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Article

Clonal Complexes Distribution of Staphylococcus aureus Isolates from Clinical Samples from the Caribbean Islands

by
Stefan Monecke
1,2,3,*,
Patrick Eberechi Akpaka
4,
Margaret R. Smith
4,
Chandrashekhar G. Unakal
4,
Camille-Ann Thoms Rodriguez
5,
Khalil Ashraph
4,
Elke Müller
1,2,
Sascha D. Braun
1,2,
Celia Diezel
1,2,
Martin Reinicke
1,2 and
Ralf Ehricht
1,2,6
1
Leibniz Institute of Photonic Technology (IPHT), 07745 Jena, Germany
2
InfectoGnostics Research Campus, 07743 Jena, Germany
3
Institute for Medical Microbiology and Virology, Dresden University Hospital, 01307 Dresden, Germany
4
Department of Para-Clinical Sciences, Faculty of Medical Sciences, St. Augustine Campus, The University of the West Indies, St. Augustine, Trinidad and Tobago
5
Department of Microbiology, Faculty of Medical Sciences, Mona Campus, The University of the West Indies, Kgn7, Kingston, Jamaica
6
Institute of Physical Chemistry, Friedrich-Schiller University, 07743 Jena, Germany
*
Author to whom correspondence should be addressed.
Antibiotics 2023, 12(6), 1050; https://0-doi-org.brum.beds.ac.uk/10.3390/antibiotics12061050
Submission received: 17 May 2023 / Revised: 9 June 2023 / Accepted: 13 June 2023 / Published: 14 June 2023
Browse Figures
Versions Notes

Abstract

:
The aim of this study was to comprehensively characterise S. aureus from the Caribbean Islands of Trinidad and Tobago, and Jamaica. A total of 101 S. aureus/argenteus isolates were collected in 2020, mainly from patients with skin and soft tissue infections. They were characterised by DNA microarray allowing the detection of ca. 170 target genes and assignment to clonal complexes (CC)s and strains. In addition, the in vitro production of Panton–Valentine leukocidin (PVL) was examined by an experimental lateral flow assay. Two isolates were identified as S. argenteus, CC2596. The remaining S. aureus isolates were assigned to 21 CCs. The PVL rate among methicillin-susceptible S. aureus (MSSA) isolates was high (38/101), and 37 of the 38 genotypically positive isolates also yielded positive lateral flow results. The isolate that did not produce PVL was genome-sequenced, and it was shown to have a frameshift mutation in agrC. The high rate of PVL genes can be attributed to the presence of a known local CC8–MSSA clone in Trinidad and Tobago (n = 12) and to CC152–MSSA (n = 15). In contrast to earlier surveys, the USA300 clone was not found, although one MSSA isolate carried the ACME element, probably being a mecA-deficient derivative of this strain. Ten isolates, all from Trinidad and Tobago, were identified as MRSA. The pandemic ST239–MRSA–III strain was still common (n = 7), but five isolates showed a composite SCCmec element not observed elsewhere. Three isolates were sequenced. That showed a group of genes (among others, speG, crzC, and ccrA/B-4) to be linked to its SCC element, as previously found in some CC5– and CC8–MRSA, as well as in S. epidermidis. The other three MRSA belonged to CC22, CC72, and CC88, indicating epidemiological connections to Africa and the Middle East.

1. Introduction

Staphylococcus aureus, a ubiquitous bacterium, is a common cause of hospital- and community-associated infections in humans around the world [1,2,3,4,5]. Bacterial infections caused by methicillin-resistant S. aureus (MRSA) have become a serious global healthcare problem [6,7]. Aside from resistance, which limits options for treatment, another cause for concern is its continuous evolution and global spread of emerging and/or virulent clones [1]. Indeed, MRSA strains are associated with a number of widespread or even pandemic lineages. To describe these lineages, clonal complexes (CCs) based on multilocus sequence typing (MLST; [8]) are identified. The classification of CCs is based on the sequencing of seven ubiquitous housekeeping genes and the analysis of their sequence variations [8]. In addition, Staphylococcal cassette chromosome mec (SCCmec) elements can be assigned to distinct types [9,10]. These are large mobile genetic elements that carry mecA or mecC genes, responsible for methicillin/beta-lactam resistance—thereby defining MRSA [11]—as well as other resistance and/or virulence-associated markers. Methicillin-resistant S. aureus infections are among the most challenging infection prevention and control issues, particularly in hospitals. Hospital and other healthcare-related infections are frequently severe and can be fatal [1]. Apart from hospital-acquired MRSA infections (HA–MRSA), community-acquired MRSA (CA–MRSA) infections are emerging as a human health problem in many countries and have been reported in people who have had little or no previous contact with healthcare systems [12,13,14,15,16,17]. Despite being—in many cases—more susceptible to antibiotics other than beta-lactams, CA–MRSA infections have been detected in hospitals and are responsible for a large percentage of hospital-onset MRSA infections [18,19,20,21,22]. Furthermore, these CA–MRSA strains have been reported to be more virulent than some HA–MRSA strains. This is usually attributable to the presence of Panton–Valentine leukocidin (PVL) [5,17,23,24,25,26]. This is a pore-forming bicomponent toxin with high specificity to human leukocytes. It is associated with severe, chronic, or recurrent skin and soft tissue infections as well as with highly lethal but rare necrotising pneumonia. The PVL genes (lukF–PV and lukS–PV) are localised on prophages, and thus, they can horizontally be transferred across different strains and lineages of S. aureus [27,28,29,30].
The knowledge on S. aureus population structure and circulating MRSA clones for Caribbean islands is limited, with few published studies discussing a rather low number of typed isolates. On Francophone islands (Guadeloupe and Martinique), MRSA strains were observed that were also common in France (CC5 “Geraldine and CC8 “Lyon” clones as well as PVL-positive CC80–MRSA–IV; [31,32]). Regarding MSSA, several lineages were identified, including CC5, CC7, CC152, CC188, and CC398 [32]. A study from St. Kitts and Nevis showed high rates of the USA300/ST8–MRSA–IV (PVL+/ACME+) strain [33]. This strain was also observed in Cuba [34], alongside ACME negative, PVL-positive CC8–MRSA–IV and CC72–MRSA–V in hospitals [35] as well as other CC8–MRSA–IV and CC5–MRSA–IV in livestock [36]. In Barbados, high rates of PVL-positive S. aureus and rather high MRSA rates were observed [37]. A study from Haiti revealed a presence of CC5–MRSA–II and -IV clones of CC72–MRSA–IV as well as of various MSSA lineages, including CC1, CC5, CC8, CC15, CC45, CC72, and, notably, PVL-positive CC152 [38]. In a study from the Dominican Republic [32], CC5–, CC30–, and CC72–MRSA predominated, while PVL-positive CC30–MSSA was the dominant strain among a variety of MSSA lineages.
In Trinidad and Tobago, most S. aureus strains identified during previous studies were methicillin-susceptible S. aureus (MSSA) that were assigned to various CCs [39]. Virulent community-acquired MSSA is a cause for concern as PVL genes are common, and thus they pose an interesting issue for investigation. This follows a confirmed case of fatal multi-organ failure involving a young, previously healthy child that has been documented in the literature [40]. Among MRSA, the HA–MRSA strain ST239–MRSA–III was most prevalent, with other clones such as the CC5–MRSA–II being sporadically identified [41]. Further research on MRSA strains by Akpaka et al. [42] revealed the existence of a pulse-field gel electrophoresis (PFGE) banding pattern similar to that of a Canadian strain, CMRSA–6 (corresponding to a variant of ST239). In that study, all 60 isolates were PVL-negative [42]. In Trinidad and Tobago, an increase in the emergence of CA–MRSA infections has been reported, with prevalence rising from 4.1% to 8.1% between 1999 and 2004 [43]. The emerging CA–MRSA clone USA300/ST8–MRSA–IV (PVL+/ACME+) was also identified [41]. Available data suggest that the prevalence of MRSA-related infections appears to be increasing in Trinidad, Tobago, and Jamaica [31,44,45]. In Trinidad and Tobago, a prevalence rate of 4.6% was reported by Swanston in 1995 [46]. In 2006, a 12.8% prevalence rate was reported by Akpaka et al. [47], while Orrett [43] reported a prevalence of 20.8% in the same year.
In Jamaica, the prevalence of MRSA has continued to increase since the identification of the first case at the University Hospital of the West Indies in 1988 [48]. Reports emanating from Jamaica show that MRSA has fairly remained very low in prevalence, with 4% (2004), 5% (2005), and 7% in 2008 [44,45]. This is even lower at the teaching hospital where of 7304 clinical isolates analysed, 689 were identified as S. aureus, with only 31 (4.5%) proved to be methicillin-resistant in 2017 (unpublished data). This is comparable to the 3% prevalence found in 2013. In Jamaica, commonly identified CCs include ST8–MRSA–IV, USA300, and ST5/ST225–MRSA–II, New York–Japan clone [31].
In general, knowledge of the population structure of S. aureus/MRSA on the Caribbean islands is poor, and changes to it might remain unnoticed. In order to address this, DNA microarray-based analysis was used in this study to classify and assign clinical S. aureus isolates from Trinidad and Tobago, and Jamaica into clonal complexes, strains, and SCCmec types. In addition, the presence and expression of PVL were studied.

