Staphylococcus aureus is responsible for a wide range of both community- and healthcare-acquired human diseases. It is a main cause of skin and soft tissue infections but can also produce life-threatening illnesses. p-lactam antibiotics are widely used in medicine being generally effective for the treatment of illnesses caused by this bacterium. However, there are methicillin-resistant S. aureus (MRSA) strains circulating around the world, questioning the empirical use of these antibiotics.15
Methicillin resistance in S. aureus is mostly mediated by the expression of an additional penicillin-binding-protein 2a (PBP2a) with low affinity for p-lactam antibiotics (except ceftobiprole and ceftaroline), encoded by the mecA gene or less frequently by the mecC gene. This fact determines oxacillin minimum inhibitory concentrations (MICs) of >4 pg/ml. However, S. aureus carrying the mecA gene but oxacillin-susceptible (OS-MRSA) (MICs <2 pg/ml) has been described worldwide, challenging its detection and treatment.1,3,11,13 The difference between the phenotypic and genotypic results could be explained by two previ-ously known phenomena: the existence of strains with inducible resistance and strains with high heteroresistance to oxacillin. In the former case, S. aureus carrying the mecA gene becomes phenotypically oxacillin-resistant after expo-sure to oxacillin or cefoxitin; in the second case, gene expression and, therefore, oxacillin resistance, occur in a few cells in the original bacterial population that are selected when the entire population is exposed to the antibiotic.14 Furthermore, nucleotide changes within the mecA gene, determining the emergence of a premature stop codons that reverted by point mutations after exposure to cefoxitin, restoring the gene expression and therefore the resistant phenotype,7 were described in OS-MRSA mecA positive and PBP2a negative strains (known as ''stealth methicillin-resistant S. aureus”).
In Uruguay, an OS-MRSA strain was previously reported in a case of infantile septic arthritis.6
Therefore, we set out to investigate whether other OS-MRSA strains were circulating in our country and to know their phenotypic and genotypic characteristics.
Between January and June 2018, we analyzed a set of 27, consecutive, non-duplicate S. aureus strains with oxacillin MIC values between 1 and 2 pg/ml and negative cefoxitin screening test according to the Vitek 2 compact system (bioMérieux, AST-P577 card), software version 6.2.
The strains were isolated in different clinical micro-biology laboratories at public and private health centers in Montevideo (n = 19) and 3 other regions: Treinta y Tres (n = 2), Durazno (n = 2) and Canelones (n = 4) and were recov-ered from skin and soft tissue infections (n = 21), blood (n =4), joint fluid (n = 1) and catheter tip (n = 1). The strains were submitted to the Bacteriology and Virology depart-ment, Medicine School, Montevideo, Uruguay.
This work was approved by the Ethics Committee of the Centro Hospitalario ''Pereira Rossell”.
We performed the cefoxitin disk diffusion test. Testing for oxacillin and cefoxitin was also done by gradient diffusion tests. Oxacillin MIC values of <2 pg/ml and cefoxitin values of <4 pg/ml were defined as susceptible. S. aureus ATCC 25923 and 29213 strains were used as quality controls 2.
The 27 strains were again analyzed by the Vitek 2 compact system (bioMérieux, AST-P577 card), software ver-sion 6.2, and also by Phoenix (Becton Dickinson) and MicroScan (Siemens Healthcare Diagnostics) panels.
PBP2a production was determined by the PBP2a SA culture colony test (Alere Inc., Scarborough, ME).
Detection of the mecA gene was carried out by PCR using the primers MECA P4 and MECA P7 according to Milheirico et al.10 SCCmec typing was done by a multiplex PCR assay.9
The obtained profiles by pulsed field gel electrophoresis (PFGE) with SmaI enzyme were analyzed by the unweighted pair group method with arithmetic average (UPGMA) using BioNumerics v.7.1. The isolates with >80% similarity were included in the same pulsotype (PT), while those that showed >95% similarity were considered to have identical pulsotype.8 S. aureus subsp. aureus (strain NCTC 8325) was included as reference.
In the disk diffusion test, 26 strains showed a cefoxitin inhibition zone of <21 mm (resistant phenotype) whereas only one displayed a diameter of 22 mm (susceptible phenotype) (Table 1). The mean value of the cefoxitin inhibition zone was 19 mm (range 12-22).
By the gradient diffusion test, 3 strains were susceptible to cefoxitin (MIC =4 ^g/ml), while the 24 remaining strains were resistant, with MIC values of 6 to 8 ^g/ml. Moreover, 2 strains were resistant to oxacillin, with MIC values of 4 and 8 ^g/ml, one strain showed a MIC value = 3 ^g/ml and the remaining ones (n = 24) were defined as susceptible with MIC values of <2 ^g/ml (Table 1).
