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Your search keyword '"Hassen, Abdennaceur"' showing total 11 results
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11 results on '"Hassen, Abdennaceur"'

3. Widespread of the Vienna/Hungarian/Brazilian CC8-ST239-SCCmec III MRSA clone in patients hospitalized in the Tunisian Burn and Traumatology Center.

Author

Said, Meriam Ben, Thabet, Lamia, Cheriet, Sarah, Messadi, Amen Allah, Gómez, Paula, Ruiz-Ripa, Laura, Sghaier, Senda, Hassen, Bilel, Hassen, Abdennaceur, Torres, Carmen, and Abbassi, Mohamed Salah

Subjects
METHICILLIN, BURN care units, METHICILLIN-resistant staphylococcus aureus, DRUG resistance in bacteria, MICROBIAL sensitivity tests, CARBAPENEMS, PUBLIC health
Abstract

The emergence and spread of methicillin-resistant Staphylococcus aureus (MRSA) in hospitals is a major global public health concern. The current study sought to characterize 25 MRSA clinical isolates collected in a Tunisian hospital from December 2015 to September 2016, with the genetic lineages, virulence factors, and antibiotic resistance mechanisms determined for these isolates. Three spa -types were detected: t037 (23 isolates), t932, and t2235 (one isolate each). Isolates were ascribed to agr I (n  = 20), agr II (n  = 1), with four nontypeable isolates. Depending on sequence type (ST), the 25 MRSA isolates were assigned to two clonal complexes (CC8 and CC5), with a predominance of the lineage ST239-CC8 (n  = 24; 96%). All isolates belonging to CC8 had the SCC mec type III, while the unique CC5 isolate had SCC mec type IV. Antimicrobial susceptibility testing revealed high levels of resistance to aminoglycosides, tetracycline, ciprofloxacin and rifampicin for the majority of isolates belonging to the ST239-CC8 lineage. The ST149-CC5 isolate was susceptible to non-β-lactam antibiotics. One isolate harbored the tsst-1 gene (4%); however, lukS/LukF -PV, eta and etb genes were not detected. The MDR ST239-CC8 clone would seem to be widespread in this hospital. Therefore, a rigorous hygienic control system is urgently required. [ABSTRACT FROM AUTHOR]

Published
2023
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4. High rates of antibiotic resistance and biofilm production in Escherichia coli isolates from food products of animal and vegetable origins in Tunisia: a real threat to human health.

Author

Badi, Souhir, Salah Abbassi, Mohamed, Snoussi, Mejdi, Werheni, Rim, Hammami, Salah, Maal-Bared, Rasha, and Hassen, Abdennaceur

Subjects
MEAT microbiology, ESCHERICHIA coli, IN vitro studies, CLAVULANIC acid, VEGETABLES, STAINS & staining (Microscopy), CULTURE media (Biology), KANAMYCIN, BIOFILMS, GENTAMICIN, TETRACYCLINES, STREPTOMYCIN, COMPARATIVE studies, GENES, DESCRIPTIVE statistics, DRUG resistance in microorganisms, POLYMERASE chain reaction, BIOLOGICAL assay, AMOXICILLIN
Abstract

The aim of this study was to compare the antibiotic susceptibility of eighty Escherichia coli isolates from vegetables and food products of animal origin in Tunisia, and to study their genes encoding antibiotic resistance and in vitro biofilm forming capacity. Antimicrobial susceptibilities were determined, as well as PCR investigation of genes associated with antibiotic resistance. Biofilm formation was tested using four different methods: the microtiter plate-, MTT-staining-, XTT-staining-, and the Congo Red Agar assays. High antibiotic resistance rates were observed for amoxicillin (68.7%), amoxicillin/clavulanic acid (73.7%), gentamicin (68.7%), kanamycin (66.2%), nalidixic acid (36.2%), streptomycin (68.7%) and tetracycline (35%). The majority of isolates was multidrug resistant and biofilm producer. MTT testing showed that vegetables isolates were significantly higher biofilm producers compared to foods of animal origins. This study showed that E. coli isolates from food products were reservoirs of genes encoding antibiotic-resistance and have a high propensity to produce biofilm. [ABSTRACT FROM AUTHOR]

Published
2022
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5. From farm to fork: identical clones and Tn6674-like elements in linezolid-resistant Enterococcus faecalis from food-producing animals and retail meat.

