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201. Antisense inhibition of lpxB gene expression in Acinetobacter baumannii by peptide-PNA conjugates and synergy with colistin.

Author

Martínez-Guitián, Marta, Vázquez-Ucha, Juan Carlos, Álvarez-Fraga, Laura, Conde-Pérez, Kelly, Bou, Germán, Poza, Margarita, and Beceiro, Alejandro

Subjects
ACINETOBACTER baumannii, GENE expression, PEPTIDE nucleic acids, COLISTIN, GREATER wax moth, ANTIBACTERIAL agents
Abstract

Background: LpxB is an enzyme involved in the biosynthesis pathway of lipid A, a component of LPS.Objectives: To evaluate the lpxB gene in Acinetobacter baumannii as a potential therapeutic target and to propose antisense agents such as peptide nucleic acids (PNAs) as a tool to combat bacterial infection, either alone or in combination with known antimicrobial therapies.Methods: RNA-seq analysis of the A. baumannii ATCC 17978 strain in a murine pneumonia model was performed to study the in vivo expression of lpxB. Protein expression was studied in the presence or absence of anti-lpxB (KFF)3K-PNA (pPNA). Time-kill curve analyses and protection assays of infected A549 cells were performed. The chequerboard technique was used to test for synergy between pPNA and colistin. A Galleria mellonella infection model was used to test the in vivo efficacy of pPNA.Results: The lpxB gene was overexpressed during pneumonia. Treatment with a specific pPNA inhibited LpxB expression in vitro, decreased survival of the ATCC 17978 strain and increased the survival rate of infected A549 cells. Synergy was observed between pPNA and colistin in colistin-susceptible strains. In vivo assays confirmed that a combination treatment of anti-lpxB pPNA and colistin was more effective than colistin in monotherapy.Conclusions: The lpxB gene is essential for A. baumannii survival. Anti-lpxB pPNA inhibits LpxB expression, causing bacterial death. This pPNA showed synergy with colistin and increased the survival rate in G. mellonella. The data suggest that antisense pPNA molecules blocking the lpxB gene could be used as antibacterial agents. [ABSTRACT FROM AUTHOR]

Published
2020
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203. Increased Antimicrobial Resistance in a Novel CMY-54 AmpC-Type Enzyme with a GluLeu217–218 Insertion in the Ω-Loop

Author

Pérez-Llarena, Francisco José, primary, Vázquez-Ucha, Juan Carlos, additional, Kerff, Frédéric, additional, Zamorano, Laura, additional, Miró, Elisenda, additional, Cabral, María Póvoa, additional, Fleites, Ana, additional, Lantero, Marta, additional, Martínez-Martínez, Luis, additional, Oliver, Antonio, additional, Galleni, Moreno, additional, Navarro, Ferrán, additional, Beceiro, Alejandro, additional, and Bou, Germán, additional

Published
2018
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205. Activity of ceftazidime-avibactam against carbapenemase-producing Enterobacteriaceae from urine specimens obtained during the infection-carbapenem resistance evaluation surveillance trial (iCREST) in Spain

Author

García-Castillo, María, primary, García-Fernández, Sergio, additional, Gómez-Gil, Rosa, additional, Pitart, Cristina, additional, Oviaño, Marina, additional, Gracia-Ahufinger, Irene, additional, Díaz-Regañón, Jazmín, additional, Tato, Marta, additional, Cantón, Rafael, additional, Bou, Germán, additional, Rodríguez, Julio García, additional, Gil, Rosa Gómez, additional, Martínez, Luis Martínez, additional, Ahufinger, Irene Gracia, additional, Vila, Jordi, additional, Marco, Francesc, additional, del Castillo, María García, additional, and Fernández, Sergio García, additional

Published
2018
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210. Contribution of the a-baumannii A1S_0114 gene to the interaction with eukaryotic cells and virulence

Author

Universidade de Santiago de Compostela. Departamento de Microbioloxía e Parasitoloxía, Rumbo Feal, Soraya, Pérez Gómez, Astrid, Ramelot, Theresa A., Álvarez Fraga, Laura, Vallejo Vidal, Juan Andrés, Beceiro, Alejandro, Ohneck, Emily J., Arivett, Brock A., Merino, María, Fiester, Steven E., Kennedy, Michael A., Actis, Luis A., Bou, Germán, Poza, Margarita, Universidade de Santiago de Compostela. Departamento de Microbioloxía e Parasitoloxía, Rumbo Feal, Soraya, Pérez Gómez, Astrid, Ramelot, Theresa A., Álvarez Fraga, Laura, Vallejo Vidal, Juan Andrés, Beceiro, Alejandro, Ohneck, Emily J., Arivett, Brock A., Merino, María, Fiester, Steven E., Kennedy, Michael A., Actis, Luis A., Bou, Germán, and Poza, Margarita

