea concentrations. production was performed by Christensen's urea slopes incubated for 24 h at 37[degrees]C. Typing Methods Resistogram typing was performed by disk diffusion against a panel of 6 chemicals and dyes: cadmium acetate (10 mmol/L), sodium arsenate ar·se·nate n. A salt of arsenic acid. arsenate an uncommon garden pesticide, as lead arsenate, or as antifungal spray on fruit trees or cattle tick dip as sodium arsenate. (0.2 [micro]mol/L), ethidium bromide Ethidium bromide (sometimes abbreviated as EtBr) is an intercalating agent commonly used as a nucleic acid stain in molecular biology laboratories for techniques such as agarose gel electrophoresis. (15 mmol/L), propamidine isethionate isethionate /is·eth·i·o·nate/ (i?se-thi´ah-nat) USAN contraction for 2-hydroxyethanesulfonate. isethionate USAN contraction for 2-hydroxyethanesulfonate. (2% [wt/vol]), mercuric chloride mercuric chloride or mercury (II) chloride, chemical compound, HgCl2, a white powder of colorless rhombohedral crystals, somewhat soluble in water. It is also called bichloride of mercury or corrosive sublimate. (0.4 [micro]mol/L), and phenylmercuric acetate (5 mmol/L) as previously described (19,20). Coagulase coagulase /co·ag·u·lase/ (-las) an antigenic substance of bacterial origin, produced by staphylococci, which may be causally related to thrombus formation. co·ag·u·lase n. gene restriction fragment length polymorphism restriction fragment length polymorphism n. Abbr. RFLP Intraspecies variations in the length of DNA fragments generated by the action of restriction enzymes and caused by mutations that alter the sites at which these enzymes act, changing (RFLP RFLP abbr. restriction fragment length polymorphism RFLP restriction fragment length polymorphism. RFLP ) typing was performed as previously described (21). Contour-clamped homogeneous electric field electrophoresis (CHEF) was performed as previously described with the CHEF DR III System (Bio-Rad Laboratories Pty Ltd PTY LTD Propriety Limited (company structure in Australia) , Regents Park, New South Wales Alternate uses: Regents Park (disambiguation) Regents Park is a western suburb of Sydney, in the state of New South Wales, Australia. Regents Park is located 22 kilometres west of the Sydney central business district, in the local government area of Auburn Council. ) (8). Chromosomal patterns were examined visually, scanned with a Fluor-S Multimager (Bio-Rad Laboratories), and digitally analyzed with Multi-Analyst/PC (Bio-Rad Laboratories). CHEF patterns were grouped according to the criteria of Tenover et al. (22) and using a dendrogram A dendrogram is a tree diagram frequently used to illustrate the arrangement of the clusters produced by a clustering algorithm (see cluster analysis). Dendrograms are often used in computational biology to illustrate the clustering of genes. similarity of >80% to assign strain relatedness. S. aureus NCTC NCTC National Conservation Training Center NCTC National Counterterrorism Center (9/11 Commission Report) NCTC National Cable Television Cooperative NCTC National Collection of Type Cultures (UK laboratory) 8325 was used as the size marker. Multilocus sequence typing (MLST) was performed as specified by Enright et al. (23) on randomly selected isolates within each pulsotype. To assign a sequence type (ST) the sequences obtained were compared with the sequences described on the MLST website (http:www. mist.net/). Using the MLST database, clones were subsequently grouped into clonal complexes (CC). SCCmec typing was performed by PCR by using previously published primers that identified the class of mec complex and type of cassette chromosome recombinase re·com·bi·nase n. An enzyme that catalyzes genetic recombination. recombinase a function of the recA protein in Escherichia coli (ccr) encoded on the element (24,25). The presence of the Panton-Valentine leukocidin (PVL) determinants were detected by PCR by using previously published primers (26) and confirmed by sequencing the products. Results A total of 4,099 MRSA isolates were studied. All isolates were initially grouped according to their antibiogram and urease production. Isolates within a group were then further characterized by using coagulase PCR-RFLP PCR-RFLP Polymerase Chain Reaction–Restriction Fragment Length Polymorphism and CHEF analysis. MLST/SCCmec typing and PVL detection were performed on randomly selected isolates within each pulsotype. Twenty-nine clones were identified, including 7 (22.5%) EMRSA clones and 22 (77.5%) CA-MRSA clones. EMRSA Clones Table 1 shows the 7 EMRSA clones identified: ST22-MRSA-IV (EMRSA-15), ST239-MRSA-III (Aus-2 and Aus-3 EMRSA), ST8-MRSA-[IV.sub.pediatric pediatric /pe·di·at·ric/ (pe?de-at´rik) pertaining to the health of children. pe·di·at·ric adj. Of or relating to pediatrics. ] (Irish-2 EMRSA), ST36-MRSA-II (EMRSA-16), ST5-MRSA-II (New York/Japan EMRSA), ST8-MRSA-[II.sub.variant] (Irish-1 EMRSA), and the classic MRSA clone ST250-MRSA-I. Only 3 EMRSA clones were typically multidrug-resistant: ST239-MRSA-III (resistant to tetracycline, erythromycin, trimethoprim, ciprofloxacin, and gentamicin), ST8-MRSA-[IV.sub.pediatric] (resistant to erythromycin, trimethoprim, and ciprofloxacin), and ST8-MRSA-[II.sub.variant] (resistant to tetracycline, erythromycin, trimethoprim, ciprofloxacin, gentamicin and mupirocin). Overall, 94.6% of EMRSA were identified either as ST22-MRSA-IV (78.1%), a urease-negative nmEMRSA clone (resistant to erythromycin and ciprofloxacin) or ST239-MRSA-III (16.5%). By using CHEF electrophoresis and resistogram typing, ST239-MRSA-III could be further classified into 2 subclones: Aus-2 EMRSA (susceptible to mercuric chloride and phenylmercuric acetate) and Aus-3 EMRSA (resistant to mercuric chloride and phenylmercuric acetate). CA-MRSA Of the 22 identified clones of CA-MRSA, 21 were WAMRSA and 1 was Western Samoan phage pattern (WSPP WSPP Work Group Server Protocol Program (Microsoft) WSPP Western System Power Pool WSPP Workgroup Server Protocol Program WSPP Web Site Privacy Policy ) MRSA (Table 2). By using CHEF electrophoresis, ST8-MRSA-IV and ST5-MRSA-V could be further classified into WA-MRSA-5 and WA-MRSA-12, and WA-MRSA-11 and WA-MRSA-14 pulsotypes, respectively. Overall, 93.7% of CA-MRSA were classified into 3 clones: ST1-MRSA-IV (55.3%), ST129-MRSA-IV (29.8%), and ST5-MRSA-IV (8.6%). Of the CA-MRSA, 97.3% were SCCmec type IV and 2.6% SCCmec type V. Four isolates carrying novel SCCmec type(s) were found in 2 STs (ST5 and ST8). Using the MLST database, the 22 clones were grouped into 10 CCs and 2 singletons. Five clones (2.3% of CA-MRSA) were PVL positive including ST30-MRSA-IV and ST93-MRSA-IV. These 2 clones were originally reported outside WA, ST30-MRSA-IV in New Zealand and ST93-MRSA-IV in Queensland. The remaining 3 clones, ST8-MRSA-IV (MRSA-12 pulso-type), ST59-MRSA-IV, and ST583-MRSA-IV accounted for only 0.3% of CA-MRSA isolated in WA. CA-MRSA Antibiograms The online Appendix Table (available from http://www. cdc.gov/ncidod/eid/vol12no02/05-0454_app.htm) shows 6 of the 22 CA-MRSA clones (17 isolates) were predictably resistant to [beta]-1actam antimicrobial drugs only. In the remaining 16 clones, 55.9% of isolates were resistant to at least 1 non-[beta]-lactam antimicrobial drug, including 47.7% to erythromycin, 10.8% to fusidic acid, 2.9% to ciprofloxacin, 2.5% to trimethoprim, 1.8% to tetracycline, 1.6% to gentamicin, 1.3% to mupirocin, and 0.2% to rifampin. In 6 of these clones, 1.5% of isolates were classified as multidrug-resistant. None of the 73 isolates found in PVL-positive clones were multidrug-resistant: 7% of ST30-MRSA-IV were resistant to rifampin, 15% of