2. Results

2.1. Analysis of Clinical Isolates

Just over half of the specimens analysed from Trinidad and Tobago (48/85; 57%) were recovered from wound swabs. The remaining isolates were recovered from blood (12/85; 14%), pus (7/85; 8%), urine (8/85; 9%), ear swabs, vulvar swabs, peritoneal swabs, joint fluid, eye swabs, and, in one case, from an undocumented specimen (10/85; 12%). Most of the Jamaican isolates (13/16; 81%) were from wounds, while the remaining isolates were recovered from a throat swab (1/16; 6%) and blood (2/16; 13%).
Table 1 and Table 2 show the specimen source distribution of MSSA, MRSA, and S. argenteus isolates from both islands. Table 3 shows the age distribution of patients infected with MSSA, MRSA, and S. argenteus strains from Trinidad and Tobago. Patients aged 30 to 39 years had the highest rate of S. aureus infections (22%; 19/85). Of the 19 patients, 95% of infections were caused by MSSA strains. MRSA accounted for one infection (5%) in this group. The second group of patients that frequently experienced infections were those in the paediatric group (0 to 9 years) and also those between 10 and 19 years of age. Both groups had 18% of patients being infected. In these groups, MRSA accounted for 13% (2/15) and 7% (1/15) of infections, while MSSA accounted for 80% (12/15) and 93% (14/15) of infections, respectively. MSSA infections were found in 92% of patients over the age of 60, while the remaining 8% were related to MRSA. S. argenteus infections were found in two patients, ages 6 and 45 years.
Data from Table 4 showed that males (n = 46) more commonly presented with staphylococcal infections than women. MSSA infections were also most prevalent in both males and females as opposed to MRSA, with 89% (41/46) occurring in males and 81% (30/37) in females. MRSA infections were found in 9% (4/46) of male patients and 16% (6/37) of female patients. S. argenteus isolates accounted for 2% (1/46) of infections in males and 3% (1/37) in females.

2.2. Distribution of S. aureus Clonal Complexes and Strains

High clonal diversity was reported from Trinidad and Tobago, as S. aureus isolates were assigned to twenty different clonal complexes and 83 strains comprising both MRSA and MSSA (Table 5). Two additional isolates were identified as S. argenteus, CC2596. The most prevalent CC identified was CC8 (15 isolates), followed by CC152 (14 isolates). Other CCs included CC97, CC6, and CC239, which comprised the majority of MRSA. The remaining CCs were rare, comprising five or fewer isolates each. All 16 isolates (100%) from Jamaica were MSSA and distributed across eight different CCs. CC1 (four isolates) and CC6 (three isolates) were the most preventable among these isolates; CC152 was also found, but CC8 was not identified. However, the numbers are too low to assess the population structure of S. aureus/MSSA on this island.
The overall distribution of CCs from both islands, the various strains identified, as well as results for the resistance and virulence markers, SCCmec elements, and toxins examined can be found in the Supplemental File S1 attached, and summarized in Table 5.
Most of the strains from Trinidad and Tobago were MSSA (73/85; 86%), and two were methicillin-susceptible S. argenteus. All isolates from Jamaica were MSSA (16/16; 100%).
Of the 85 clinical isolates from Trinidad and Tobago, only ten (10/85; 12%) strains were identified as methicillin-resistant S. aureus (Table 5). The majority (7/10; 70%) belonged to CC239, while the three remaining strains were categorized as CC22, CC72, and CC88. There were no MRSA strains isolated from Jamaica.

2.3. Observations Regarding Individual Clonal Complexes of S. aureus

Four isolates from Jamaica and one from Trinidad and Tobago belonged to CC1. All were MSSA, all lacked the SCC-borne fusidic-acid resistance gene fusC, and all were PVL-negative. All carried the enterotoxin genes seh, sek + seq, and, in addition, all Jamaican isolates were also positive for the toxic shock syndrome toxin gene tst1, as well as for the enterotoxin genes sec and sel.
Three MSSA isolates from Trinidad and Tobago were assigned to CC5. Two of them carried, in addition to PVL, the edinA gene encoding an epidermal cell differentiation inhibitor.
PVL-positive as well as PVL-negative CC6–MSSA were found in Trinidad and Tobago as well as in Jamaica. Six isolates from this CC harboured PVL genes; five were positive for the enterotoxin A gene sea.
CC7 was represented by five MSSA isolates from Trinidad and Tobago. All were PVL-negative but harboured a sea allele as known from N315 (BA000018.3; pos. 2,011,380 to 2,012,153), also known as enterotoxin P or sep.
All CC8 isolates originated from Trinidad and Tobago; not a single one was recovered from Jamaica. Twelve isolates belonged to a previously noticed CC8–MSSA that harboured PVL genes, enterotoxin genes sek and seq, as well as (in 11/12) also sed, sej and ser. Both sequenced isolates showed sed, sej, and ser to be located on the same contig as blaZ + blaI + blaR together with plasmid genes and a cadmium resistance operon. A single isolate out of these twelve genotypically PVL-positive isolates was negative for PVL production, as discussed below. Another two CC8–MSSA isolates were negative for PVL and enterotoxin genes.
CC8–MRSA were not noted, neither “North American” (ACME-positive) nor “South American (ACME-negative/mer-operon-positive) USA300 strains. However, one additional PVL-positive isolate carried ACME genes, the SCC-associated copper resistance gene copA2–SCC, opp3B, opp3C, adhC, and speG, but lacked mecA as well as all genes associated with SCCmec IV. This suggests that it might have been a mecA-deficient derivative of the North American USA300 strain.
A Clonal Complex 22 MRSA isolate was retrieved from a patient presenting with cellulitis/trauma to the left foot. It was also the only isolate assigned to this common and widespread lineage and the only PVL- and tst1- (toxic shock syndrome toxin 1) positive MRSA identified. It harboured various genes associated with SCCmec, which encodes methicillin resistance. These include ugpQ, mecA, the truncated methicillin resistance operon repressor 1, ccrA/B-2, and Q9XB68dcs. Subtyping by an additional array [49] identified the SCCmec element as SCCmec IVa.
A total of three CC72 isolates were identified; however, only one was methicillin-resistant. This was a PVL-negative strain with a composite SCCmec VT element comprising ugpQ, mecA, and ccrC genes that also included the fusidic acid resistance gene fusC (=Q6GD50). The probe for D1GU38, a marker that accompanies the second copy of ccrC in SCCmec VT, yielded a signal indicating that the composite element derived from SCCmec VT rather than V. The other two CC72 isolates were MSSA that lacked PVL but carried enterotoxin genes sec and sel.
A CC88–MRSA–IV was the only isolate of this lineage collected from a patient with a vulval abscess. As it carried a SCCmec IVa (MW2-like) element, this observation suggested an African connection. Except for the beta-lactamase operon blaZ/I/R, no other resistance genes were detected. Neither PVL nor enterotoxin or exfoliative toxin genes were detected.
Sixteen isolates (including two from Jamaica) belonged to CC152. All were MSSA, but 13 harboured the penicillinase operon. A total of 15 out of 16 were positive for PVL genes, and these 15 also yielded phenotypically detectable PVL. In addition, all were positive for the edinB gene.
CC239 comprised seven CC239–MRSA–III isolates. The majority (n = 5) of CC239 isolates carried a complex SCC [mec III + speG + Cd/czrC + ccrAB4 + ccrC] element. Three of these isolates were sequenced (see below). Four isolates from this cluster also harboured a mercury resistance operon that, however, in two sequenced isolates, was plasmid-borne rather than SCC-associated.
The other two CC239 isolates carried SCC [III + SCCmer + ccrC] elements but lacked czrC, speG, and the additional recombinase genes. Four of the seven isolates (representing both strains) were tested for sasX = sesI, and all were positive in accordance with an affiliation to the “Southeast Asian Clade” of CC239–MRSA–III.
The remaining Clonal Complexes, CC9, CC12, CC15, CC30, CC59, CC101, CC121, and CC188, accounted for sporadic PVL- and mecA-negative isolates. Details are provided in Table 5 and Supplemental File S1.