Abstract

Genetic and functional studies showed that some components of the Acinetobacter baumannii ATCC 17978 A1S_0112-A1S_0119 gene cluster are critical for biofilm biogenesis and surface motility. Recently, our group has shown that the A1S_0114 gene was involved in biofilm formation, a process related with pathogenesis. Confirming our previous results, microscopy images revealed that the ATCC 17978 10114 derivative lacking this gene was unable to form a mature biofilm structure. Therefore, other bacterial phenotypes were analyzed to determine the role of this gene in the pathogenicity of A. baumannii ATCC 17978. The interaction of the ATCC 17978 parental strain and the 10114 mutant with A549 human alveolar epithelial cells was quantified revealing that the A1S_0114 gene was necessary for proper attachment to A549 cells. This dependency correlates with the negative effect of the A1S_0114 deletion on the expression of genes coding for surface proteins and pili-assembly systems, which are known to play a role in adhesion. Three different experimental animal models, including vertebrate and invertebrate hosts, confirmed the role of the A1S_0114 gene in virulence. All of the experimental infection assays indicated that the virulence of the ATCC 17978 was significantly reduced when this gene was inactivated. Finally, we discovered that the A1S_0114 gene was involved in the production of a small lipopeptide-like compound herein referred to as acinetin 505 (Ac-505). Ac-505 was isolated from ATCC 17978 spent media and its chemical structure was interpreted by mass spectrometry. Overall, our observations provide novel information on the role of the A1S_0114 gene in A. baumannii’s pathobiology and lay the foundation for future work to determine the mechanisms by which Ac-505, or possibly an Ac-505 precursor, could execute critical functions as a secondary metabolite

Published
2017

211. Quantitative and automated MALDI-TOF MS-based detection of the plasmid-mediated quinolone resistance determinant AAC(6′)-Ib-cr in Enterobacteriaceae

Author

Instituto de Salud Carlos III, European Commission, Red Española de Investigación en Patología Infecciosa, Ministerio de Economía y Competitividad (España), Oviaño, María, Gómara, Marta, Barba, María José, Sparbier, Katrin, Pascual, Álvaro, Bou, Germán, Instituto de Salud Carlos III, European Commission, Red Española de Investigación en Patología Infecciosa, Ministerio de Economía y Competitividad (España), Oviaño, María, Gómara, Marta, Barba, María José, Sparbier, Katrin, Pascual, Álvaro, and Bou, Germán

Published
2017

212. MIC of amoxicillin/clavulanate according to CLSI and EUCAST: discrepancies and clinical impact in patients with bloodstream infections due to Enterobacteriaceae

Author

Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), European Commission, Red Española de Investigación en Patología Infecciosa, Delgado-Valverde, Mercedes, Valiente-Méndez, Adoración, Torres, Eva, Almirante, Benito, Gómez-Zorrilla, Silvia, Borrell, Núria, Aller-García, Ana Isabel, Gurguí, Mercè, Almela, Manel, Sanz, Mercedes, Bou, Germán, Martínez-Martínez, Luis, Cantón, Rafael, Lepe, José A., Causse, Manuel, Gutiérrez-Gutiérrez, Belén, Pascual, Álvaro, Rodríguez-Baño, Jesús, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (España), European Commission, Red Española de Investigación en Patología Infecciosa, Delgado-Valverde, Mercedes, Valiente-Méndez, Adoración, Torres, Eva, Almirante, Benito, Gómez-Zorrilla, Silvia, Borrell, Núria, Aller-García, Ana Isabel, Gurguí, Mercè, Almela, Manel, Sanz, Mercedes, Bou, Germán, Martínez-Martínez, Luis, Cantón, Rafael, Lepe, José A., Causse, Manuel, Gutiérrez-Gutiérrez, Belén, Pascual, Álvaro, and Rodríguez-Baño, Jesús