ST93-MRSA-IV were resistant to erythromycin, 50% of ST583-MRSA-IV were resistant to fusidic acid and tetracycline, and 50% were resistant to fusidic acid and erythromycin; all the ST59-MRSA-V were resistant to tetracycline and erythromycin, and 75% and 25% of ST8-MRSA-IV (MRSA-12 pulsotype) were resistant to erythromycin and tetracycline, respectively. The 11 strains classified as ST5-MRSA-V (WA-MRSA-11 pulsotype) were all resistant to gentamicin. This strain was involved in a single strain outbreak in a burn unit. Discussion In WA, colonization or infection with MRSA has been a notifiable notifiable /no·ti·fi·a·ble/ (no?ti-fi´ah-b'l) necessary to be reported to a government health agency. notifiable necessary to be reported to the relevant government authority. Said of individual diseases. condition since 1982, which has enabled the rapid and widespread emergence of CA-MRSA to be monitored. In rural areas, the overall MRSA notification rate has increased from 10/100,000 persons in 1983 to 542/100,000 persons in 2002. Similarly, in the same period rates increased in the Perth metropolitan area from 7/100,000 to 520/100,000. Although part of this increase in the metropolitan area from 1998 was due to an increase in EMRSA notifications, most can be attributed to CAMRSA (unpub. data). In this study, 22.5% (n = 921) of MRSA isolates were classified as EMRSA. Six international epidemic clones and the classic MRSA clone, ST250-MRSA-I, were identified (Table 1). More than 78% of EMRSA isolates were identified as ST22-MRSA-IV (EMRSA-15), an nmEMRSA with the community type IV SCCmec. Originally described in the United Kingdom in the early 1990s and now the predominant epidemic strain in that country (27), ST22-MRSA-IV was first isolated in WA in 1997 in preemployment screening of healthcare workers coming from the United Kingdom and Ireland (28). Notifications have increased from 55 in 1998 to 383 in 2002 (unpub. data). Although recent national surveillance studies have also reported the emergence of ST22-MRSA-IV in other Australian states (29), the predominant EMRSA in most Australian capital cities There are eight capital cities in Australia, all of which function at a sub-national level. Of these, Canberra has also acted as the national capital since 1927. Between 1901 and the current national capital's opening, Melbourne functioned as the seat of national government. is ST239-MRSA-III (30). The 6 epidemic clones reported in this study have 6 STs which can be grouped into 4 of the 5 major epidemic CCs described by Enright et al. (5), CC5, CC8, CC22, and CC30. CC8 also includes the ancestral MRSA genotype ST250-MRSA-I, which evolved from the methicillin-susceptible strain ST250-MSSA, which is thought to have arisen from ST8-MSSA by a chromosomal mutation Noun 1. chromosomal mutation - (genetics) any event that changes genetic structure; any alteration in the inherited nucleic acid sequence of the genotype of an organism genetic mutation, mutation (5). Other STs isolated in this study, which form part of CC8, were ST8-MRSA-[IV.sub.pediatric], ST8-MRSA-[II.sub.variant], and ST239-MRSA-III. ST5-MRSA-II, ST22-MRSA-IV, and ST36-MRSA-II belong to CC5, CC22, and CC30, respectively. CA-MRSA made up 77.5% of the isolates. These MRSA have several characteristics that differentiate them from most nosocomial nosocomial /noso·co·mi·al/ (nos?o-ko´me-il) pertaining to or originating in a hospital. nos·o·co·mi·al adj. 1. Of or relating to a hospital. 