Author

Elghaieb, Houyem, Tedim, Ana P, Abbassi, Mohamed S, Novais, Carla, Duarte, Bárbara, Hassen, Abdennaceur, Peixe, Luísa, and Freitas, Ana R

Subjects
FOOD animals, ENTEROCOCCUS faecalis, HUMAN cloning, MOLECULAR cloning, MEAT, RESEARCH, POULTRY, SEQUENCE analysis, DNA, ANIMAL experimentation, RESEARCH methodology, PETS, FOOD microbiology, MEDICAL cooperation, EVALUATION research, GRAM-positive bacterial infections, COMPARATIVE studies, ENTEROCOCCUS, DRUG resistance in microorganisms, ANTIBIOTICS, MICROBIAL sensitivity tests, PHARMACODYNAMICS
Abstract

Objectives: Increasing numbers of linezolid-resistant Enterococcus carrying optrA are being reported across different niches worldwide. We aimed to characterize the first optrA-carrying Enterococcus faecalis obtained from food-producing animals and retail meat samples in Tunisia.Methods: Seven optrA-carrying E. faecalis obtained from chicken faeces (n=3, August 2017) and retail chicken meat (n=4, August 2017) in Tunisia were analysed. Antimicrobial susceptibility was determined by disc diffusion, broth microdilution and Etest against 13 antibiotics, linezolid and tedizolid, respectively (EUCAST/CLSI). optrA stability (∼600 bacterial generations), transfer (filter mating) and location (S1-PFGE/hybridization) were characterized. WGS (Illumina-HiSeq) was done for four representatives that were analysed through in silico and genomic mapping tools.Results: Four MDR clones carrying different virulence genes were identified in chicken faeces (ST476) and retail meat (the same ST476 clone plus ST21 and ST859) samples. MICs of linezolid and tedizolid were stably maintained at 8 and 1-2 mg/L, respectively. optrA was located in the same transferable chromosomal Tn6674-like element in ST476 and ST21 clones, similar to isolates from pigs in Malaysia and humans in China. ST859 carried a non-conjugative plasmid of ∼40 kb with an impB-fexA-optrA segment, similar to plasmids from pigs and humans in China.Conclusions: The same chromosomal and transferable Tn6674-like element was identified in different E. faecalis clones from humans and animals. The finding of retail meat contaminated with the same linezolid-resistant E. faecalis strain obtained from a food-producing animal highlights the potential role of the food chain in the worrisome dissemination of optrA that can be stably maintained without selective pressure over generations. [ABSTRACT FROM AUTHOR]

Published
2020
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6. Dispersal of linezolid-resistant enterococci carrying poxtA or optrA in retail meat and food-producing animals from Tunisia.

Author

Elghaieb, Houyem, Freitas, Ana R, Abbassi, Mohamed Salah, Novais, Carla, Zouari, Mohamed, Hassen, Abdennaceur, and Peixe, Luísa

Subjects
FOOD animals, POULTRY, DOMESTIC animals, ENTEROCOCCUS faecalis, ENTEROCOCCUS faecium, BOS, MEAT, CHICKENS
Abstract

Objectives: The epidemiology of Enterococcus resistant to priority antibiotics including linezolid has mainly been investigated in developed countries and especially in hospitals. We aimed to evaluate the contribution of different non-human reservoirs for the burden of MDR enterococci in Tunisia, where scarce data are available.Methods: Samples (n = 287) were collected from urban wastewater (n = 57), retail meat (n = 29; poultry/bovine/ovine), milk (n = 89; bovine/ovine), farm animal faeces (n = 80; poultry/bovine/ovine) and pets (n = 32; rabbit/dogs/cats/birds) in different Tunisian regions (2014-17). They were plated onto Slanetz-Bartley agar after pre-enrichment without antibiotics. Standard methods were used for bacterial identification and characterization of antibiotic resistance and virulence genes (PCR), antibiotic susceptibility testing (disc diffusion/broth microdilution; EUCAST/CLSI) and clonality (SmaI-PFGE/MLST).Results: All samples carried Enterococcus (n = 377 isolates) resistant to antibiotics considered to be critical or highly important by WHO. Even without antibiotic selection, 38% of Enterococcus faecalis (Efs) and 22% of Enterococcus faecium (Efm) were identified as MDR. Linezolid-resistant isolates (5%; MIC = 8 mg/L) comprised six poxtA-carrying Efm (cow milk), seven optrA-carrying Efs (chicken faeces/meat) and five Efm lacking cfr/optrA/poxtA (poultry/bovine/ovine/wastewater). Clinically relevant Efm clones (clade A1) were identified in animal/meat sources. Ampicillin resistance (1%) was confined to ST18/ST78-like MDR Efm clones from bovine meat/milk samples carrying relevant virulence markers (e.g. ptsD/IS16).Conclusions: This study provides evidence of the contribution of livestock and foodstuffs to the dispersal of acquired linezolid resistance genes including poxtA and optrA. We report the first poxtA-carrying Efm in Tunisia, and for the first time in bovine samples, stressing the urgent need for alternative measures to counteract the spread of linezolid-resistant enterococci globally. [ABSTRACT FROM AUTHOR]

Published
2019
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7. Pedologic characteristics and fungi community in unmanaged cork oak forest soil of two Mediterranean regions: Sardinia and Tunisia