Abstract

[Objectives] To compare results of amoxicillin/clavulanate susceptibility testing using CLSI and EUCAST methodologies and to evaluate their impact on outcome in patients with bacteraemia caused by Enterobacteriaceae., [Patients and methods] A prospective observational cohort study was conducted in 13 Spanish hospitals. Patients with bacteraemia due to Enterobacteriaceae who received empirical intravenous amoxicillin/clavulanate treatment for at least 48 h were included. MICs were determined following CLSI and EUCAST recommendations. Outcome variables were: failure at the end of treatment with amoxicillin/clavulanate (FEAMC); failure at day 21; and 30 day mortality. Classification and regression tree (CART) analysis and logistic regression were performed., [Results] Overall, 264 episodes were included; the urinary tract was the most common source (64.7%) and Escherichia coli the most frequent pathogen (76.5%). Fifty-two isolates (19.7%) showed resistance according to CLSI and 141 (53.4%) according to EUCAST. The kappa index for the concordance between the results of both committees was only 0.24. EUCAST-derived, but not CLSI-derived, MICs were associated with failure when considered as continuous variables. CART analysis suggested a ‘resistance’ breakpoint of > 8/4 mg/L for CLSI-derived MICs; it predicted FEAMC in adjusted analysis (OR = 1.96; 95% CI: 0.98–3.90). Isolates with EUCAST-derived MICs >16/2 mg/L independently predicted FEAMC (OR = 2.10; 95% CI: 1.05–4.21) and failure at day 21 (OR= 3.01; 95% CI: 0.93–9.67). MICs >32/2 mg/L were only predictive of failure among patients with bacteraemia from urinary or biliary tract sources., [Conclusions] CLSI and EUCAST methodologies showed low agreement for determining the MIC of amoxicillin/clavulanate. EUCAST-derived MICs seemed more predictive of failure than CLSI-derived ones. EUCAST-derived MICs >16/2 mg/L were independently associated with therapeutic failure.

Published
2017

213. Global assessment of small RNAs reveals a non-coding transcript involved in biofilm formation and attachment in Acinetobacter baumannii ATCC 17978

Author

Instituto de Salud Carlos III, European Commission, Ministerio de Economía y Competitividad (España), Xunta de Galicia, Miami University, Red Española de Investigación en Patología Infecciosa, Sociedad Española de Enfermedades Infecciosas y Microbiología Clínica, Societat Catalana de Malalties Infeccioses i Microbiologia Clínica, Álvarez-Fraga, Laura, Rumbo-Feal, Soraya, Pérez, Astrid, Gómez, Manuel José, Gayoso, Carmen, Vallejo, Juan Andrés, Ohneck, Emily J., Valle Turrillas, Jaione, Actis, L. A., Beceiro, Alejandro, Bou, Germán, Poza, Margarita, Instituto de Salud Carlos III, European Commission, Ministerio de Economía y Competitividad (España), Xunta de Galicia, Miami University, Red Española de Investigación en Patología Infecciosa, Sociedad Española de Enfermedades Infecciosas y Microbiología Clínica, Societat Catalana de Malalties Infeccioses i Microbiologia Clínica, Álvarez-Fraga, Laura, Rumbo-Feal, Soraya, Pérez, Astrid, Gómez, Manuel José, Gayoso, Carmen, Vallejo, Juan Andrés, Ohneck, Emily J., Valle Turrillas, Jaione, Actis, L. A., Beceiro, Alejandro, Bou, Germán, and Poza, Margarita

Abstract

Many strains of Acinetobacter baumannii have been described as being able to form biofilm. Small non-coding RNAs (sRNAs) control gene expression in many regulatory circuits in bacteria. The aim of the present work was to provide a global description of the sRNAs produced both by planktonic and biofilm-associated (sessile) cells of A. baumannii ATCC 17978, and to compare the corresponding gene expression profiles to identify sRNAs molecules associated to biofilm formation and virulence. sRNA was extracted from both planktonic and sessile cells and reverse transcribed. cDNA was subjected to 454- pyrosequencing using the GS-FLX Titanium chemistry. The global analysis of the small RNA transcriptome revealed different sRNA expression patterns in planktonic and biofilm associated cells, with some of the transcripts only expressed or repressed in sessile bacteria. A total of 255 sRNAs were detected, with 185 of them differentially expressed in the different types of cells. A total of 9 sRNAs were expressed only in biofilm cells, while the expression of other 21 coding regions were repressed only in biofilm cells. Strikingly, the expression level of the sRNA 13573 was 120 times higher in biofilms than in planktonic cells, an observation that prompted us to further investigate the biological role of this noncoding transcript. Analyses of an isogenic mutant and over-expressing strains revealed that the sRNA 13573 gene is involved in biofilm formation and attachment to A549 human alveolar epithelial cells. The present work serves as a basis for future studies examining the complex regulatory network that regulate biofilm biogenesis and attachment to eukaryotic cells in A. baumannii ATCC 17978.