2. MRSA. They harbor a smaller, SCCmec (SCCmec IV and V), are susceptible to most antimicrobial drugs other than the [beta]-lactam agents, and are more likely to encode the virulence factor PVL (31). In this study, 21 clones of WA-MRSA were identified by MLST/SCCmec typing with further delineation into 23 chromosomal DNA DNA: see nucleic acid. DNA or deoxyribonucleic acid One of two types of nucleic acid (the other is RNA); a complex organic compound found in all living cells and many viruses. It is the chemical substance of genes. pulsotypes and numerous pulsosubtypes by CHEF. Also identified was the Western Pacific CA-MRSA (ST30-MRSA-IV) first isolated in Auckland, New Zealand (32). CA-MRSA from different parts of the world has been reported with varied genetic backgrounds (24). The results presented here demonstrate that this is also the case for CA-MRSA isolated within a single state of Australia (WA). The 22 STs were grouped into 10 CCs (CC1, CC5, CC8, CC9, CC30, CC45, CC59, CC78, CC80, and CC121) and 2 singletons (ST75-MRSA-IV and ST93-MRSA-IV). The 10 CCs identified include 4 of the 5 major epidemic CCs (CC5, CC8, CC30, and CC45). Five CCs had >1 clone (2 clones in CC1 and CC45, 3 clones in CC8 and CC59, and 5 clones in CC5). The 2 predominant CA-MRSA clones isolated were ST1-MRSA-IV and ST129-MRSA-IV (55.3% and 29.8% of CA-MRSA, respectively). ST1-MRSA-IV belongs to CC1, which has the same allelic al·lele n. One member of a pair or series of genes that occupy a specific position on a specific chromosome. [German Allel, short for Allelomorph, allelomorph, from English profile as the S. aureus that is the proposed ancestor of MW2 CA-MRSA that was responsible for the deaths of 4 children in the United States (33). CC1 CA-MRSA has also been reported in France (13) and other areas of Australia (24), which indicates that this clone is particularly successful. ST129-MRSA-IV belongs to CC78, a smaller CC that includes strains isolated elsewhere in Australia, Portugal, and Japan (http://www.mlst.net). Despite the diversity of CCs, the CA-MRSA strains were remarkably uniform in their SCCmec allotypes. SCCmec IV was identified in 14 STs and SCCmec V was identified in 5. This suggests that in WA these 2 allotypes are well adapted to the community environment. Two STs were found to have novel SCCmec types. Unlike SCCmec types II and III, which carry a number of inserted plasmids and transposons Transposons Types of transposable elements which comprise large discrete segments of deoxyribonucleic acid (DNA) capable of moving from one chromosome site to a new location. downstream of the mecA complex, community-associated SCCmec types IV and V are smaller and lack other resistance genes. However, resistance may be encoded elsewhere on the chromosome or the isolate may carry resistance plasmids. Although CA-MRSA isolated in WA is typically nonmultidrug-resistant, all strains harbor a large plasmid that varies in size (34). This plasmid encodes determinants for [beta]-lactamase production and cadmium resistance. In addition, some isolates have been reported to carry a 41.4-kb plasmid that also encodes [beta]-lactamase and resistance to mupirocin, tetracycline, trimethoprim, and cadmium and a smaller plasmid (2 kb) that encodes inducible erythromycin resistance (34). Chromosomal fusidic acid and tetracycline resistance determinants have also been reported (34); however, the location of these determinants on the chromosome is unknown. In this study, 44% of CA-MRSA were resistant to [[beta]-lactam antimicrobial drugs only. Of the remaining 56%, 54.5% were also resistant to 1-2 non-[beta]-lactam agents, and 1.5% to [greater than or equal to] 3 non-[beta]-lactam agents, including 3 isolates resistant to 5 additional antimicrobial drugs (online Appendix Table). CA-MRSA have been shown to express several virulence genes, including the determinants for PVL (35). PVL is a necrotizing necrotizing /nec·ro·tiz·ing/ (nek´ro-tiz?ing) causing necrosis. Necrotizing Causing the death of a specific area of tissue. Human bites frequently cause necrotizing infections. toxin that causes leukocyte leukocyte (l  `kəsīt'): see blood. leukocyte or white blood cell or white corpuscle