Abstract
Staphylococcus aureus is a leading cause of bloodstream infections (BSI) and diseases that may be caused by hematogenous spread. The staphylococcal adhesin, for which the association with the infections emerging as a complication of septicemia has been well documented, is a bone sialoprotein-binding protein (Bbp). The aim of the study was to assess the prevalence of a bbp gene in S. aureus bloodstream isolates associated with BSI and to investigate to what degree the distribution of this gene is linked to the clonality of the population. Spa typing, used in order to explore the genetic population structure of the isolates, yielded 29 types. Six spa clusters and seven singletons were identified. The most frequent was spa clonal complex CC021 associated with MLST CC30 (38 %). The bbp gene was found in 47 % of isolates. Almost all isolates (95 %) clustered in spa clonal complex CC021 were positive for this gene. All isolates carrying the bbp gene were sensitive to methicillin, and if clustered in the spa CC021, belonged to agr group III. Our study shows that Bbp is not strictly associated with BSI. However, one may conclude that for clonally related S. aureus strains most commonly causing BSI, the risk of Bbp-mediated complications of septicemia is expected to be higher than for other strains.
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Introduction
Staphylococcus aureus is a leading cause of bloodstream infections (BSI) (Grundmann et al. 2010). Hospital BSIs caused by this bacterium are associated with significant morbidity and mortality, particularly in populations at high risk of infection. An early and critical step in establishing BSI process is bacterial adhesion and colonization of host tissues (Naber 2009). In S. aureus, surface proteins interacting with host molecules were named Microbial Surface Components Recognizing Adhesive Matrix Molecules (MSCRAMMs) (Patti and Höök 1994 ). The relationship between the tissue tropism and the expression of particular MSCRAMMs is still insufficiently cleared but the adhesin, for which the association with the infections emerging as a complication of septicemia has been well documented, is a bone sialoprotein-binding protein (Bbp) (Cunningham et al. 1996; Rydén et al. 1987, 1989). Moreover, there is evidence that the role of Bbp can be broader than that of a simple tissue tropism (Persson et al. 2009; Vazquez et al. 2011).
The Bbp interacts with bone sialoprotein (BSP), an essential component of bone and dentine extracellular matrix (Yacoub et al. 1994). It is possible that Bbp may function in two capacities: as an important factor in the colonization of bone tissue and as a contributing factor in S. aureus hematologic diseases (Berendt and Byren 2004). In an in vivo animal model, BSP binding capacity was found in all staphylococci-producing septic arthritis (Bremell et al. 1991). Moreover, the serum from patients suffering from bone and joint infection contained antibodies that reacted with the fusion protein of the BSP-binding protein, indicating that the protein is expressed during an infection and is immunogenic (Persson et al. 2009). The study of Vazquez et al. (2011) showed that human fibrinogen is also a ligand for Bbp which can manipulate the biology of the fibrinogen in the host (Vazquez et al. 2011). Thus, a specificity of Bbp for a factor other than BSP cannot be excluded.
The diseases preferentially associated with Bbp are osteomyelitis and septic arthritis (Bremell et al. 1991; Rydén et al. 1987, 1997). The presence of bbp gene encoding for Bbp in S. aureus-caused orthopedic implant infections has been described (Campoccia et al. 2009). Moreover, co-existence of bbp and collagen-binding protein (cna) gene in such isolates suggests that these two adhesins may act together in the implant infections (Campoccia et al. 2009). The combination of the bbp and cna genes was also found in the pandemic type of community-acquired methicillin-resistant S. aureus (CA-MRSA) (Arnold et al. 2006). According to evidence, the expression of S. aureus bbp gene may correlate with genes for methicillin-resistance and Panton-Valentine leukocidin (PVL) (Otsuka et al. 2006; Witte et al. 2005). The association between the accessory gene regulator (agr) system and bbp presence in S. aureus has also been described (Montanaro et al. 2010).
The species S. aureus has a highly clonal population structure (Feil et al. 2003) but the frequency of Bbp in S. aureus isolates causing bacteremia has not been well documented. Moreover, the diseases associated with Bbp may be a complication of septicemia as the staphylococci reach a bone or joint region via the bloodstream. For this reason, the aim of the present study was to assess the prevalence of the bbp gene in S. aureus isolates associated with BSI and to investigate to what degree the distribution of this gene is linked to the clonality of the population.