Published
2017

214. Bioinformatics approaches to the study of antimicrobial resistance.

Author

Seoane, Alejandro and Bou, Germán

Subjects
BIOINFORMATICS, DRUG resistance in bacteria, WHOLE genome sequencing, MASS spectrometry, DATA analysis
Abstract

Detection and monitoring of antimicrobial resistance are two pillars on which clinical microbiology will be based in the coming decades. The implementation of certain technologies such as whole genome sequencing (WGS) or mass spectrometry and the creation of national and international databases that include and gather data on antimicrobial resistance from around the world has allowed the application of bioinformatics in the study of antimicrobial resistance in microorganisms involved in human pathology. [ABSTRACT FROM AUTHOR]

Published
2021
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215. Acinetobacter baumannii en pacientes críticos: epidemiología molecular, características clínicas y predictores de mortalidad

Author

Garnacho-Montero, José, Gutiérrez-Pizarraya, A., Díaz-Martín, Ana, Cisneros, José Miguel, Cano, María Eugenia, Gato, Eva, Ruiz de Alegría, Carlos, Fernández-Cuenca, Felipe, Vila, Jordi, Martínez-Martínez, Luis, Tomás, María, Pascual, Álvaro, Bou, Germán, Pachón, Jerónimo, and Rodríguez-Baño, Jesús

Subjects
Acinetobacter baumannii, Medicina intensiva, Intensive medicine, Clonalidad, Mortalidad, Infectious diseases, Enfermedades infecciosas, Mortality, Clonality
Abstract

[Introduction] The main aim of this study was to assess changes in the epidemiology and clinical presentation of Acinetobacter baumannii over a 10-year period, as well as risk factors of mortality in infected patients. [Method] Prospective, multicentre, hospital-based cohort studies including critically ill patients with A. baumannii isolated from any clinical sample were included. These were divided into a first period (“2000 study”) (one month), and a second period (“2010 study”) (two months). Molecular typing was performed by REP-PCR, PFGE and MSLT. The primary endpoint was 30-day mortality. [Results] In 2000 and 2010, 103 and 108 patients were included, and the incidence of A. baumannii colonization/infection in the ICU decreased in 2010 (1.23 vs. 4.35 cases/1000 patient-days; p < 0.0001). No differences were found in the colonization rates (44.3 vs. 38.6%) or infected patients (55.7 vs. 61.4%) in both periods. Overall, 30-day mortality was similar in both periods (29.1 vs. 27.8%). The rate of pneumonia increased from 46.2 in 2000 to 64.8% in 2010 (p < 0.001). Performing MSLT, 18 different sequence types (ST) were identified (18 in 2000, 8 in 2010), but ST2 and ST79 were the predominant clones. ST2 isolates in the ICU increased from 53.4% in the year 2000 to 73.8% in 2010 (p = 0.002). In patients with A. baumannii infection, the multivariate analysis identified appropriate antimicrobial therapy and ST79 clonal group as protective factors for mortality. [Conclusions] At 10 years of the first analysis, some variations have been observed in the epidemiology of A. baumannii in the ICU, with no changes in mortality. Epidemic ST79 clone seems to be associated with a better prognosis and adequate treatment is crucial in terms of survival. [Introducción] El principal objetivo fue evaluar los cambios en la epidemiología a lo largo de un periodo de 10 años, así como la presentación clínica y los factores predictores de mortalidad en los pacientes críticos infectados por Acinetobacter baumannii. [Método] Estudio de cohortes prospectivo y multicéntrico en el que se incluyeron pacientes críticos con A. baumannii aislado de cualquier muestra clínica. Se consideró un primer período («estudio de 2000») (un mes) y un segundo («estudio de 2010») (2 meses). La tipificación molecular se realizó mediante REP-PCR, PFGE y MSLT. La variable resultado primaria fue la mortalidad a los 30 días. [Resultados] En 2000 y 2010 se incluyeron 103 y 108 pacientes, respectivamente, y la incidencia de colonización/infección por A. baumannii en la UCI disminuyó en 2010 respecto al 2000 (1,23 vs. 4,35 casos/1.000 pacientes-días; p < 0,0001). No se encontraron diferencias en la tasa de colonización (44,3 vs. 38,6%) o infección (55,7 vs. 61,4%) en ambos periodos. En general, la mortalidad a los 30 días fue similar en ambos periodos (29,1 vs. 27,8%). La tasa de neumonía aumentó desde el 46,2% en 2000 al 64,8% en 2010 (p < 0,001). Mediante MSLT, se identificaron 18 tipos de secuencias diferentes (ST) (18 en 2000, 8 en 2010), pero ST2 y ST79 fueron los clones predominantes. La identificación de ST2 aumentó en la UCI desde el 53,4% en 2000 al 73,8% en 2010 (p = 0,002). En los pacientes infectados, el tratamiento antimicrobiano apropiado y el grupo clonal ST79 fueron factores protectores de mortalidad en el análisis multivariante. [Conclusiones] A los 10 años del primer análisis se han observado algunos cambios en la epidemiología de A. baumannii en la UCI, sin cambios en la mortalidad. El clon ST79 epidémico parece estar asociado con un mejor pronóstico, y el tratamiento adecuado es crucial en términos de supervivencia.