All the strains (n = 27) were methicillin-susceptible, 15 displayed the inducible resistance phenotype to macrolides, lincosamides and streptogramin B antibiotics (iMLSB) and one was also resistant to gentamicin (Fig. 1). None of the strains showed resistance to the other antibiotics included in the panels.
Phoenix® and MicroScan® systems detected resistance to methicillin in 25 and 27 strains, respectively (Table 1).
Twenty-six OS-MRSA strains tested positive for PBP2a.
All strains tested positive for the mecA gene by PCR. Twenty-six OS-MRSA strains carried SCCmec type V and one the SCCmec type IV (see Table 1). PFGE analysis showed that 24 strains belonged to a large cluster or pulsotype (named A, Fig. 1) that carried the SCCmec type V. At the moment and for economic reasons, we performed the MLST assay in only one strain (# 25, isolated from blood culture, SCCmec type V and PT A) (Fig. 1) that corresponded to sequence type 8 (ST8).
This study shows the spread of a set of mecA gene positive S. aureus strains, all misidentified as MSSA by the Vitek 2 system version 6.2. Similar isolates were previously reported from cases of human and animal infections.1,3,10"12,14 In Uruguay, OS-MRSA was first reported by Giudice et al., arising from a discrepancy in the methicillin susceptibility results between two isolates of S. aureus recovered from two clinical samples of the same patient (both strains carry-ing SCCmec type V and with an identical SmaI-PFGE profile).6 Most strains analyzed in this study (n = 24) showed oxacillin MICs of <2 ^g/ml by the gradient diffusion test. These data are consistent with the known fact that oxacillin is not reli-able for the detection of methicillin resistance mediated by the mecA gene in S. aureus. Cefoxitin is more reliable but may not yet detect heterogeneous resistance to methicillin. In this sense, three strains were also misidentified as MSSA by the cefoxitin gradient diffusion test and one by the cefoxitin disk assay. Anyway, most strains showed cefoxitin inhibition zones close to the breakpoint value.
As we described before, the discrepancy between these genotypic and phenotypic results could be due, among other reasons, to heterogeneously resistant and inducible MRSA strains.3,4,14,15 We believe that most of the OS-MRSA strains studied here (n = 26, all of them PBP 2a-positive) exhibit the oxacillin heteroresistance phenotype.
Only one strain was negative to PBP 2 a and could cor-respond to ''stealth methicillin-resistant Staphylococcus” aureus due to mecA gene instability.7 However, to rule out or confirm this hypothesis, it is necessary to carry out at least the complete sequencing of the mecA gene.
Additional problems for the correct identification of this MRSA could be related to the use of automated systems for identification and susceptibility testing. In 2018, the United States Food and Drug Administration recalled Vitek 2 Gram-positive antimicrobial susceptibility testing cards due to false results for some strains of MRSA.5 Taking care of this matter, the local agent of bio Mérieux in Uruguay updated the Vitek 2 software to version 8.01. The 27 strains of OS-MRSA were subsequently retested using this new version, and all of them were correctly identified as methicillin-resistant strains (data not shown).
Unlike the findings of Andrade-Figueiredo et al.1 in which the OS-MRSA strains analyzed were highly diverse by MLST and SmaI-PFGE, the results of PFGE in this work suggest the dissemination of a cluster of S. aureus with SCCmec V in 4 regions of Uruguay. Interestingly, a strain named SA454 with similar phenotypic and genotypic characteristics to most of those described in this work (oxacillin MIC of 1 g/ml by the E-test, diameter of the inhibition halo = 22mm to cefoxitin disk, mecA and PBP2a positive with SCCmec V, recovered in 2009 from a patient with surgical site infection) was previ-ously reported in Argentina. This suggests that similar or even identical OS-MRSA strains could be present in both countries of the Río de la Plata.3 Other studies that compare in detail the genome of OS-MRSA strains present in both countries are needed to evaluate this hypothesis. One of analyzed 27 strains corresponded to ST8; to better assess the clonality of this set, it would be necessary to carry out this and other procedures of molecular epidemiology on all of them.
We analyzed 27 S. aureus strains carrying the mecA gene that had laboratory problems to be identified as MRSA, probably due to a heteroresistant phenotype. The major-ity (n=26) exhibited SCCmec type V and belonged to the same pulsotype. The cefoxitin disk and the detection of PBP2a after the induction tests appear to be the most reli-able to identify this OS-MRSA. Both procedures are relatively simple and are available in low-complexity microbiology laboratories. However, we must bear in mind that they can yield false negative results; therefore, when there is a suspicion of MRSA for any clinical reason or in strains isolated from severe diseases, it is advisable to use both tests and also detect the presence of the mecA and mecC genes.