Materials and methods
Bacterial isolates
The study was performed on 53 S. aureus bloodstream isolates obtained from patients of 19 departments of the University Clinical Center (UCC) in Gdańsk, including the following: cardiology (12); nefrology, transplantology, and internal medicine—NTIM (6); hematology (4); internal medicine, endocrinology, and homeostasis disturbances—IMEHD (4); gastrohepatology (3); hypertension and diabetology (3); adult neurology (3); intensive care unit—ICU (3); oncology and radiology (2); internal medicine and intoxications—IMI (2); isolation unit (2); cardiac surgery; hypertension, internal medicine, hemodialysis, and transplant medicine—HIMHTM; venerology and allergology; rehabilitation; pediatric nefrology; pediatric oncology, hematology and endocrinology—POHE; neurological surgery (1 each); not classified (2). All the patients were considered to have true bloodstream infection defined as at least one blood culture positive for S. aureus during the presence of the systemic inflammatory response syndrome. The additional data about clinical recognitions and risk factors associated with BSI in individual patients were not available. The strains were isolated in the UCC laboratory from March 2008 to March 2009 (13 months) and sent to the Microbiology Department of the Medical University of Gdańsk for further analyses. The first isolate from patient was included in the study. The bacteria were cultured on sheep blood agar (Oxoid, UK) and were re-identified by API ID32 Staph system (Bio Mérieux, France). For further purposes, the isolates were subcultured on nutrient broth and stored in glycerol at −70 °C.
Bacterial DNA isolation
Genomic DNA used as an amplification template was extracted from the bacterial cultures using Gene MATRIX Bacterial & Yeast Genomic DNA Purification Kit (EURx Ltd., Poland) according to the manufacturer’s instruction.
Antimicrobial drug susceptibility testing
Resistance to methicillin was primary tested using disc diffusion method on Mueller Hinton agar (Oxoid, UK), with oxacillin and cefoxitin discs (Becton Dickinson, Germany) and confirmed by the detection of mecA gene by polymerase chain reaction (PCR) (Barski et al. 1996). The susceptibility to antimicrobial agents was determined by the disc diffusion method according to recommendations given by Hryniewicz et al. (2005) and the CLSI guidelines (2006). The antibiotics tested were the following: penicillin, erythromycin, clindamycin, ciprofloxacin, co-trimoxazole, tetracycline, gentamicin, vancomycin, teicoplanin, fusidic acid, rifampicin, linezolid, quinupristin-dalfopristin, chloramphenicol (Becton Dickinson, Germany), and mupirocin (Oxoid, UK). For all the isolates beta-lactamase production was checked by nitrocefin test (Becton Dickinson, Germany). For isolates identified as resistant to erythromycin, but susceptible to clindamycin, D-test was performed to detect inducible clindamycin resistance (Fiebelkorn et al. 2003). The susceptibility to vancomycin was confirmed by the minimal inhibitory concentration (MIC) using E-tests, as described by the manufacturer (AB Biodisc, Sweden).
Detection of bbp and cna genes
Detection of bbp and cna genes was performed by PCR. The nucleotide sequence of the primers and thermal cycling conditions were described by Tristan et al. (2003).
Detection of PVL genes
All the isolates were screened for the presence of lukS-PV and lukF-PV genes by PCR as described by Lina et al. (1999).
Spa typing and based upon repeat pattern analysis
The polymorphic X region of the protein A gene (spa) was amplified from the isolates by PCR according to the procedure described by Harmsen et al. (2003). Spa types were determined by using Ridom Staph Type software (Harmsen et al. 2003). The spa types were clustered into spa CCs (clonal complexes) using the algorithm based upon repeat pattern (BURP) (Rupptisch et al. 2006).
Determination of MLST clonal complexes
Since spa typing, together with the algorithm BURP, and multilocus sequence typing (MLST) are highly concordant (Enright et al. 2000; Strommenger et al. 2008), the associated MLST CCs were allocated through the Ridom SpaServer database (www.spaserver.ridom.de).
Agr typing
The agr group-specific multiplex PCR was performed with the use of primers and thermal cycling conditions described previously (Shopsin et al. 2003).
SCCmec typing
Typing of the staphylococcal chromosomal cassette (SCC) mec was done in MRSA isolates as described previously (Milheiriço et al. 2007).
Results
The results of the current bbp gene research, in relation to spa typing and clonal complexes analysis, are provided in Table 1. Spa–typing yielded 29 types. BURP analysis of the spa types identified six clusters and seven singletons. The most frequent was spa CC021, associated with MLST CC30, harboring 38 % of the isolates. Within the spa CC021, consisted of nine types, the most common was t021 (7/20 = 35 %). The second frequent was singleton represented by 13 % of the isolates, with only one spa type t127 related to MLST CC1. The third one was spa CC085 (9 %) consisted of three types: t084, t085, t355 associated with MLST CC15. The bbp gene was found in 47 % of the isolates. Most of the isolates positive for bbp belonged to the spa CC021 (76 %). The bbp gene occurred in 19/20 isolates of this cluster (95 %). The remaining isolates carrying the bbp gene were included in a cluster without the primary founder of a group (t645 and t4495), associated with MLST CC121, or in spa CC775 related to MLST CC25 (t056 and t775). One isolate with spa repeat pattern uncorrelated with other types was also positive for bbp. No one isolate belonging to the most frequent singleton or to the spa CC085 carried the bbp gene.