destruction and tissue necrosis and is associated with abscesses and severe pneumonia. PVL is present in most of the CA-MRSA studied in Europe and the United States (13). In WA, CA-MRSA infrequently carries the genes encoding PVL (34); however, 2 CA-MRSA clones, ST30-MRSA-IV, and ST93-MRSA-IV, more commonly isolated in eastern Australia are PVL positive. ST30-MRSA-IV was first noted in Australia in 1997 in the Polynesian population living in the eastern Australian states and the Australian Capital Territory Australian Capital Territory (1991 pop. 276,468), 939 sq mi (2,432 sq km), SE Australia, an enclave within New South Wales, containing Canberra, capital of Australia. It was called the Federal Capital Territory until 1938. (9). ST93-MRSA-IV was first identified as a cause of community-acquired infection in the Caucasian population in Ipswich, Queensland, in 2000 (11). Both clones are now frequently isolated in several areas of Australia (29). In WA, ST30-MRSA-IV and ST93-MRSA-IV were first isolated in 2001. In this study, PVL was detected in 5 MRSA clones, including ST30-MRSA-IV, ST93-MRSA-IV, ST8-MRSA-IV (pulsotype WA-MRSA-12), ST59-MRSA-V, and ST583-MRSA-IV. However, these 5 clones were infrequently isolated and accounted for only 2.3% of all CA-MRSA. PVL genes have been transmitted by a temperate phage designated [phi]PVL (36), which indicates that the PVL determinants are transferable. Recently, a PVL-positive ST1-MRSA-IV strain was isolated in Queensland (37) and New South Wales (38), Australian states that have reported an increasing incidence of ST30-MRSA-IV and ST93-MRSA-IV (9-11). This finding suggests that the PVL determinants are being transferred and raises the prospect that more CA-MRSA in WA may acquire PVL determinants in the future. Some researchers have proposed that CA-MRSA may arise either by hospital strains escaping into the community, where they spread person to person, or de novo [Latin, Anew.] A second time; afresh. A trial or a hearing that is ordered by an appellate court that has reviewed the record of a hearing in a lower court and sent the matter back to the original court for a new trial, as if it had not been previously heard nor decided. when the SCCmec complex is acquired by a methicillin-susceptible S. aureus isolate (24,39). In WA, the genetic background of nosocomial MRSA is different from that of CA-MRSA, and therefore, community strains have likely evolved independently of hospital strains. In addition, in WA hospitals, apart from 2 single-strain outbreaks in a large metropolitan hospital (ST1-MRSA-IV [13] and ST5-MRSA-V (WA-MRSA-11 pulsotype), little evidence has been found of CA-MRSA spreading within healthcare facilities. Although person-to-person spread most likely occurs in the community, the increasing number of MRSA in the WA community may also be due to mobility of the community SCCmec types. The genetic diversity of CA-MRSA isolated in WA and the presence of at least 3 SCCmec types also support this possibility. Conclusions Although a comprehensive MRSA screening and control program has prevented the mEMRSA from emerging, it has not prevented SCCmec type IV and type V MRSA clones, including nmEMRSA (ST22-MRSA-IV) and CA-MRSA, from becoming established in WA. SCCmec types IV and V are now found in MRSA with distantly related genetic backgrounds. In addition, at least 1 novel SCCmec type has been detected. Initially nonmultidrug-resistant, many of these CA-MRSA clones have acquired plasmids and chromosomal resistance determinants allowing some strains to become resistant to up to 5 non-[beta]-lactam antimicrobial agents, including erythromycin, tetracycline, trimethoprim, ciprofloxacin, gentamicin, rifampin, fusidic acid, and mupirocin. With the detection of 5 PVL-positive clones and the recent emergence of PVL in a previously reported