Published
2016

216. Activity of the β-Lactamase Inhibitor LN-1-255 against Carbapenem-Hydrolyzing Class D β-Lactamases from Acinetobacter baumannii

Author

Vázquez-Ucha, Juan Carlos, primary, Maneiro, María, additional, Martínez-Guitián, Marta, additional, Buynak, John, additional, Bethel, Christopher R., additional, Bonomo, Robert A., additional, Bou, Germán, additional, Poza, Margarita, additional, González-Bello, Concepción, additional, and Beceiro, Alejandro, additional

Published
2017
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218. Global assessment of small RNAs reveals a non-coding transcript involved in biofilm formation and attachment in Acinetobacter baumannii ATCC 17978

Author

Álvarez-Fraga, Laura, primary, Rumbo-Feal, Soraya, additional, Pérez, Astrid, additional, Gómez, Manuel J., additional, Gayoso, Carmen, additional, Vallejo, Juan A., additional, Ohneck, Emily J., additional, Valle, Jaione, additional, Actis, Luis A., additional, Beceiro, Alejandro, additional, Bou, Germán, additional, and Poza, Margarita, additional

Published
2017
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221. Contribution of the A. baumannii A1S_0114 Gene to the Interaction with Eukaryotic Cells and Virulence

Author

Rumbo-Feal, Soraya, primary, Pérez, Astrid, additional, Ramelot, Theresa A., additional, Álvarez-Fraga, Laura, additional, Vallejo, Juan A., additional, Beceiro, Alejandro, additional, Ohneck, Emily J., additional, Arivett, Brock A., additional, Merino, María, additional, Fiester, Steven E., additional, Kennedy, Michael A., additional, Actis, Luis A., additional, Bou, Germán, additional, and Poza, Margarita, additional

Published
2017
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224. Overproduction of outer membrane protein A (OmpA) by Acinetobacter baumannii is a risk factor for nosocomial pneumonia, bacteremia and mortality increase.

Author

Sánchez-Encinales, Viviana, primary, Álvarez-Marín, Rocío, additional, Pachón-Ibáñez, María Eugenia, additional, Fernández-Cuenca, Felipe, additional, Pascual, Alvaro, additional, Garnacho-Montero, José, additional, Martínez-Martínez, Luis, additional, Vila, Jordi, additional, Tomás, María Mar, additional, Cisneros, José Miguel, additional, Bou, Germán, additional, Rodríguez-Baño, Jesús, additional, Pachón, Jerónimo, additional, and Smani, Younes, additional

Published
2017
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227. Recommendations of the Spanish Antibiogram Committee (COESANT) for selecting antimicrobial agents and concentrations for in vitrosusceptibility studies using automated systems

Author

Cantón, Rafael, Oliver, Antonio, Alós, Juan Ignacio, de Benito, Natividad, Bou, Germán, Campos, José, Calvo, Jorge, Canut, Andrés, Castillo, Javier, Cercenado, Emilia, Domínguez, Maria Ángeles, Fernández-Cuenca, Felipe, Guinea, Jesús, Larrosa, Nieves, Liñares, Josefina, López-Cerero, Lorena, López-Navas, Antonio, Marco, Francesc, Mirelis, Beatriz, Moreno-Romo, Miguel Ángel, Morosini, María Isabel, Navarro, Ferran, Oteo, Jesús, Pascual, Álvaro, Pérez-Trallero, Emilio, Pérez-Vázquez, María, Soriano, Alex, Torres, Carmen, Vila, Jordi, and Martínez-Martínez, Luis

Abstract

Automated antimicrobial susceptibility testing devices are widely implemented in clinical microbiology laboratories in Spain, mainly using EUCAST (European Committee on Antimicrobial Susceptibility Testing) breakpoints. In 2007, a group of experts published recommendations for including antimicrobial agents and selecting concentrations in these systems. Under the patronage of the Spanish Antibiogram Committee (Comité Español del Antibiograma, COESANT) and the Study Group on Mechanisms of Action and Resistance to Antimicrobial Agents (GEMARA) from the Spanish Society of Infectious Diseases and Clinical Microbiology (SEIMC), and aligned with the Spanish National Plan against Antimicrobial Resistance (PRAN), a group of experts have updated this document. The main modifications from the previous version comprise the inclusion of new antimicrobial agents, adaptation of the ranges of concentrations to cover the EUCAST breakpoints and epidemiological cut-off values (ECOFFs), and the inference of new resistance mechanisms. This proposal should be considered by different manufacturers and users when designing new panels or cards. In addition, recommendations for selective reporting are also included. With this approach, the implementation of EUCAST breakpoints will be easier, increasing the quality of antimicrobial susceptibility testing data and their microbiological interpretation. It will also benefit epidemiological surveillance studies as well as the clinical use of antimicrobials aligned with antimicrobial stewardship programs.

Published
2020
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228. Association between Pseudomonas aeruginosa O-antigen serotypes, resistance profiles and high-risk clones: results from a Spanish nationwide survey.