2.4. Observations Regarding S. argenteus

Two isolates were assigned to S. argenteus. They yielded signals for agr III and capsule type 5 alleles, harboured cna but lacked the egc enterotoxin gene cluster as the genome sequence of H115100079; GenBank CCEP/SAMEA1557135 does. Thus, they were assigned to CC2596. Both isolates lacked PVL genes, and any resistance or enterotoxin genes were covered by the array.

2.5. Detection of PVL

Among isolates from Trinidad and Tobago (Figure 1), PVL genes were common, albeit no MRSA and no S. argenteus with these genes were identified. Thirty-two out of 73 (44%) MSSA isolates harboured lukF/S–PV genes. PVL genes were found in CC5, CC6, CC8, and CC152, with CC8 and CC152 being the dominant lineages among PVL positives (thirteen isolates each). Of these isolates, CC8 and CC152 were the largest contributors of PVL, with thirteen PVL-positive strains each. However, the CC8 strain commonly found in Trinidad and Tobago was not found among the Jamaica isolates. PVL-positive isolates from that island belonged to CC6 and CC152.
While thirty-two isolates carried lukF/S–PV, only thirty-one were found to be phenotypically positive for LukF–PV production by the lateral flow. Thus, the lateral flow assay—compared to genotyping—yielded a sensitivity of 96.9%, a specificity of 100%, a positive predictive value of 100%, and a negative predictive value of 98.6%. The one genotypically positive but phenotypically negative isolate (a CC8–MSSA; 2020-042_7641M) was re-cultured and re-tested, but the results remained unchanged. It was then subjected to genome sequencing, in parallel to a pheno- and genotypically PVL-positive isolate of the same strain, in order to find a reason for the discrepant results. It showed a frameshift mutation in agrC because of a deletion of a single nucleotide (see Supplemental File S2, 2020-042_7641M chromosome, positions 2,055,453 to 2,056,744; whereas agrC of a phenotypically PVL positive control can be found at Supplemental File S2, 2020-043_7352M, chromosome, pos. 2,099,143 to 2,100,435).
The other agr genes (agrA, agrB, and agrD) and hld were inconspicuous (for an alignment to the sequences of reference strain NCTC8325 and PVL-producing 2020-043_7352M, see Supplemental File S3), as were the lukF–PV and lukS–PV genes.