Author

Fumi, Maria Daria, Mazzoleni, Valeria, Novelli, Elisa, Galli, Roberta, Busconi, Matteo, Blaghen, Mohamed, Hassen, Abdennaceur, Hursthouse, Andrew, Mclellan, Iain, Pintus, Agostino, Silva Pereiira, Cristina, Varela, Adelia, and Ruiu, Pino Angelo

Subjects
oil fungi, Tunisia, Settore AGR/15 - SCIENZE E TECNOLOGIE ALIMENTARI, Sardinia, pedologic characteristics, pedologic characteristics, cork oak forest, Sardinia
Published
2014

8. Intraspecific characterization of Vibrio alginolyticus isolates recovered from aquaculture systems and marine biotopes in Tunisia by PCR-RFLP, ECP and OMPs profiling.

Author

Lajnef, Rim, Abdallah, Lotfi Ben, Tapia-Paniagua, Silvana, Turki, Yosra, Medina, Alberto, Mehri, Ines, Moriñigo, Miguel Angel, and Hassen, Abdennaceur

Subjects
*VIBRIO alginolyticus, *MARICULTURE, *MEMBRANE proteins, *DNA polymerases, *FISH farming
Abstract

A total of 54 presumptive Vibrio alginolyticus strains isolated from a variety of Tunisian marine biotopes, such as seawater, sediment samples from some bathing areas, and aquaculture farms, were characterized and identified by several biochemical tests. DNA polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP) analysis, extracellular products (ECP) and outer membrane protein (OMP) profiling were used to evaluate their usefulness as a tool to investigate the Vibrio alginolyticus diversity within this complex group. Results showed that there is great heterogeneity in the diversity observed via the PCR-RFLP method related to the number of genotypes generated by the two enzymes SduI and FaqI tested. This heterogeneity was observed not only according to the origin (seawater, sediment, fish and bivalve aquaculture farms) but also within the same type of sample. The two other methods, ECP and OMP resulted in 32 and 26 profiles, respectively. The discriminatory index determined in this study highlighted the good ability of the PCR-RFLP method to discriminate similar V. alginolyticus strains. [ABSTRACT FROM AUTHOR]

Published
2023
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9. Detection of Aichi virus genotype B in two lines of wastewater treatment processes.

Author

Ibrahim, Chourouk, Hammami, Salah, Mejri, Selma, Mehri, Ines, Pothier, Pierre, and Hassen, Abdennaceur

Subjects
*ENTEROVIRUSES, *VIRAL gastroenteritis, *WASTEWATER treatment, *REVERSE transcriptase polymerase chain reaction, *GENOTYPE-environment interaction, ENVIRONMENTAL aspects
Abstract

Enteric viruses are released in important quantities into the environment where they can persist for a very long time. At very low doses, they can cause human gastroenteritis, and are responsible for a substantial number of waterborne diseases. The aims of this study were multiple: firstly, to study the circulation of Aichi viruses ( AiV ) in wastewater sampled at the scale of a pilot wastewater treatment plant; secondly, to evaluate the performance of two wastewater treatment procedures, as natural oxidizing lagoons and rotating Biodisks, concerning the AiV removal; and finally, to determine the different type of AiV genotype found during this study. Hence, the pilot wastewater treatment plant is principally irrigated by the wastewater of three neighbouring clinics. Wastewater samples were collected during 2011 from the two lines of biological treatment procedures. AiV detection in wastewater were achieved using the Reverse Transcription Polymerase Chain Reaction (RT-PCR) technique, and the identification of AiV genotype was realized by the direct sequencing of PCR products. The result revealed that AiV strains were identified in 50% (n = 51) of the wastewater samples. A significant increase of the AiV detection frequency was registered from upstream to downstream of the five ponds constituting the natural oxidizing lagoon process, and at the exit of the rotating Biodisks procedure. All detected AiV strains showed the highest nucleotide sequence identity to genotype B that has been recently observed in patients in Asia. This finding represented the first Tunisian survey that revealed and mentioned the first detection of AiV genotype B in sewage and by the same argued for a noticeable resistance or survival of this type of virus in the two lines of treatment considered. [ABSTRACT FROM AUTHOR]

Published
2017
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10. Genetic characterization of Staphylococcus aureus isolated from nasal samples of healthy ewes in Tunisia. High prevalence of CC130 and CC522 lineages.