Author

Barrio-Tofiño, Ester del, Sánchez-Diener, Irina, Zamorano, Laura, Cortes-Lara, Sara, López-Causapé, Carla, Cabot, Gabriel, Bou, Germán, Martínez-Martínez, Luis, Oliver, Antonio, GEMARA-SEIMC/REIPI, and Del Barrio-Tofiño, Ester

Subjects
CEFTAZIDIME, PSEUDOMONAS aeruginosa, AMIKACIN, SEROTYPES, INFECTION prevention, FOOT & mouth disease, IMMUNE serums, MOLECULAR cloning
Abstract

Objectives: To evaluate the correlation of O-antigen serotypes with resistance profiles and high-risk clones in a Spanish nationwide survey.Methods: Up to 30 consecutive healthcare-associated Pseudomonas aeruginosa isolates were collected during October 2017 from each of 51 hospitals (covering all Spanish regions) with a total of 1445 isolates studied. MICs of 13 antipseudomonal agents and MDR/XDR profiles had been previously determined, as well as whole-genome sequences of 185 representative XDR isolates. O-antigen serotypes (O1-O16) were determined by agglutination using serotype-specific antisera (BioRad). The Pseudomonas aeruginosa serotyper (PAst) program was used for in silico serotyping.Results: The most frequent serotypes were O6 (17.8%), O1 (15.4%) and O11 (13.3%). In contrast, the most frequent serotype among XDR isolates (17.3%) was O4 (34.1%), distantly followed by O11 (15.9%). Within serotypes, XDR phenotypes were more frequent for O12 (60.0%) and O4 (57.3%). The most frequent clone among the XDR isolates was ST175 (40.9%), followed by CC235 (10.7%), ST308 (5.2%) and CC111 (3.6%). Up to 81.6% of XDR ST175 isolates typed O4, whereas 18.4% were non-typeable. O4 genotype was detected in all sequenced (n=55) ST175 isolates. On the other hand, CC235 and ST308 were associated with O11, whereas CC111 was linked to serotype O12.Conclusions: O4 serotype is linked to the MDR/XDR profile of widespread ST175 (typically only susceptible to colistin, amikacin and the novel combinations ceftolozane/tazobactam and ceftazidime/avibactam) and therefore, after local validation, its detection in the microbiology laboratory might be useful for guiding semi-empirical antipseudomonal therapies and infection control measures in Spanish hospitals. [ABSTRACT FROM AUTHOR]

Published
2019
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229. Spanish nationwide survey on Pseudomonas aeruginosa antimicrobial resistance mechanisms and epidemiology.

Author

Barrio-Tofiño, Ester del, Zamorano, Laura, Cortes-Lara, Sara, López-Causapé, Carla, Sánchez-Diener, Irina, Cabot, Gabriel, Bou, Germán, Martínez-Martínez, Luis, Oliver, Antonio, Group, GEMARA-SEIMC/REIPI Pseudomonas study, Del Barrio-Tofiño, Ester, and GEMARA-SEIMC/REIPI Pseudomonas study Group

Subjects
CEFTAZIDIME, PSEUDOMONAS aeruginosa, BETA lactamases, CARBAPENEMASE, MOLECULAR epidemiology, EPIDEMIOLOGY
Abstract

Objectives: To undertake a Spanish nationwide survey on Pseudomonas aeruginosa molecular epidemiology and antimicrobial resistance.Methods: Up to 30 consecutive healthcare-associated P. aeruginosa isolates collected in 2017 from each of 51 hospitals were studied. MICs of 13 antipseudomonal agents were determined by broth microdilution. Horizontally acquired β-lactamases were detected by phenotypic methods and PCR. Clonal epidemiology was evaluated through PFGE and MLST; at least one XDR isolate from each clone and hospital (n = 185) was sequenced.Results: The most active antipseudomonals against the 1445 isolates studied were colistin and ceftolozane/tazobactam (both 94.6% susceptible, MIC50/90 = 1/2 mg/L) followed by ceftazidime/avibactam (94.2% susceptible, MIC50/90 = 2/8 mg/L). Up to 252 (17.3%) of the isolates were XDR. Carbapenemases/ESBLs were detected in 3.1% of the isolates, including VIM, IMP, GES, PER and OXA enzymes. The most frequent clone among the XDR isolates was ST175 (40.9%), followed by CC235 (10.7%), ST308 (5.2%) and CC111 (4.0%). Carbapenemase production varied geographically and involved diverse clones, including 16.5% of ST175 XDR isolates. Additionally, 56% of the sequenced XDR isolates showed horizontally acquired aminoglycoside-modifying enzymes, which correlated with tobramycin resistance. Two XDR isolates produced QnrVC1, but fluoroquinolone resistance was mostly caused by QRDR mutations. Beyond frequent mutations (>60%) in OprD and AmpC regulators, four isolates showed AmpC mutations associated with resistance to ceftolozane/tazobactam and ceftazidime/avibactam.Conclusions: ST175 is the most frequent XDR high-risk clone in Spanish hospitals, but this nationwide survey also indicates a complex scenario in which major differences in local epidemiology, including carbapenemase production, need to be acknowledged in order to guide antimicrobial therapy. [ABSTRACT FROM AUTHOR]