2.6. Sequencing the Composite SCCmec Element in Clonal Complex 239 Isolates

Three CC239 isolates (2020-021_7037M, 2020-048_8421A, and 2020-009_371M) were sequenced (Supplemental File S2) to characterise the novel composite SCCmec element. It encompassed approximately 67,500 base pairs. Its gene content is summarised in Table 6, and a graphical overview is provided in Figure 2.
It comprised, directly adjacent to orfX, a gene encoding a type I restriction–modification system site-specificity determinate, hsdS, followed by a truncated transposase gene, the spermidine N-acetyltransferase gene speG, five genes encoding “putative proteins” (one of which was present in two copies), and recombinase genes ccrA/B-4. These are followed by a truncated ccr-associated cassette chromosome helicase gene (cch), yet another gene encoding a “putative protein,” as well as by yozA (HTH-type transcriptional repressor) and czrC (cadmium and zinc resistance gene C, formerly known as cadA or copA; [50]).
The remaining part of the composite SCCmec III element of the Trinidad and Tobago strain was essentially identical to the corresponding part of the SCCmec element of the Southeast Asian Clade CC239 strain TW20, FN433596.1:(34140 to 48481) and in CMRSA-6 (CP027788.1). Besides the mec element (including mecA, mecI, mecR2 and mecR1, psmMEC, ydeM, ugpQ, and the dru region) and recombinase genes ccrA/B-3 as well as ccrAA/C, it harboured the aminoglycoside resistance gene ant9 and the macrolide/clindamycin resistance gene erm(A) as well as a cadmium-resistance operon (cadC, cadA, cadD).
Contrarily to TW20 and CMRSA-6, where the mercury resistance operon is localised on the SCCmec element, it was plasmid-borne in two of the three sequenced strains, and absent in the third one. When present, it was accompanied by yet another set of cadmium resistance genes and by quaternary ammonium compound resistance markers (qacA/R).
In one of the three isolates sequenced (2020-009_371M), a region comprising roughly 27,000 base pairs flanked on both sides by multiple transposase genes was inverted in order and orientation. It contained the mec element, the cadmium, and cstR/A/B–SCC operons, as well as ant9 and erm(A).
Table
Table 6. SCCmec III composite elements in three CC239 isolates from Trinidad and Tobago.
Table 6. SCCmec III composite elements in three CC239 isolates from Trinidad and Tobago.
Gene IDGene Product/ExplanationPosition in SCC of 2020-021_7037MPosition in SCC of 2020-048_8421AOrientation in
2020-021_7037M and 048_8421A		Position in SCC of 2020-009_371MOrientation in 2020-009_371MPresent in ATCC1228, M1, etc.
DR-SCCdirect repeat of SCC1 to 191 to 19n/a *1 to 19n/a-
SCCterm07terminus of SCC towards orfX20 to 12220 to 122n/a20 to 122n/aX **
hsdStype I restriction-modification system site-specificity determinate256 to 1458256 to 1458forward256 to 1458forwardX
tnp trnc.transposase for IS12721513 to 17121513 to 1712trnc.1513 to 1712trnc.X
speGspermidine N-acetyltransferase1781 to 22781781 to 2278rev. compl.1781 to 2278rev. compl.X
A9UFT0LPXTG protein homologue2531 to 27532531 to 2753rev. compl., trnc., frameshift2531 to 2753rev. compl., trnc., frameshiftX
PF11070putative PF11070 family protein2950 to 33602950 to 3360rev. compl.2950 to 3360rev. compl.X
A9UFT0LPXTG protein homologue3523 to 37433523 to 3743rev. compl.3523 to 3743rev. compl.X
Q9KX75putative protein3758 to 42613758 to 4261rev. compl.3758 to 4261rev. compl.X
Q7A207putative protein4277 to 45884277 to 4588rev. compl.4277 to 4588rev. compl.X
Q7A206putative protein4675 to 50254675 to 5025rev. compl.4675 to 5025rev. compl.X
UTR_ccrB-4conserved 3’-untranslated region of ccrB5026 to 55255026 to 5525n/a5026 to 5525n/aX
ccrB-4cassette chromosome recombinase B, type 45526 to 71545526 to 7154rev. compl.5526 to 7154rev. compl.X
ccrA-4cassette chromosome recombinase A, type 47151 to 85127151 to 8512rev. compl.7151 to 8512rev. compl.X
cchcassette chromosome helicase8699 to 93348699 to 9334rev. compl., trnc.8699 to 9335rev. compl., trnc.X
D2N398putative protein9787 to 10,1469787 to 10,146rev. compl.9787 to 10,146rev. compl.X
yozAHTH-type transcriptional repressor10,353 to 10,67910,353 to 10,679forward10,353 to 10,679forwardX
czrCcadmium and zinc resistance gene C11,000 to 12,93411,000 to 12,934forward11,000 to 12,934forwardX
SCCterm 02terminus of SCC towards orfX13,941 to 14,25713,941 to 14,257n/a13,941 to 14,257n/a-
Q2FKL3HNH endonuclease family protein14,258 to 14,62414,258 to 14,624trnc., frameshift14,258 to 14,624trnc., frameshift-
D1GU38putative protein14,689 to 15,55214,689 to 15,552forward14,689 to 15,552forward-
D2N370putative protein15,660 to 17,13415,660 to 17,134forward15,660 to 17,134forward-
Q4LAG3putative protein17,361 to 18,46117,361 to 18,461forward17,361 to 18,461forward-
Q3T2M7putative protein18,454 to 18,82518,454 to 18,825forward18,454 to 18,825forward-
ccrAAcassette chromosome recombinase “AA”18,822 to 20,46518,822 to 20,465forward18,822 to 20,465forward-
ccrCcassette chromosome recombinase C20,690 to 22,29220,690 to 22,292forward, trnc.20,690 to 22,292forward, trnc.-
tnp_IS200transposase of IS20022,423 to 22,90822,423 to 22,908forward22,422 to 22,907forward-
ccrCcassette chromosome recombinase C23,030 to 23,11123,030 to 23,111forward, trnc.23,029 to 23,110forward, trnc.-
Q4LAF9putative protein23,200 to 23,53823,200 to 23,538forward23,199 to 23,537forward-
Q7A206putative protein23,544 to 23,63023,544 to 23,630forward, trnc.23,543 to 23,629forward, trnc.-
Q7A207putative protein23,632 to 23,94323,632 to 23,943forward23,631 to 23,942forward-
Q9KX75putative protein23,959 to 24,46523,959 to 24,465forward23,958 to 24,464forward-
A5INT3putative protein24,486 to 24,80324,486 to 24,803forward24,485 to 24,802forward-
tnpA_Tn554transposase A of transposon Tn55424,922 to 26,00724,922 to 26,007forward24,921 to 26,006forward-
tnpB_Tn554transposase B of transposon Tn55426,004 to 27,89626,004 to 27,896forward26,003 to 27,895forward-
tnpC_Tn554transposase C of transposon Tn55427,903 to 28,28027,903 to 28,280forward27,902 to 28,279forward-
ant9adenyltransferase AAd928,431 to 29,21328,431 to 29,212forward54,251 to 55,033rev. compl.-
erm(A)rRNA adenine N-6-methyltransferase29,339 to 30,07029,338 to 30,069rev. compl.53,394 to 54,125forward-
lp_erm(A)leader peptide of erm(A)30,128 to 30,18730,127 to 30,186rev. compl.53,277 to 53,336forward-
Q9KX74putative methyltransferase30,579 to 31,24130,578 to 31,240forward52,223 to 52,885rev. compl.-
Q4W1I0putative DNA binding regulator31,789 to 32,66131,788 to 32,660forward50,803 to 51,675rev. compl.-
D1GU55putative membrane protein32,709 to 33,00832,708 to 33,007forward50,456 to 50,755rev. compl.-
D1GU56putative protein33,024 to 33,51233,023 to 33,511forward49,952 to 50,440rev. compl.-
Q93IA1putative membrane protein33,647 to 34,17433,646 to 34,173forward49,290 to 49,817rev. compl.-
Q9KX75putative protein34,753 to 35,10534,752 to 35,104forward trnc.48,358 to 48,711rev. compl., trnc., frameshift-
A9UFT0LPXTG protein homologue35,119 to 35,34035,118 to 35,339forward48,123 to 48,344rev. compl.-
D1GU60putative protein35,490 to 36,05635,489 to 36,055forward47,407 to 47,973rev. compl.-
hsdR-SCCtrnc. fragment of hsdR36,136 to 38,34936,135 to 38,348rev. compl. trnc.45,114 to 47,327forward, trnc.-
IR_IS431inverted repeat of IS43138,352 to 38,36738,351 to 38,366n/a45,096 to 45,111n/a-
Q7A213putative protein38,352 to 38,37938,351 to 38,378forward trnc. frameshift45,084 to 45,111rev. compl., trnc., frameshift-
tnp_IS431transposase for IS43138,411 to 39,08538,410 to 39,084rev. compl.44,378 to 45,052forward-
IR_IS431inverted repeat of IS43139,116 to 39,14939,115 to 39,148trnc.44,322 to 44,337trnc.-
Teg143trans-encoded RNA associated with tnpIS43139,126 to 39,14139,125 to 39,140n/a44,314 to 44,347n/a-
mvaS-SCCtrnc. 3-hydroxy-3-methylglutaryl CoA synthase39,158 to 39,51039,157 to 39,509forward, frameshift43,953 to 44,305rev. compl., frameshift-
Q5HJW6putative protein39,608 to 39,91139,607 to 39,910forward trnc.43,552 to 43,855rev. compl., trnc.-
druSCC direct repeat units39,748 to 40,30539,747 to 40,304n/a43,158 to 43,715n/a-
ugpQglycerophosphoryl diester phosphodiesterase40,507 to 41,25040,506 to 41,249forward42,213 to 42,956rev. compl.-
ydeMputative dehydratase41,347 to 41,77541,346 to 41,774forward41,688 to 42,116rev. compl.-
mecApenicillin-binding protein 2a41,821 to 43,82741,820 to 43,826rev. compl.39,637 to 41,642forward-
mecR1methicillin resistance operon repressor 143,927 to 45,68443,926 to 45,683forward37,779 to 39,537rev. compl.-
mecImethicillin resistance regulatory protein45,684 to 46,05545,683 to 46,054forward37,408 to 37,779rev. compl.-
psmMECphenol-soluble modulin from SCCmec46,140 to 46,20846,139 to 46,207rev. compl.37,255 to 37,323forward-
mecR2methicillin resistance operon repressor 246,528 to 47,67646,527 to 47,675forward35,786 to 36,935rev. compl.-
cstB-SCCCsoR-like sulphur transferase-regulated gene B47,790 to 49,12447,789 to 49,123rev. compl.34,338 to 35,672forward-
cstA-SCCCsoR-like sulphur transferase-regulated gene A49,156 to 50,22049,155 to 50,219rev. compl.33,242 to 34,306forward-
cstR-SCCcopper-sensing transcriptional repressor50,356 to 50,61650,355 to 50,615forward32,846 to 33,106rev. compl.-
DUF81-SCCputative sulfite/sulfonate efflux50,616 to 51,25950,615 to 51,258forward32,203 to 32,846rev. compl.-
cadD_R35cadmium transport protein D51,527 to 52,14451,526 to 52,143rev. compl. frameshift31,318 to 31,935forward-
cadA_Tn554cadmium efflux adenosine triphosphatase52,225 to 54,63952,224 to 54,638rev. compl.28,823 to 31,237forward-
cadC_Tn554putative regulator of cadmium efflux54,632 to 54,99754,631 to 54,996rev. compl.28,465 to 28,830forward-
tnpC_Tn554transposase C of transposon Tn55455,183 to 55,56155,182 to 55,559rev. compl.55,184 to 55,561rev. compl.-
tnpB_Tn554transposase B of transposon Tn55455,568 to 57,46055,566 to 57,458rev. compl.55,568 to 57,460rev. compl.-
A5INT3putative protein57,655 to 57,97857,653 to 57,976rev. compl.57,655 to 57,978rev. compl.-
D1GUI6putative protein57,971 to 58,17757,969 to 58,175rev. compl.57,971 to 58,177rev. compl.-
Q9KX75putative protein58,179 to 58,70058,177 to 58,698rev. compl.58,179 to 58,700rev. compl.-
Q0P7G0putative protein58,719 to 59,03058,717 to 59,028rev. compl.58,719 to 59,030rev. compl.-
Q93IE0putative protein59,115 to 59,46559,113 to 59,463rev. compl.59,115 to 59,465rev. compl.-
ccrB-3cassette chromosome recombinase B, type 359,935 to 61,56259,933 to 61,560rev. compl.59,936 to 61,563rev. compl.-
ccrA-3cassette chromosome recombinase A, type 361,583 to 62,92961,581 to 62,927rev. compl.61,584 to 62,930rev. compl.-
D1GUJ2putative protein63,122 to 63,39763,120 to 63,395rev. compl.63,123 to 63,398rev. compl.-
cchcassette chromosome helicase63,487 to 65,27463,485 to 65,272rev. compl.63,488 to 65,275rev. compl.-
DUF1413putative protein associated with ccr65,274 to 65,56165,272 to 65,559rev. compl.65,275 to 65,562rev. compl.-
Q2FKL7putative protein65,695 to 66,74465,693 to 66,742forward65,696 to 66,745forward-
Q933A2putative ADP-ribosyltransferase66,797 to 67,36966,795 to 67,367forward66,798 to 67,370forward-
DR-SCCdirect repeat of SCC67,459 to 67,47767,457 to 67,475n/a67,460 to 67,478n/a-
* n/, not applicable. Non-coding regions. ** Genes marked with ”X” are present in sequences of ATCC1228 and M1.
Antibiotics 12 01050 g002 550
Figure 2. Schematic representation of a part of the SCC element in S. epidermidis ATCC12228 (GenBank AE015929.1; positions 51,506 to 66,000) and the SCCmec elements in CMRSA-6 (GenBank CP027788.1) as well as the three sequenced CC239 study strains.
Figure 2. Schematic representation of a part of the SCC element in S. epidermidis ATCC12228 (GenBank AE015929.1; positions 51,506 to 66,000) and the SCCmec elements in CMRSA-6 (GenBank CP027788.1) as well as the three sequenced CC239 study strains.
Antibiotics 12 01050 g002