PVL-negative CA-MRSA clone, more severe staphylococcal disease caused by CA-MRSA can be expected in the future. SCCmec types that can be acquired by multiple genotypes of S. aureus over a short period and the isolation of multidrug-resistant or PVL-positive CA-MRSA are major public health concerns and emphasize the importance of typing in tracing the origin of isolates and in designing antimicrobial drug prescribing policies for their control, if possible, in the community. Acknowledgments We thank the scientific staff from the Gram-positive Bacteria Typing and Research Unit (Mary Malkowski, Rebecca Lee, David Atlas and Ngan Pham) and the referring Western Australian medical microbiology laboratories, including PathWest Laboratory Medicine WA, Western Diagnostic Pathology, General Pathology, Clinipath, and Saint John of God Pathology. 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Identification of a novel staphylococcal cassette chromosome mec (type V) driven by a novel cassette chromosome ccrC. Antimicrob Agents Chemother. 2004;48:2637-51. (26.) Fey PD, Said-Salim B, Rupp ME, Hinrichs SH, Boxrud DJ, Davis CC, et al. Comparative molecular analysis of community- or hospital-acquired methicillin-resistant Staphylococcus aureus. Antimicrob Agents Chemother. 2003;47:196-203. (27.) O'Neill GL, Murchan S, Gil-Setas A, Aucken HM. Identification and characterization of phage variants of a strain of epidemic methicillin-resistant Staphylococcus aureus (EMRSA-15). J Clin Microbiol. 2001;39:1540-8. (28.) Pearman JW, Coombs GW, Grubb WB, O'Brien FG. A British epidemic strain of methicillin-resistant Staphylococcus aureus (UK EMRSA-15) has become established in Australia. Med J Aust. 2001;174:662. (29.) Coombs GW, Nimmo GR, Bell J, Huygens F, O'Brien FG, Malkowski MJ, et al. Genetic diversity among community methicillin-resistant Staphylococcus aureus strains causing outpatient infections in Australia. J Clin Microbiol. 2004;42:4735-43. (30.) Coombs GW, Malkowski MJ, Pearson JC, Bell JM, Nimmo GR. Epidemic MRSA in Australia. In: Abstracts of the 10th International Symposium on Staphylococci and Staphylococcal Infections Staphylococcal Infections Definition Staphylococcal (staph) infections are communicable conditions caused by certain bacteria and generally characterized by the formation of abscesses. ; 2002 Oct 16-19; Tsukuba, Japan. Abstract 203-02. (31.) Charlebois ED, Perdreau-Remington F, Kreiswirth B, Bangsberg DR, Ciccarone D, Diep BA, et al. Origins of community strains of methicillin-resistant Staphylococcus aureus. Clin Infect Dis. 2004;39:47-54. (32.) Mitchell JM, MacCulloch D, Morris AJ. MRSA in the community. NZ Med J NZ MED J New Zealand Medical Journal . 1996;109:411. (33.) From the Centers for Disease Control and Prevention Centers for Disease Control and Prevention (CDC), agency of the U.S. Public Health Service since 1973, with headquarters in Atlanta; it was established in 1946 as the Communicable Disease Center. . Four pediatric deaths from community-acquired methicillin resistant Staphylococcus aureus--Minnesota and North Dakota, 1997-1999. JAMA JAMA abbr. Journal of the American Medical Association . 1999;282:1123-5. (34.) O'Brien FG, Lim TT, Chong FN, Coombs GW, Enright MC, Robinson DA, et al. Diversity among isolates of methicillin-resistant Staphylococcus aureus in Australia. J Clin Microbiol. 2004;42: 3185-90. (35.) Baba T, Takeuchi F, Kuroda M, Yuzawa H, Aoki K, Oguchi A, et al. Genome and virulence determinants of high virulence community-acquired MRSA. Lancet. 