Published
2019
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230. Métodos microbiológicos para la vigilancia del estado de portador de bacterias multirresistentes

Author

Oteo, Jesús, Bou, Germán, Chaves, Fernando, and Oliver, Antonio

Abstract

La existencia de pacientes colonizados es una de las principales vías de propagación de las bacterias multirresistentes, y su contención una prioridad asistencial y de salud pública. Los estudios de vigilancia son imprescindibles para una detección precoz de la colonización por estas bacterias. Este artículo aborda los diferentes métodos microbiológicos, basados en el cultivo y moleculares, para la detección del estado de portador de bacterias multirresistentes. Se incluyen aquellas especies de mayor interés debido a su impacto clínico/epidemiológico y a las dificultades terapéuticas que generan: Staphylococcus aureusresistente a meticilina, Enterococcusspp. resistente a los glucopéptidos, enterobacterias productoras de β-lactamasas de espectro extendido o β-lactamasas plasmídicas de tipo AmpC, enterobacterias productoras de carbapenemasas, Acinetobacter baumanniimultirresistente y Pseudomonas aeruginosamultirresistente. La información recogida en este documento debe considerarse como una estructura matriz que deberá adaptarse a las necesidades específicas de cada centro.

Published
2024
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232. Ertapenem for the treatment of bloodstream infections due to ESBL-producing Enterobacteriaceae: a multinational pre-registered cohort study

Author

Ministerio de Economía y Competitividad (España), Instituto de Salud Carlos III, European Commission, Red Española de Investigación en Patología Infecciosa, US Department of Veterans Affairs, Geriatric Research Education and Clinical Center (US), National Institute of Allergy and Infectious Diseases (US), National Institutes of Health (US), Gutiérrez-Gutiérrez, Belén, Bonomo, Robert A., Carmeli, Yehuda, Paterson, David L., Almirante, Benito, Martínez-Martínez, Luis, Oliver, Antonio, Calbo, Esther, Peña, Carmen, Akova, Murat, Pitout, Johann, Origüen, Julia, Pintado, Vicente, García Vázquez, Elisa, Gasch, Oriol, Hamprecht, Axel, Prim, Nuria, Tumbarello, Mario, Bou, Germán, Viale, Pierluigi, Tacconelli, Evelina, Almela, Manel, Pérez, Federico, Giamarellou, Helen, Cisneros, José Miguel, Schwaber, Mitchell J., Venditti, Mario, Lowman, Warren, Bermejo, Joaquín, Hsueh, Po-Ren, Mora-Rillo, Marta, Gracia-Ahufinger, Irene, Pascual, Álvaro, Rodríguez-Baño, Jesús, Ministerio de Economía y Competitividad (España), Instituto de Salud Carlos III, European Commission, Red Española de Investigación en Patología Infecciosa, US Department of Veterans Affairs, Geriatric Research Education and Clinical Center (US), National Institute of Allergy and Infectious Diseases (US), National Institutes of Health (US), Gutiérrez-Gutiérrez, Belén, Bonomo, Robert A., Carmeli, Yehuda, Paterson, David L., Almirante, Benito, Martínez-Martínez, Luis, Oliver, Antonio, Calbo, Esther, Peña, Carmen, Akova, Murat, Pitout, Johann, Origüen, Julia, Pintado, Vicente, García Vázquez, Elisa, Gasch, Oriol, Hamprecht, Axel, Prim, Nuria, Tumbarello, Mario, Bou, Germán, Viale, Pierluigi, Tacconelli, Evelina, Almela, Manel, Pérez, Federico, Giamarellou, Helen, Cisneros, José Miguel, Schwaber, Mitchell J., Venditti, Mario, Lowman, Warren, Bermejo, Joaquín, Hsueh, Po-Ren, Mora-Rillo, Marta, Gracia-Ahufinger, Irene, Pascual, Álvaro, and Rodríguez-Baño, Jesús