2.7. The sasX = sesI Gene in the Clonal Complex 239 Sequences

The sasX = sesI gene encoding an LPxTG motif “surface-anchored protein X” [51] was accompanied, likewise in all three sequences, by several copies of transposase genes, genes encoding integrases, holins, exonucleases, and amidases, as well as by the aminoglycoside resistance genes aacA–aphD, aphA3, and the streptothricin resistance gene sat. This region encompassed as many as roughly 127,000 bp and is integrated into yeeE = DUF395 (“SAUR2215 (SAR_RS11075)”; see https://pubmlst.org, accessed on 16 May 2023). This is the same constellation as in TW20 ([52]; FN433596, pos. 2,180,899 to 2,309,183) and in CMRSA-6 (CP027788.1).

3. Discussion

The DNA microarray analysis approach, along with MLST and SCCmec typing, provided a comprehensive characterization and assignment of all isolates into clonal complexes and strains. Some clinically useful data with respect to antimicrobial resistance, virulence, and toxin gene carriage were also revealed. Results confirmed a high diversity of S. aureus clonal complexes from Trinidad and Tobago, with CC8 being the most prominent. While most of the infections in Trinidad and Tobago were caused by MSSA (73/85; 86%), all were caused by MSSA in Jamaica. Although the sample size from both islands was relatively small, most of the findings were consistent when compared to previous studies conducted on S. aureus isolates from both islands on much larger sample sizes. In the present study, most of the S. aureus infections occurred in patients with wound infections, mainly post-surgical in nature. Similar findings have been reported previously by several authors from Trinidad and Tobago [42,43,46,47,53,54] and Jamaica [45]. The exact reason for this occurrence is unknown; some authors have outlined possible explanations in reports from Trinidad and Tobago. Akpaka et al. [47] attributed the high levels of infection to excessive wound swabbing following medical procedures, and, in another report, noted that some surgical procedures can result in nosocomial infections with S. aureus as the main aetiological agent [54]. According to Orrett [43], the hands of health care providers may contribute to infection during dressing exercises, whereas Swanston [46] attributed the high usage of antibiotics to the increase in MRSA isolates from the surgical wards at the Port of Spain General Hospital. While any of the reasons outlined may be plausible as a contributory factor, it re-emphasizes the importance of implementing a strict infection control policy and applying guidelines for the prevention of surgical site infections in hospitals. This would include some form of multifaceted approach involving all team members to provide quality service before, during, and after surgical procedures.
Of the studies emanating from Trinidad and Tobago, Akpaka et al. [54] discovered a high prevalence of S. aureus infections in children aged 0 to 9. This high infection rate was attributed to an underdeveloped immune system and its inability to recognize staphylococcal components during infection at that age. Usually, older people tend to be more vulnerable to infections because aging is associated with immune dysfunction, multiple comorbidities, increased hospitalizations, and increased antibiotic use. Ramdass et al. [55] reported, at the Port of Spain General Hospital Trinidad, a peak age range of 60 to 69 years, in which 93% (14/15) of the MRSA-positive patients had used antibiotics (mainly beta-lactams) prior to admission into the hospital, had comorbidities (diabetes and hypertension), had long hospital stays (>1 week), were previously hospitalized and had previous surgery. In Trinidad and Tobago, most infections occurred among patients aged 30 to 39. This was followed by 0 to 9, 10 to 19 and finally patients over 60 years of age. Similar to the risk factors associated with infants and elderly, who are most often confined to nurseries and nursing homes, overcrowding may be a contributing factor to the high infection rate among the 10 to 39 age group. Persons in this age group frequently congregate in crowded areas of the community where the risk and exposure to infection are increased, such as correctional facilities, military/army camps, schools, and sports club settings. In Trinidad and Tobago, Orrett [53] outlined other major contributory factors that could be applied; these include the inappropriate use of antimicrobials and patients discontinuing therapy after being discharged due to the cost of prescriptions at local pharmacies. Most S. aureus infections in this study occurred in males from Trinidad and Tobago. Though not statistically significant, high S. aureus infection rates among males have been reported previously in other studies from the island [54,55]. According to Akpaka et al. [47], no obvious reason for the impact of gender on the prevalence of MRSA or MSSA in community or hospital settings has been reported in the literature. However, similar observations also have been made in other parts of the world.
Reports on the molecular characteristics and prevalence of MRSA in hospitals and within the community are constantly expanding in Trinidad and Tobago. The 12% MRSA prevalence observed herein was consistent with previously reported rates ranging from 9.8% to 15.3% [39,42,47,53,54,56], although, in 2018, Vire et al. [57] recorded the highest reported rate for the island, 44.4%. The most common MRSA strain was CC239–MRSA–III (8.3% of all S. aureus isolates, and 70% of MRSA). It has already been identified as the most prevalent clone in Trinidad and Tobago [41,54,56]. Until 2004, one variant of this strain (CMRSA-6) was the only MRSA clone circulating in Trinidad and Tobago [42]. According to previous work [58,59], CC239 with SCCmec III is a major dominant hospital-associated MLST type that has been described as the oldest truly pandemic MRSA strain in circulation since the 1970s and as the most successful international epidemic clone of MRSA. Its clade harbouring the virulence factor sasX/sesI is known to be widespread in Southeast Asia [51], but it was also, surprisingly, present in Trinidad and Tobago [59]. In this study, isolates were also tested positive for this gene. Sequencing revealed the localisation of sasX/sesI on a large mobile element, together with aminoglycoside genes (aacA–aphD and aphA3) and genes for phage enzymes. However, genes encoding phage structural proteins, such as those forming the capsid or tail, were not noted. Essentially the same complex can be found in TW20 (FN433596.1) and CMRSA-6 (CP027788.1), confirming the previous observation on the close relationship of the Trinidad and Tobago CC239 strains to the “South East Asian” Clade of CC239–MRSA–III and CMRSA-6 [42].
The Trinidad and Tobago variant of the “Southeast Asian” CC230–MRSA–III lineage, as described herein, harbours a composite SCCmec element including speG, czrC, and ccrA/B-4 recombinase genes in addition to its SCCmec III element. This variant has, to the best of our knowledge, exclusively been described from Trinidad and Tobago. Apparently, it has been extant there for at least 10 years (see [41]; when six out of seventy-six CC239 isolates collected in 2010 yielded array hybridisation signals for ccrA/B-4 genes).
The first 12,000 base-pairs of the SCC element of this strain are essentially identical to a “SCC–M1” element with speG and crzC that was found nearly years ago in two Irish epidemic CC8 strains, CC8–MRSA–[IIA/B/C/D/E + SCC–M1], “Irish AR13/14” and CC8–MRSA–[IVG/E + ccrAB4] (see [60] and GenBank HE858191.1, LS483301.1) and a Danish CC8–MRSA, (see [61] and GenBank HF937103.1). It was also identified in CC5, which includes MSSA with an SCC element harbouring speG, czrC, and ccrA/B-4 (GenBank CP053634.1), an MRSA strain from the US, where this element accompanies SCCmec II (see [62] and GenBank CP053636.1) and a Spanish epidemic MRSA strain in which it is linked to SCCmec IV (GenBank ASTH/SAMN02146299).