2002;359:1819-27. (36.) Kaneko J, Kimura T, Narita S, Tomita T, Kamio Y. Complete nucleotide sequence and molecular characterization of the temperate staphylococcal bacteriophage [phi]PVL carrying Panton-Valentine leukocidin genes. Gene. 1998;215:57-67. (37.) Stephens AJ, Huygens F, Nimmo G, Giffard E Variable binary gene typing increases resolution of methicillin-resistant Staphylococcus aureus MLST clonal groups defined by SNP SNP Scottish National Party Noun 1. SNP - (genetics) genetic variation in a DNA sequence that occurs when a single nucleotide in a genome is altered; SNPs are usually considered to be point mutations that have been evolutionarily typing. In: Abstracts of the 11th International Symposium on Staphylococci and Staphylococcal Infections; 2004 Oct 24 27; Charleston, South Carolina South Carolina, state of the SE United States. It is bordered by North Carolina (N), the Atlantic Ocean (SE), and Georgia (SW). Facts and Figures Area, 31,055 sq mi (80,432 sq km). Pop. (2000) 4,012,012, a 15. . Abstract ME-30. (38.) Gosbell IB, Barbagiannakos T, Burke H, Kennedy C, Vickery A, Lambie P, et al. Community MRSA in far western New South Wales: Emergence of two epidemic clones and emergence of Panton-Valentine leukocidin in a previous naive clone. In: Abstracts of the 11th International Symposium on Staphylococci and Staphylococcal Infections; 2004 Oct 24-27; Charleston, South Carolina. Abstract CA-10. (39.) Daum RS, Ito T, Hiramatsu K, Hussain F, Mongkolrattanothai K, Jamklang M, et al. A novel methicillin-resistance cassette in community-acquired methicillin-resistant Staphylococcus aureus isolates of diverse genetic backgrounds. J Infect Dis. 2002; 186:1344-7. Geoffrey W. Coombs, * ([dagger]) Julie C. Pearson, * Frances G. O'Brien, ([dagger]) Ronan J. Murray, * Warren B. Grubb, ([dagger]) and Keryn J. Christiansen * ([dagger]) * Royal Perth Hospital, Perth, Western Australia This article is about the metropolitan area of Perth, Western Australia. For the local government area, see City of Perth. Perth is the capital of the Australian state of Western Australia. , Australia; and ([dagger]) Curtin University of Technology, Bentley, Western Australia Bentley is a southern suburb of Perth, the capital city of Western Australia, and is located 8 km southeast of Perth's central business district. Its Local Government Areas are the City of Canning and the Town of Victoria Park. , Australia Address for correspondence: Keryn Christiansen, Department of Microbiology and Infectious Diseases, Royal Perth Hospital, PathWest Laboratory Medicine WA, Wellington St, Perth 6000, Western Australia, Australia; fax: 61-8-9224-1989; email: keryn.christiansen@health.wa. gov.au Dr Coombs is the principal scientist at the Department of Microbiology and Infectious Diseases and the Gram-positive Bacteria Typing and Research Unit at Royal Perth Hospital, Western Australia; a microbiology research fellow at Curtin University of Technology; and a lecturer at Notre Dame University, Fremantle. His major area of research is the epidemiologic typing and molecular characterization of MRSA.
Table 1. Characteristics of EMRSA clones * (of 4,099 total MRSA
isolates), Western Australia, July 1, 2003-December 31, 2004
CHEF pattern
Clone (pulsotypes) n (% of total MRSA)
ST22-MRSA-IV EMRSA-15 719 (17.54)
ST239-MRSA-III Aus-2 EMRSA 95 (2.32)
Aus-3 EMRSA 57 (1.39)
ST8-MRSA-IVp Irish-2 EMRSA 20 (0.49)
ST36-MRSA-II EMRSA-16 16 (0.39)
ST5-MRSA-II New York/Japan EMRSA 11 (0.27)
ST8-MRSA-IIv Irish-1 EMRSA 2 (0.05)
ST250-MRSA-I Classic MRSA 1 (0.02)
Total 921 (22.47)
Coagulase PCR
Clone CC Urease RFLP pattern PVL toxin
ST22-MRSA-IV 22 Neg 22 Neg
ST239-MRSA-III 8 Pos 24 Neg
8 Pos 24 Neg
ST8-MRSA-IVp 8 Neg 18 Neg
ST36-MRSA-II 30 Pos 18 Neg
ST5-MRSA-II 5 Pos 36 Neg
ST8-MRSA-IIv 8 Neg 18 Neg
ST250-MRSA-I 8 Pos 18 Neg
Total
* EMRSA, epidemic methicillin-resistant Staphylococcus aureus;
CHEF, contour-clamped homogeneous electric field; CC, clonal
complex; PCR, polymerase chain reaction, RFLP, restriction
fragment length polymorphisms; PVL, Panton-Valentine leukocidin;
MRSA, me thicillin-resistant S. aureus; p, pediatric, v, variant.
