Introduction. Extended-spectrum β-lactamase (ESβL)-producing
Materials/Methods. Bacterial identification and the preliminary antibiotic susceptibilities was performed using the VI-TEK® 2 Compact automated system. Genes encoding ESβLs were amplified by CTX-Mplex PCR and PCR reactions. The presence of nine genes encoding virulence factors was studied by multiplex PCR. Clonality was investigated by PFGE after digestion with
Results.
Conclusions. Our results indicate that the presence of a wide variety of MDR
Keywords
- ESβL-producing
- MDR
- molecular epidemiology
- PFGE
- virulence-associated genes
The effective worldwide spread of extended-spectrum β-lactamase (ESβL)-producing
ESβLs are β-lactamases able of conferring bacterial resistance to the penicillins; first-, second-, third-generation cephalosporins; and aztreonam (but not the cephamycins or carbapenems) by hydrolysis of these antibiotics, which are inhibited by β-lactamase inhibitors such as clavulanic acid [5]. In recent years, most ESβL-producing organisms have also been found to be resistant to other major classes of antibiotics, such as aminoglycosides, fluoroquinolones, and sulfonamides, owing to the coexistence of associated resistant genes encoded in and transmitted by plasmids [6].
ESβL-producing bacteria were first detected in Europe in the 1980s. Although the initial reports were from Germany and England, the vast majority of reports in the first decade after the discovery of ESβLs were from France [5]. According to the SENTRY Antimicrobial Surveillance Program (1997 to 2016), the prevalence rate of ESβL-producing
The global problem of the presence of ESβL-producing
Our work aimed to characterize a collection the clinical isolates of
A total of 139
The demographic information (sample type, ward) of the patients and ESβL-producing isolate information (number, infectious site, and antibiotic susceptibility profile) were collected from the microbiological laboratory in the hospital.
The initial species identification, performed by the laboratory staff as part of routine diagnostics, was based on the assays of biochemical profiles of the isolates using the VITEK® 2 Compact system with GN ID card (bioMérieux, France). In vitro susceptibility of
Confirmed ESβL-producing strains were screened for
Multiplex PCR assays as published by Compain et al. were used to detect the presence of nine virulence-associated genes, including those encoding for regulators of capsular serotype K1 and hypermucoviscosity phenotype (
The genetic relatedness of the ESβL-producing
All statistical analyses were performed using R (version 3.5.3; The R Foundation for Statistical Computing, Austria). Statistical significance was assessed via the Fisher’s exact test for categorical variables in order to compare the resistance to selected antibiotics and the presence of virulence factors among the four main PFGE clonal types identified (A–D). The correlation analysis between virulence genes and resistance genes in the studied
All examined
Figure 1:
Antimicrobial resistance patterns of ESβL-producing

The isolates were phenotypically confirmed as ESβL producers and carried
Multiplex polymerase chain reaction analysis demonstrated that the
Twenty-five different combinations were observed based on the coexistence of virulence genes with resistance genes [Fig. 3]. The largest group of isolates (n=52, 37.4%) were strains with three genes encoding virulence factors and four resistance genes in different lists:
Figure 2:
Dendrogram illustrating the PFGE patterns of 139 ESβL-producing

Figure 3:
Correlation between virulence genes and resistance genes in ESβL-producing

PFGE identified 41 different profiles which fell into 4 major clusters (A–D) in 85 isolates (comprising 61% of the entire collection), based on a similarity of ≥ 98% (cut-off) [Fig. 2]. The largest cluster, A, accounted for 28.1% (n=39) of all isolates and contained strains from four hospital wards, including 19 (48.7%) isolates from CARDIO, 15 (38.5%) from PULMO, 4 (10.2%) isolates from NEURO, and 1 (2.6%) isolate from the DIAGNOST ward. The next clusters were B (16.5%, n=23) with 14 (60.9%) isolates from CARDIO, 6 (26%) isolates from PULMO, 2 (8.7%) isolates from NEURO, and 1 (4.3%) isolate from the DIAGNOST ward; cluster C (8.6%, n=12) with 7 (58.3%) isolates from CARDIO, 3 (25%) isolates from PULMO, 1 (8.3%) isolate from INFECT DIS, and 1 (8.3%) isolate from the DIAGNOST ward; cluster D (7.2%, n=10) with 7 (70%) isolates from CARDIO, 2 (50%) isolates from PULMO, and 1 (10%) isolates from INFECT DIS. Clone A was mostly isolates extracted from bronchial aspirates (46%), clones B and C were mostly isolates from urine (34.8% and 41.7%, respectively), clone D was mostly isolates from urine (50%). Isolates classified into clonal type A demonstrated a significantly higher sensitivity to trimethoprim/sulfamethoxazole than isolates from the other three main PFGE clonal types (B–D) (p=0.06). Isolates classified into clonal type C demonstrated a significantly lower resistance to amikacin and piperacillin/tazobactam than isolates from the remaining main clonal types A, B, D (p<0.001). Isolates classified into clonal type D showed a significantly higher sensitivity to gentamicin than isolates from the remaining clonal types A, B, and C (p<0.001). As for other antibiotics, the results were not statistically significant. Among the main clonal types A–D, three subgroups were distinguished, which differed as regards the presence of
ESβL-producing
In
This study investigates drug resistance profiles, the presence of genes encoding selected virulence factors, and genetic diversity of the ESβL-producing
In their analysis of hospital-acquired infections caused by ESβL-producing
The results of drug susceptibility testing as regards the
It should be underlined that our investigations revealed a high percentage (54.7%) of strains resistant to piperacillin/tazobactam. Similar results were obtained by other Polish researchers, Mrowiec et al., who recorded 53.5% of
In this study, examinations conducted using PCR confirmed the presence of genes encoding ESβL in all the studied
A review of the literature indicates that in
In the course of analysis of the most common genes encoding virulence factors in the studied pool of
As for the
The epidemiological situation of a hospital or a given ward may be influenced by many factors; among them, the specificity of the facility, the profile of patients that are treated there, the antibiotics employed, hygienic and sanitary measures undertaken or the persistence of certain pathogenic microorganisms.
To conclude, due to worldwide reports of a significant increase in resistance of
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