The speG, czrC, and ccrA/B-4 cluster or “SCC–M1” element might have been transferred into S. aureus from Staphylococcus epidermidis. To the best of our knowledge, the oldest strain in which that element can be found is ATCC12228 (see [63] and GenBank AE015929.1), which was isolated many decades ago [64]. In ATCC12228, it differs only in an apparently random integration of a transposase gene, and it is not linked to a SCCmec element but to an SCC element carrying, among other genes, heavy metal resistance genes and a second copy of speG. The speG, czrC, and ccrA/B-4 cluster is also present in several other sequences of S. epidermidis, including the one of strain ATCC14990 (GenBank CP035288.1), which was isolated in 1963 [65].
For two reasons, it might be speculated that the acquisition of this element might confer an evolutionary advantage. First, it recently appeared in several unrelated S. aureus strains in distant parts of the world. Second, in Trinidad and Tobago, it was noted in 6 out of 76 isolates collected in 2010, but in 5 out of 7 in 2020, indicating an increasing prevalence (with the caveat of low numbers). The gene crzC causes cadmium and zinc resistance [50], and it is frequently observed in livestock-associated MRSA [66], which might have benefited from resistance to formerly widely used zinc supplements to animal fodder. Whether the dermatological use of zinc-containing cremes and ointments might pose a selective pressure favouring this strain remains to be clarified. The speG gene, encoding a spermidine N-acetyltransferase, can also be found as part of ACME elements, such as in the USA300 strain and in composite SCCmec elements (see above and [67]). It has been associated with resistance to exogenous polyamines [68].
Similar to the CC239–MRSA–III, the rapidly emerging “USA300” CC8 (ST8–MRSA–IV) clone has been isolated previously in Trinidad and Tobago and appeared to be quite common [31,39,41,54,56]. This well-known pandemic CA–MRSA strain is common in various regions of the globe. A direct transfer of this strain from North American visitors was proposed as a reason for its high local prevalence [54], along with its emergence from the Caribbean/Latin American region [69]. However, in this study, no USA300 isolate was found. Only one CC8–MSSA isolates harboured both PVL and ACME in this study and was assumed to be a variant of “USA300” that lost its mecA/SCCmec IV element. Thus, it is tempting to speculate that the prevalence of this hypervirulent, multi-resistant clone in Trinidad and Tobago may be declining. The related but distinct “Spanish/Latin American USA300” CC8–MRSA–IV ([70], as represented by the genomes with GenBank accession numbers CP007670; CP007672), was also not detected despite geographical proximity.
Frequent domestic and international travel to Trinidad and Tobago has resulted in the discovery of several strains with global and regional connections. This study identified one CC88–MRSA–IVa strain, which has previously been reported in Africa and Australia [71]. The CC22–MRSA–IV (PVL+/tst1+) strain with a SCCmec IVa (MW2-like) element might indicate a Middle Eastern/Persian Gulf connection. It was observed in the Middle Eastern/Persian Gulf region and in Central Asia (see [72,73,74,75] as well as GenBank CP038850.1, from Pakistan). Another strain, CC72–MRSA–[VT + fusC], could also have been brought from there as composite SCCmec elements harbouring fusC are abundant in the Greater Middle East, and, indeed, similar or identical isolates have previously been observed from the UAE [76]. Findings of this nature should initiate a thorough investigation into a patient’s travel history, which should provide a clear indication of the strains’ possible origin. Moreover, a possible emergence of strains with composite SCCmec elements harbouring fusC should be closely monitored, as fusidic acid is commonly used in Trinidad and Tobago.
Another interesting observation is the high prevalence of PVL-positive S. aureus, reported consistently over the last decade with rates from 48% or 50% [39,77] to up to 62% [57]. In this study, the overall PVL prevalence for Trinidad and Tobago was lower, at 39%. CC8– and CC152–MSSA strains were the most common PVL-positive strains accounting for 15% and 14% of all Trinidad and Tobago isolates tested, with the former one apparently decreasing and the latter increasing compared to earlier studies [39,77]. The authors had already proposed an endemicity of the PVL-positive CC8–MSSA strains based on earlier observations [39], including the case of a severe and fatal infection in a previously healthy child [40]. Another common, endemic strain is PVL-positive CC152–MSSA. Interestingly, CC152 is an abundant lineage in Africa [78,79,80,81,82], and it was also observed in Haiti and Martinique [32,38]. Thus, it might be speculated that it was brought to the Caribbean islands together with people of African descent sometime in the history of colonisation. This might also apply to CC72. Since PVL-positive CC8– and CC152–MSSA has dominated Trinidad and Tobago for at least a decade [41], the rate of infection and possible patterns of evolution of these two clonal complex lineages will need to be closely monitored in the future.
While little information on PVL and MSSA is available for Jamaica, the 25% of PVL-positive MSSA strains identified should be monitored.
In Trinidad and Tobago’s literature, there are currently limited reports of S. argenteus strains. A low prevalence of S. argenteus strains to belong to CC2596 (2/85; 2.35%) was reported in this study, which is comparable with previous findings by Monecke et al. [39], where seven (7/294; 2.38%) S. argenteus strains were identified. When re-assessing hybridisation patterns of S. argenteus isolates from all Trinidad and Tobago studies by the authors, three can be assigned to CC2596 (23%, including the two from this study), three to CC1223 (23%) and seven to CC2250 (54%), but none to CC1850 (“ST75”, the longest known S. argenteus lineage). No S. argenteus isolate was found positive for mecA or PVL genes. Despite a low prevalence in both studies, S. argenteus should not be overlooked as this non-staphyloxanthin-producing strain [83], previously thought to be less virulent than S. aureus, is said to be becoming clinically important, with significant global prevalence and a virulence comparable to the one of S. aureus [84,85]. In the future, it is recommended that these strains should closely be monitored and reported [86]. The creation of a database within laboratories for the epidemiology, clinical impact, and implications for infection control of such isolates would be beneficial to combat potential outbreaks or increases in prevalence or virulence, given especially the observations of emerging PVL-positive [87] or methicillin-resistant S. argenteus [88,89]
Isolates in this study harboured a slew of resistance genes, virulence factors, and toxins. Despite this, all were vancomycin susceptible. This indicates that vancomycin remains the first-line treatment for (severe and/or bloodstream) infections with MRSA or with any S. aureus as long as susceptibility tests are pending, as previously reported from Trinidad and Tobago and Jamaica [44,47].
Unfortunately, with a strong local presence of virulent, PVL-positive strains in the community and the ongoing evolution of multidrug-resistant MRSA in healthcare settings, a need for vaccine development, ongoing surveillance, proper infection control, and reinforcement of preventative measures in both hospital and community settings, remains.

4. Materials and Methods

4.1. Study Design and Eligibility

This cross-sectional study was conducted using 101 clinical samples recovered from Trinidad and Tobago and Jamaica. Samples were collected from August to September 2020. All eligible subjects, regardless of ethnic group, gender, social status, or educational level, who agreed to participate by means of written consent and assent, were included in this study. This includes patients with varying clinical presentations who were diagnosed with various S. aurei infections such as furunculosis or carbuncles, as well as with cutaneous abscesses, mastitis, and other prominent and severe skin and soft tissue infections (SSTI; necrotizing fasciitis, chronically purulent and painful “spider bites”, particularly in cases with travel history) and recurrent or chronic SSTIs and necrotizing community-acquired pneumonia, including cases associated with influenza.