Table 2 shows that in the total studied population only three isolates (6 %) were resistant to methicillin. The MRSA isolates were identified as t032/SccmecIV, t008/SccmecIV, and t003/SccmecII (shown in footnote below the table). None of the MRSA isolates were positive for bbp, whereas 3/7 of the PVL-positive isolates carried the bbp gene. The cna gene was detected in 33/53 isolates (62 %) of which 19 (58 %) also carried bbp. The agr polymorphism study revealed that the most frequent were the agr types III (29/53 = 55 %) and I (14/53 = 26 %). The bbp gene possessed 69 % of the isolates of the agr group III, 14 % of the isolates of the agr group I and all the isolates of the agr group IV. No isolate belonging to the agr group II was positive for bbp.
The subpopulation of isolates positive for bbp was described in Table 3. According to our data, such isolates were distributed in 16 departments and were constantly present in the UCC throughout the observed period. The bbp positive isolates were obtained with the highest frequency from patients of the cardiology (16 %) and the nefrology, transplantology, and internal medicine department (12 %). Almost all isolates with the bbp gene (92 %) were resistant to penicillin. All penicillin-resistant isolates produced beta-lactamase (data not shown). Resistance to penicillin only was observed in 56 % of isolates, in terms of the spa CC021 and one of the clusters without the primary founder of a group. In five isolates (20 %) exhibiting penicillin resistance, additional resistance to macrolides, inducible or constitutive, was observed. Three isolates (12 %), including two belonging to the spa CC775/agr type I and one to CC021, were sensitive to all the antibiotics. Only one isolate was resistant to penicillin, macrolides, ciprofloxacin, tetracycline, and chloramphenicol. The isolates harboring the bbp gene belonged to agr group III in 84 % were positive for cna gene in 88 % and for PVL in 12 %. None of the isolates belonging to the spa CC021 harbored the PVL gene.
Discussion
In the first step of our investigations, we focused on molecular characterization of the S. aureus isolates associated with BSI. In order to explore the genetic population structure of the isolates, we used spa genotyping as a method with both a high discriminatory power and results that can be easily compared between laboratories (Strommenger et al. 2008). Spa typing is based on the variation of the polymorphic region within the staphylococcal protein A gene (Harmsen et al. 2003). There is a high concordance between spa typing and other genotyping methods, including MLST (Enright et al. 2000; Strommenger et al. 2008). Thus, we analyzed the results considering the relationship to MLST clones described in database.
Looking at the clonal structure of the isolates, our results confirm several major findings of previously published surveys (Fenner et al. 2003; Grundmann et al. 2010; Nulens et al. 2008). The most frequent in our collection was spa CC021 related to MLST CC30, with the main spa type t021. According to the data obtained by international multicenter trials, t021 belongs to the 20 most frequent spa types among S. aureus isolates causing invasive infections in Europe (Grundmann et al. 2010). We confirmed findings of a study on local population of S. aureus in Eastern Pomerania, Poland, where within CC30, the t021 dominated the bloodstream isolates (Holtfreter et al. 2007). But, interestingly, in that study, CC30 was significantly more common among nasal strains than among blood culture isolates. It could mean that CC30 is widely disseminated among Polish S. aureus strains population in general. In contrast, in other European countries, CC30 is reported as more prevalent in invasive strains than in noninvasive (Wertheim et al. 2005). For example, spa types corresponding with CC30 were observed in invasive MSSA in a Swiss University Hospital (Fenner et al. 2003) and in bloodstream isolates collected from a Dutch University Hospital (Nulens et al. 2008). The more recent study from Norway showed that CC30 was the most frequent clonal complex in MSSA isolates from deep surgical site infections in orthopedic patients (Aamot et al. 2012). However, there were some differences, when comparing our results to data published by others. The t002/ST-5 and t084/ST-15 were described as the first spa types among MSSA from invasive infections in Europe in 2010. In Polish laboratories participating in that study, the most prevalent among MSSA were t127/ST-1, t084/ST-15, and t015/ST-45 (Grundmann et al. 2010). In our collection, t127 was observed as frequently as t021 but with no correlation to other spa types and t002 was not found at all.