Table 2. Characteristics of community MRSA clones * (of 4,099 total
MRSA isolates), Western Australia, July 1, 2003-December 31, 2004
CHEF pattern n (% of total
Clone (pulsotypes) MRSA) CC Urease
ST1-MRSA-IV WA MRSA-1 1,757 (42.86) 1 Pos
ST129-MRSA-IV WA MRSA-2 947 (23.10) 78 Pos
ST5-MRSA-IV WA MRSA-3 273 (6.66) 5 Pos
ST45-MRSA-V WA MRSA-4 60 (1.46) 45 Pos
ST8-MRSA-IV WA MRSA-5 27 (0.66) 8 Pos
WA MRSA-12 4 (0.1) 8 Pos
ST93-MRSA-IV WA MRSA-7 34 (0.83) S Pos
ST75-MRSA-IV WA MRSA-8 9 (0.22) S Pos
ST59-MRSA-V WA MRSA-9 3 (0.07) 59 Pos
ST573-MRSA-V WA MRSA-10 2 (0.05) 1 Pos
ST5-MRSA-V WA MRSA-11 11 (0.27) 5 Pos
WA MRSA-14 4 (0.09) 5 Pos
ST584MRSA-IV WA MRSA-13 1 (0.2) 9 Pos
ST59-MRSA-IV WA MRSA-15 3 (0.07) 59 Pos
ST8-MRSA-Novel WA MRSA-16 1 (0.2) 8 Neg
ST583-MRSA-IV WA MRSA-17 2 (0.5) 80 Pos
ST5-MRSA-Novel WA MRSA-18 1 (0.02) 5 Pos
ST609-MRSA-IV WA MRSA-19 1 (0.02) 8 Neg
ST5-MRSA-Novel WA MRSA-21 2 (0.5) 5 Pos
ST577-MRSA-V WA MRSA-22 3 (0.07) 121 Pos
ST45-MRSA-IV WA MRSA-23 1 (0.02) 45 Neg
ST87-MRSA-IV WA MRSA-24 1 (0.02) 59 Pos
ST575-MRSA-IV WA MRSA-25 1 (0.02) 5 Pos
ST30-MRSA-IV WSPP MRSA 30 (0.73) 30 Pos
Total 3,178 (77.53)
CHEF pattern Coagulase PCR
Clone (pulsotypes) RFLP pattern PVL toxin
ST1-MRSA-IV WA MRSA-1 20 Neg
ST129-MRSA-IV WA MRSA-2 258 Neg
ST5-MRSA-IV WA MRSA-3 36 Neg
ST45-MRSA-V WA MRSA-4 DNC Neg
ST8-MRSA-IV WA MRSA-5 18 Neg
WA MRSA-12 18 Pos
ST93-MRSA-IV WA MRSA-7 32 Pos
ST75-MRSA-IV WA MRSA-8 DNA Neg
ST59-MRSA-V WA MRSA-9 40 Pos
ST573-MRSA-V WA MRSA-10 34 Neg
ST5-MRSA-V WA MRSA-11 34 Neg
WA MRSA-14 40 Neg
ST584MRSA-IV WA MRSA-13 32 Neg
ST59-MRSA-IV WA MRSA-15 40 Neg
ST8-MRSA-Novel WA MRSA-16 18 Neg
ST583-MRSA-IV WA MRSA-17 DNC Pos
ST5-MRSA-Novel WA MRSA-18 36 Neg
ST609-MRSA-IV WA MRSA-19 18 Neg
ST5-MRSA-Novel WA MRSA-21 34 Neg
ST577-MRSA-V WA MRSA-22 42 Neg
ST45-MRSA-IV WA MRSA-23 22 Neg
ST87-MRSA-IV WA MRSA-24 40 Neg
ST575-MRSA-IV WA MRSA-25 256 Neg
ST30-MRSA-IV WSPP MRSA 24 Pos
Total
* MRSA, methicillin-resistant Staphylococcus aureus; CHEF,
contour-clamped homogeneous electric field; CC, clonal complex; PCR,
polymerase chain reaction; RFLP, restriction fragment length
polymorphisms; PVL, Panton-Valentine leukocidin; WA MRSA, Western
Australia MRSA; DNC, did not cut; S, singleton; DNA, did not amplify;
WSPP MRSA, Western Samoan phage pattern MRSA.
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