4.2. Laboratory Identification of Isolates

Samples were subjected to routine screening tests for the detection and isolation of S. aureus/argenteus. The clinical samples were cultured on mannitol fermentation salt agar at 37 °C for 24–48 h. Presumptive S. aureus was identified as gram-positive cocci isolates that produced yellow colonies with a yellow halo on mannitol salt agar. Colonies that were mannitol-salt-positive were conventionally identified as S. aureus based on colony morphology, Gram stain, haemolysis on sheep blood agar, catalase, and coagulase/latex agglutination tests.
Antibiotics susceptibility tests for sixteen antibiotics (including ampicillin, ampicillin + clavulanic acid, cefoxitin, ceftriaxone, cefuroxime, ceftazidime, ciprofloxacin, clindamycin, chloramphenicol, ertapenem, erythromycin, gentamicin, norfloxacin, penicillin, vancomycin, tetracycline) were routinely tested using the Kirby Bauer disc diffusion method on Mueller–Hinton agar in accordance with the Clinical and Laboratory Standards Institute (CLSI) guidelines. Cefoxitin 1 μg and oxacillin 30 μg antibiotic discs were used to screen for methicillin resistance. S. aureus strains ATCC 29213 and ATCC 25923 were used as controls.
All suspected S. aureus/argenteus samples were subjected to molecular testing using DNA microarray analysis as described below. This led to the exclusion of nine coagulase-negative Staphylococcus spec. isolates and the identification of two S. argenteus isolates, which were included in the analysis. An experimental lateral flow test was applied to all of these isolates to detect PVL expression (see below).

4.3. Microarray Analysis

The detection of virulence genes and resistance markers, as well as the assignment to clonal complexes, epidemic strains, and SCCmec types, was performed by microarray analysis using the StaphyType DNA microarray (Abbott [Alere Technologies GmbH], Jena, Germany) and the INTER-ARRAY Genotyping Kit S.aureus (Inter-Array GmbH, Bad Langensalza, Germany). The probes, primers, and procedures were previously described [2,49,90]. SCCmec subtyping and detection of sasX = sesI, using a second experimental array, was carried out on selected isolates as previously described [49]. In short, isolates were cultured overnight at 37 °C on Columbia blood agar. DNA was purified using Qiagen columns (Qiagen, Hilden, Germany) after enzymatic lysis of staphylococcal cells. The assay was based on a linear primer elongation that used one primer per target but amplified all targets simultaneously. During amplification, biotin-16-dUTP was incorporated into the single-stranded amplicons. After hybridisation to the DNA probes immobilised on the surface of the microarray, washing, and blocking, horseradish-peroxidase-streptavidin was conjugated. In case of a positive reaction, this conjugate bound to the biotin labels incorporated into the amplicons, causing in the next step a localised dye precipitation resulting in a visible and detectable formation. A transmission image of the microarray was recorded and analysed using a designated reader and software. This allowed the detection of individual target genes, as well as an automated comparison to a reference database facilitating assignment to CCs, strains, and SCCmec types [2,49,90].

4.4. Nanopore Sequencing

The Oxford Nanopore MinION platform was used to sequence the genomes of two MSSA isolates (2020-042_7641M, 2020-043_7352M) in order to investigate the lack of PVL production in the former. In addition, three CC239–MRSA (2020-009_371M, 2020-021_7037M, and 2020-048_8421A) were sequenced with the aim of describing their SCCmec elements.
The library preparation was performed using the 1D genomic DNA ligation kit (SQK-LSK109 with barcoding kit EXP-NBD104, and SQK-NBD114.24; Oxford Nanopore Technologies, Oxford, UK) following the manufacturer’s instructions for flow cells (FLO-MIN106 containing an R9.4.1 pore, and FLO-MIN114 containing an R10.4.1 pore). Prior to library preparation, a size selection was performed using AMPure-beads (Beckman Coulter, Krefeld, Germany) in a ratio of 1:1 (v/v) with the isolated DNA sample. The flow cell was loaded with a total of approximately 600 ng/µL DNA (according to Qubit4 Fluorometer; Thermo Fisher Scientific, Waltham, MA, USA). The sequencing ran for 72 h using MinKNOW software version 22.12.5, and 22.12.7 starting with a total of 1200–1600 active pores.
The guppy basecaller (version 6.4.6 + ae70e8f, Oxford Nanopore Technologies) was utilised to translate MinION raw reads (FAST5) into quality tagged sequence reads (4000 reads per FASTQ-file) using its barcode trimming option (model version: dna_r9.4.1_450bps_sup.cfg, and dna_r10.4.1_e8.2_400bps_sup). Flye (version 2.9.1-b1780) was used to assemble each strain’s quality tagged sequence reads into a complete, circular contig. Assemblies were polished in two steps. First, racon (v1.5.0) was iteratively used four times with the following parameters: match 8; mismatch 6; gap 8, and windows-lengths 500. Then, medaka (version 1.7.3) ran on the last racon-polished assembly using the model r941_min_sup_g507, and r10.4.1_e82_400bps_sup_g615. The resulting corrected assembly was used for further analysis.

4.5. PVL Lateral Flow Test

For the detection of PVL production, an experimental lateral flow assay (Senova, Weimar, Germany) was utilised as previously described [91]. In short, the assay relied on monoclonal antibodies targeting the LukF–PV protein. In order to test them, subcultured S. aureus isolates were incubated overnight or maximally up to 24 h at 37 ± 2 °C on Columbia Blood Agar. One inoculation loop (~10 µL) full of culture material was inoculated into 300 µL of the kit buffer and vortexed for 15–30 s in order to produce a homogenous suspension of cells. Then, the buffer with the inoculum was centrifuged at 2000× g for 30 s. A total of 100 µL of the supernatant was pipetted onto the sample well of the test device, and it was then incubated for 10 min at room temperature. The appearance of test and/or control lines was assessed visually, and the lateral flow device was photographed. The image of the test result was independently reviewed by two authors.

5. Conclusions

This study was conducted on 101 clinical S. aureus/argenteus isolates from Trinidad and Tobago and Jamaica. Samples were collected from August to September 2020. Ten isolates, all from Trinidad and Tobago, were identified as MRSA. The pandemic ST239–MRSA–III strain was still common (n = 7), but five of these isolates showed a novel composite SCCmec element in which a group of genes including speG, crzC, and ccrA/B-4 was linked to SCCmec III. The prevalence of PVL genes was high (in 38/101 isolates), although lower than in previous studies from Trinidad and Tobago. The USA300 PVL–MRSA strain was not found anymore, while the predominant PVL-positive strains were CC6–, CC8–, and CC152–MSSA.

Supplementary Materials

The following supporting information can be downloaded at: https://0-www-mdpi-com.brum.beds.ac.uk/article/10.3390/antibiotics12061050/s1, Supplemental File S1: Hybridisation profiles and CC/strain affiliations of tested isolates (pdf). Supplemental File S2: Genome sequences of isolates 2020-042_7641M (CC8–MSSA, PVL-non-producer), 2020-043_7352M (CC8–MSSA, PVL-producer, as control), 2020-009_371M (CC239–MRSA–III var. with partially flipped/inverted SCCmec), 2020-021_7037M (CC239–MRSA–III var.) and 2020-048_8421A (CC239–MRSA–III var.). Supplemental File S3: Alignment of hld and the agr genes of the CC8 reference sequence NCTC8325 CP000253.1, the PVL-non-producer 2020-042_7641M (TT-042), and the PVL-producing isolate 2020-043_7352M (TT-043). The red arrow indicates a deletion in agrC-I of 2020-042_7641M (TT-042).

Author Contributions

S.M.: Conceptualization, formal analysis, visualization, writing—original draft preparation; P.E.A.: Conceptualization, resources, investigations, writing—original draft preparation; M.R.S.: methodology/investigations; C.G.U.: methodology/investigations; C.-A.T.R.: methodology/investigations, K.A.: methodology/investigations; E.M.: methodology/investigations; S.D.B.: methodology/investigations, formal analysis; C.D.: methodology/investigations, formal analysis; M.R.: methodology/investigations, formal analysis; R.E.: writing—review and editing, supervision, project administration, funding acquisition: All authors have read and agreed to the published version of the manuscript.

Funding

There was no external funding for the Caribbean groups. The Jena group acknowledges support by the German Federal Ministry of Education and Research and the German Federal Ministry for Economic Affairs and Energy, within the framework of four projects, “ADA” (13GW0456) and “ResiCheck” (13GW0422) aiming to develop rapid assays for the detection and characterisation of resistance genes and virulence factors in S. aureus, “LPI-BT5” aiming on novel technologies for rapid diagnostic assays (13N15717) and “Development of a leukocidin rapid assay” (49MF180153).