The main conception of our study was to assess the prevalence of the bbp gene, in relation to the clonality of the population described above. The results could mean that Bbp is not strongly associated with BSI, as the gene for this factor was found in almost half of the isolates. It may be not surprising, since our strain collection was not restricted to patients with selected risk factors for a particular location of infection, as it has been described in the literature (Aamot et al. 2012; Luedicke et al. 2010; Rydén et al. 1989). For example, in the Aamot et al. study (2010) on MSSA isolates from deep surgical site infections in orthopedic patients, 95 % of the isolates from invasive diseases were positive for bbp. Moreover, our investigations were not restricted to the departments where, according to evidence, the bbp-positive strains among S. aureus isolates were supposed to occur with the highest frequency (Aamot et al. 2012). But the findings of previously published investigations on S. aureus strains associated with blood infections were not consistent. For example, in the study of Tristan et al. (2003), the bbp gene was strictly associated with S. aureus strains involved in human hematogenous infections. By contrast, in the Hogevik et al. report (1998), no correlation was found between the potential bacterial virulence factors, including Bbp and infective endocarditis. What comes to our notice is that almost all bbp positive isolates were clustered to the spa CC021, corresponding to MLST CC30—the most widely disseminated clonal complex among the S. aureus bloodstream isolates from the UCC. It is interesting in view of the hypothesis that CC30 causes systemic infections only under very accommodating conditions (Holtfreter et al. 2007).
The production of toxins and surface proteins in S. aureus is globally regulated by the agr system. Four allelic groups of agr have been recognized in S. aureus (Novick et al. 1993). Some epidemiological findings suggest that the particular agr group can correspond to the genetic background in this bacterium and may be associated with virulence profile suitable to clinically specific infections (Montanaro et al. 2010). In our study, the most frequently observed agr III group was generally associated with the presence of the bbp gene, whereas the second one agr I was rather negative. Additionally, a few isolates of agr IV showed full association with the bbp gene, in contrast to agr II, fully negative for this gene. The similar observation was done by Montanaro et al. (2010) in S. aureus isolates from orthopedic implants infections. They showed that agr III differed clearly from agr I and II, exhibiting high prevalence of bbp, whereas agr I and II generally did not harbor this gene. Moreover, the same authors described agr II in such isolates as to be frequent in epidemic clones.
The association between the presence of bbp and cna genes, similar to that found in S. aureus causing orthopedic implant infections (Campoccia et al. 2009) was not observed in our bloodstream isolates. The frequencies of the cna gene in bbp-negative and bbp-positive isolates were similar. However, most of the isolates carrying the bbp gene were positive for cna. Thus, the conclusion that these two adhesins act together in BSI may not be excluded. It is clear that the interactions of S. aureus with host cells are complex.
The lack of the bbp gene in any MRSA strains may be explained by relatively low prevalence of MRSA among bloodstream isolates at the UCC in the study period. Our earlier investigations, performed on MRSA population in this hospital, revealed the predominance of spa CC010 and spa types related to CA-MRSA (Wiśniewska et al. 2012). The present study confirmed that in the bloodstream collection isolates two spa types associated with CA-MRSA: t008/SCCmecIV and t0032/SccmecIV occurred, but both were negative for bbp. Looking at the antibiotic resistance patterns of the bbp positive strains, selective pressure of antibiotics which may affect the frequency of this factor in the bloodstream isolates seems to be unlikely. One of the distinguishing features of CA-MRSA is that high percentage of such strains is positive for PVL (Witte et al. 2005). In our collection of bloodstream isolates, the PVL gene occurred occasionally. Moreover, the frequency of this gene in bbp-positive subpopulation, versus bbp-negative subpopulation, was similar. As a consequence, an association could be excluded.
To sum up, our study shows that Bbp is not strictly associated with BSI. However, from the results one may conclude that for clonally related S. aureus strains most commonly causing BSI, the risk of Bbp-mediated complications of septicemia is expected to be higher than for other strains. We found the clonal complex widely distributed among invasive S. aureus strains in Europe as to be strongly associated with Bbp. In fact, the high frequency of the bbp gene in the most prevalent clone could mean that Bbp contributes to the disease. Although, coincidental presence of this gene in the clone, which is common for other reasons than the carriage, may not be excluded (Aamot et al. 2012).
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Wiśniewska, K., Piórkowska, A., Kasprzyk, J. et al. Clonal distribution of bone sialoprotein-binding protein gene among Staphylococcus aureus isolates associated with bloodstream infections. Folia Microbiol 59, 465–471 (2014). https://doi.org/10.1007/s12223-014-0321-7
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DOI: https://doi.org/10.1007/s12223-014-0321-7