Author

Ben Said, Meriam, Abbassi, Mohamed Salah, Gómez, Paula, Ruiz-Ripa, Laura, Sghaier, Senda, El Fekih, Oussama, Hassen, Abdennaceur, and Torres, Carmen

Subjects
*STAPHYLOCOCCUS aureus genetics, *EWES, *MICROBIAL virulence genetics, *MULTIDRUG tolerance (Microbiology), *MICROBIAL sensitivity tests
Abstract

Staphylococcus aureus is a versatile bacterium, which can infect or colonize a variety of host species. The objective of this study was to characterize S. aureus isolates recovered from nasal swabs of 167 healthy ewes sampled from 12 farms in different areas of Tunisia during the period of 2014–2015. Genetic lineages, virulence factors and antibiotic resistance mechanisms were determined for recovered isolates. S. aureus was detected in 45 out of 167 tested samples (26.9%). All isolates were methicillin-susceptible (MSSA) and the majority of them were susceptible to tested antibiotics with few exceptions (% of resistance): penicillin (8.8), ciprofloxacin (4.4), and tobramycin or tetracycline (2.2, each). Twelve different spa types were detected (t15098, t15099, t1773, t3576, t1534, t5428, t3750, t5970 t254, t2883, t127 and t933), two of them were new (t15098 and t15099). S. aureus isolates were ascribed to agr I (n = 23), agr II (n = 1) and agr III (n = 20), and one was non-typeable. According to the sequence-type (ST) determined and/or the spa- type detected, the 45 S. aureus isolates were assigned to six clonal complexes, with CC522 (44.4%) and CC130 (37.7%) being the most common lineages. Twenty-one (46.6%) and two (4.2%) isolates harbored the tst and eta genes encoding TSST-1 and ETA, respectively. In conclusion, nares of healthy ewes could be a reservoir of MSSA CC522 and CC130, lineages associated with TSST-1 and ETA that might represent a risk to human health. [ABSTRACT FROM AUTHOR]

Published
2017
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11. mcr-1 encoding colistin resistance in CTX-M-1/CTX-M-15- producing Escherichia coli isolates of bovine and caprine origins in Tunisia. First report of CTX-M-15-ST394/D E. coli from goats.

Author

Hassen, Bilel, Saloua, Benlabidi, Abbassi, Mohamed Salah, Ruiz-Ripa, Laura, Mama, Olouwafemi M., Hassen, Abdennaceur, Hammami, Salah, and Torres, Carmen

Subjects
*COLISTIN, *ESCHERICHIA coli, *GOAT milk, *RAW milk, *MICROBIAL sensitivity tests, *GOATS
Abstract

• 120 bovine faecal samples and 103 raw bovine/caprine milk samples analysed. • Eight samples (3.6%) contained ESBL-producing E. coli (ESBL-EC) (5: raw milk; 3: cattle faeces). • Four colistin-resistant ESBL-EC isolates of bovine origin (mcr -1-positive). • ESBL-EC strains: mcr -1/CTX-M-1/D-ST1642, mcr -1/CTX-M-1/A-ST10, CTX-M-15/B1-ST394, and CTX-M-15/A-ST46. • Most of bovine ESBL-EC isolates were multidrug-resistant. The objective of this study was to isolate and characterize ESBL-producing Escherichia coli (ESBL-EC) from raw bovine and caprine milk samples, as well as from bovine faeces in Tunisia. Therefore, 120 bovine faecal samples and 9 caprine raw milk samples were collected from 2 extensive dairy-cow-farms and 5 ovine farms, respectively. In addition, 94 raw bovine milk samples, from containers and holding tanks from 50 small public-markets in the North of Tunisia, were processed for the isolation of cefotaxime-resistant E. coli (CTXR). Antimicrobial susceptibility testing was carried out by disc-diffusion/broth-microdilution methods. The presence of genes encoding ESBL, as well as those encoding colistin (mcr -1 to 5 genes)- sulfonamide-, tetracycline-, gentamicin-, quinolone and chloramphenicol-resistance and class 1 integrons were tested by PCR (and sequencing in some cases). ESBL-EC isolates were further characterized by phylogrouping and MLST/PFGE typing. Eight samples (3.6%) contained ESBL-EC isolates (3/2 from raw bovine/goat milk and 3 from cattle faeces) and one isolate/sample was characterized. Four ESBL-EC isolates, all of bovine origin (3 faeces/1 milk), were resistant to colistin (MIC: 8–16 μg/ml), harboured the mcr -1 gene and carried IncP- and IncFIB-type plasmids. The 8 ESBL-EC strains had the following characteristics: a) bovine faeces: mcr -1/CTX-M-1/D-ST1642 (3 strains); b) raw milk: mcr -1/CTX-M-1/A-ST10 (1 strain); CTX-M-15/B1-ST394 (3 strains), and CTX-M-15/A-ST46 (1 strain). Most of bovine ESBL-EC isolates were multidrug-resistant (4/5). Our results showed that ESBL-EC were detected in bovine and caprine samples (CTX-M-1/CTX-M-15 producers), being some of them colistin-resistant (associated with mcr -1 gene), and they belonged to international clonal lineages. [ABSTRACT FROM AUTHOR]

Published
2019
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