Institutional Review Board Statement

This study was carried out in accordance with guidelines approved by the University of the West Indies Campus Ethics Committee, as well as the ethical review boards of the Trinidad and Tobago Regional Health Authorities (RHAs).

Informed Consent Statement

Not applicable.

Data Availability Statement

All relevant data are provided as Supplementary Files. The sequences of the genomes discussed, including the SCCmec element discussed, can be accessed under BioProject accession number PRJNA978032, and GenBank accession numbers CP127017 to CP127027.

Acknowledgments

The authors would like to express their gratitude to all laboratory techs in the laboratories in Trinidad and Tobago and Jamaica, as well as Annett Reissig and Maximillan Collatz at IPHT Jena for assisting in this study. We acknowledge Albrecht Ziegler (Dresden, Germany) and Peter Slickers (Jena) for help regarding software and databases used to analyse genome sequences. The publication of this article was funded by the Open Access Fund of the Leibniz Association.

Conflicts of Interest

The authors have not declared any conflict of interest.

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Antibiotics 12 01050 g001 550
Figure 1. Clonal distribution of PVL-positive MSSA strains from Trinidad and Tobago.
Figure 1. Clonal distribution of PVL-positive MSSA strains from Trinidad and Tobago.
Antibiotics 12 01050 g001
Table
Table 1. Specimen source distribution of MSSA, MRSA, and S. argenteus isolates from Trinidad and Tobago (%).
Table 1. Specimen source distribution of MSSA, MRSA, and S. argenteus isolates from Trinidad and Tobago (%).
StrainN (%)W/SwabBloodPusUrineOther
MSSA73 (86)419788
MRSA10 (12)62002
S. argenteus2 (2)11000
Total85 (100)48 (57)12 (14)7 (8)8 (9)10 (12)
MRSA, Methicillin-resistant Staphylococcus aureus; MSSA, Methicillin-susceptible Staphylococcus aureus; N, number encountered; W/Swab, Wound swab.
Table
Table 2. Specimen source distribution of MSSA and MRSA isolates from Jamaica (%).
Table 2. Specimen source distribution of MSSA and MRSA isolates from Jamaica (%).
StrainN (%)W/SwabThroatBlood
MSSA16 (100)1312
MRSA0 (0)000
Total16 (100)13 (81)1 (6)2 (13)
MRSA, Methicillin-resistant Staphylococcus aureus; MSSA, Methicillin-susceptible Staphylococcus aureus; N, number encountered; W/Swab, Wound swab.
Table
Table 3. Age group distribution of patients infected with MSSA, MRSA, and S. argenteus strains from Trinidad and Tobago.
Table 3. Age group distribution of patients infected with MSSA, MRSA, and S. argenteus strains from Trinidad and Tobago.
Age Group (Years)N (%)MRSAMSSAS. argenteus
0–915 (18)2 12 1
10–1915 (18)1 14 0
20–294 (5)1 3 0
30–3919 (22)1 180
40–499 (11)1 7 1
50–5910 (12)37 0
60–697 (8)1 6 0
70–792 (2)0 2 0
80+3 (3)0 3 0
Other/unrecorded1 (1)0 1 0
Total85 (100)10 (12)73 (86)2 (2)
MRSA, Methicillin-resistant Staphylococcus aureus; MSSA, Methicillin-susceptible Staphylococcus aureus; N, number encountered.
Table
Table 4. Gender distribution of patients infected with MSSA, MRSA, and S. argenteus strains from Trinidad and Tobago.
Table 4. Gender distribution of patients infected with MSSA, MRSA, and S. argenteus strains from Trinidad and Tobago.
Age Group (Years)N (%)MRSA MSSA S. argenteus
    Male46 (54)4411
    Female37 (44)6301
    Not recorded2 (2)020
Total85 (100)10 (12)73 (86)2 (2)
MRSA, Methicillin-resistant Staphylococcus aureus; MSSA, Methicillin-susceptible Staphylococcus aureus; N, number encountered.
Table
Table 5. Distribution of S. aureus clonal complexes, MSSA strains, and SCCmec elements as identified by array hybridisation for Trinidad, Tobago, and Jamaica.
Table 5. Distribution of S. aureus clonal complexes, MSSA strains, and SCCmec elements as identified by array hybridisation for Trinidad, Tobago, and Jamaica.
CCStrainSCCmec TypeN (%) for Trinidad and TobagoN (%) for Jamaica
CC1CC1–MSSA-1 (1.2%)4 (25%)
CC5CC5–MSSA-1 (1.2%)-
CC5–MSSA (PVL+)-2 (2.4%)-
CC6CC6–MSSA-4 (4.7%)1 (6.3%)
CC6–MSSA (PVL+)-4 (4.7%)2 (12.5%)
CC7CC7–MSSA-5 (5.9%)-
CC8CC8–MSSA-2 (2.4%)-
CC8–MSSA (PVL+)-12 (14.1%)-
CC8–MSSA (ACME/PVL+)ACME-I + speG + adhC + copA21 (1.2%)-
CC9CC9–MSSA-1 (1.2%)-
CC12CC12–MSSA-1 (1.2%)-
CC15CC15–MSSA-3 (3.5%)-
CC22CC22–MRSA–IV (PVL+/tst+)SCCmec IVa1 (1.2%)-
CC30CC30–MSSA-1 (1.2%)-
CC45CC45–MSSA-2 (2.4%)2 (12.5%)
CC59CC59–MSSA-1 (1.2%)-
CC72ST72–MSSA-2 (2.4%)2 (12.5%)
ST72–MRSA–[mecVT + fus]SCCmec VT + fus1 (1.2%)-
CC88CC88–MRSA IVSCCmec IVa1 (1.2%)-
CC97CC97–MSSA-9 (10.6%)1 (6.3%)
CC101CC101–MSSA-1 (1.2%)1 (6.3%)
CC121CC121–MSSA-1 (1.2%)-
CC152CC152–MSSA-1 (1.2%)-
CC152–MSSA (PVL+)-13 (15.3%)2 (12.5%)
CC188CC188–MSSA--1 (6.3%)
CC239CC239–MRSA–III, atypical “Southeast Asian Clade” *Composite SCCmec III *5 (5.9%)-
CC239–MRSA–[mec III + Cd/Hg + ccrC], “Southeast Asian Clade”SCC [mec III + Cd/Hg + ccrC] (Bmb9393)2 (2.4%)-
CC398CC398–MSSA-5 (5.9%)-
S. argenteus CC2596CC2596–MSSarg-2 (2.4%)-
* See separate paragraph and Table 6 for further explanation.
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Monecke, S.; Akpaka, P.E.; Smith, M.R.; Unakal, C.G.; Thoms Rodriguez, C.-A.; Ashraph, K.; Müller, E.; Braun, S.D.; Diezel, C.; Reinicke, M.; et al. Clonal Complexes Distribution of Staphylococcus aureus Isolates from Clinical Samples from the Caribbean Islands. Antibiotics 2023, 12, 1050. https://0-doi-org.brum.beds.ac.uk/10.3390/antibiotics12061050

AMA Style

Monecke S, Akpaka PE, Smith MR, Unakal CG, Thoms Rodriguez C-A, Ashraph K, Müller E, Braun SD, Diezel C, Reinicke M, et al. Clonal Complexes Distribution of Staphylococcus aureus Isolates from Clinical Samples from the Caribbean Islands. Antibiotics. 2023; 12(6):1050. https://0-doi-org.brum.beds.ac.uk/10.3390/antibiotics12061050

Chicago/Turabian Style

Monecke, Stefan, Patrick Eberechi Akpaka, Margaret R. Smith, Chandrashekhar G. Unakal, Camille-Ann Thoms Rodriguez, Khalil Ashraph, Elke Müller, Sascha D. Braun, Celia Diezel, Martin Reinicke, and et al. 2023. "Clonal Complexes Distribution of Staphylococcus aureus Isolates from Clinical Samples from the Caribbean Islands" Antibiotics 12, no. 6: 1050. https://0-doi-org.brum.beds.ac.uk/10.3390/antibiotics12061050

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