Abstract

[Objectives] Data about the efficacy of ertapenem for the treatment of bloodstream infections (BSI) due to ESBL-producing Enterobacteriaceae (ESBL-E) are limited. We compared the clinical efficacy of ertapenem and other carbapenems in monomicrobial BSI due to ESBL-E., [Methods] A multinational retrospective cohort study (INCREMENT project) was performed (ClinicalTrials.gov identifier: NCT01764490). Patients given monotherapy with ertapenem or other carbapenems were compared. Empirical and targeted therapies were analysed. Propensity scores were used to control for confounding; sensitivity analyses were performed in subgroups. The outcome variables were cure/improvement rate at day 14 and all-cause 30 day mortality., [Results] The empirical therapy cohort (ETC) and the targeted therapy cohort (TTC) included 195 and 509 patients, respectively. Cure/improvement rates were 90.6% with ertapenem and 75.5% with other carbapenems (P = 0.06) in the ETC and 89.8% and 82.6% (P = 0.02) in the TTC, respectively; 30 day mortality rates were 3.1% and 23.3% (P = 0.01) in the ETC and 9.3% and 17.1% (P = 0.01) in the TTC, respectively. Adjusted ORs (95% CI) for cure/improvement with empirical and targeted ertapenem were 1.87 (0.24–20.08; P = 0.58) and 1.04 (0.44–2.50; P = 0.92), respectively. For the propensity-matched cohorts it was 1.18 (0.43–3.29; P = 0.74). Regarding 30 day mortality, the adjusted HR (95% CI) for targeted ertapenem was 0.93 (0.43–2.03; P = 0.86) and for the propensity-matched cohorts it was 1.05 (0.46–2.44; P = 0.90). Sensitivity analyses were consistent except for patients with severe sepsis/septic shock, which showed a non-significant trend favouring other carbapenems., [Conclusions] Ertapenem appears as effective as other carbapenems for empirical and targeted therapy of BSI due to ESBL-E, but further studies are needed for patients with severe sepsis/septic shock.

Published
2016

233. Analysis of the role of the LH92_11085 gene of a biofilm hyper-producing Acinetobacter baumannii strain on biofilm formation and attachment to eukaryotic cells

Author

Instituto de Salud Carlos III, European Commission, Ministerio de Economía y Competitividad (España), Xunta de Galicia, Álvarez-Fraga, Laura, Pérez, Astrid, Rumbo-Feal, Soraya, Merino, María, Vallejo, Juan Andrés, Ohneck, Emily J., Edelmann, Richard E., Beceiro, Alejandro, Vázquez-Ucha, Juan C., Valle Turrillas, Jaione, Actis, L. A., Bou, Germán, Poza, Margarita, Instituto de Salud Carlos III, European Commission, Ministerio de Economía y Competitividad (España), Xunta de Galicia, Álvarez-Fraga, Laura, Pérez, Astrid, Rumbo-Feal, Soraya, Merino, María, Vallejo, Juan Andrés, Ohneck, Emily J., Edelmann, Richard E., Beceiro, Alejandro, Vázquez-Ucha, Juan C., Valle Turrillas, Jaione, Actis, L. A., Bou, Germán, and Poza, Margarita

Abstract

Acinetobacter baumannii is a nosocomial pathogen that has a considerable ability to survive in the hospital environment partly due to its capacity to form biofilms. The first step in the process of establishing an infection is adherence of the bacteria to target cells. Chaperone-usher pili assembly systems are involved in pilus biogenesis pathways that play an important role in adhesion to host cells and tissues as well as medically relevant surfaces. After screening a collection of strains, a biofilm hyper-producing A. baumannii strain (MAR002) was selected to describe potential targets involved in pathogenicity. MAR002 showed a remarkable ability to form biofilm and attach to A549 human alveolar epithelial cells. Analysis of MAR002 using transmission electron microscopy (TEM) showed a significant presence of pili on the bacterial surface. Putative protein-coding genes involved in pili formation were identified based on the newly sequenced genome of MAR002 strain (JRHB01000001/2 or NZ_JRHB01000001/2). As assessed by qRT-PCR, the gene LH92_11085, belonging to the operon LH92_11070-11085, is overexpressed (ca. 25-fold more) in biofilm-associated cells compared to exponential planktonic cells. In the present work we investigate the role of this gene on the MAR002 biofilm phenotype. Scanning electron microscopy (SEM) and biofilm assays showed that inactivation of LH92_11085 gene significantly reduced bacterial attachment to A549 cells and biofilm formation on plastic, respectively. TEM analysis of the LH92_11085 mutant showed the absence of long pili formations normally present in the wild-type. These observations indicate the potential role this LH92_11085 gene could play in the pathobiology of A baumannii.

Published
2016

234. Epidemiologic and Clinical Impact of Acinetobacter baumannii Colonization and Infection

Author

Villar, Macarena, Cano, María E., Gato, Eva, Garnacho-Montero, José, Miguel Cisneros, José, Ruíz de Alegría, Carlos, Fernández-Cuenca, Felipe, Martínez-Martínez, Luis, Vila, Jordi, Pascual, Alvaro, Tomás, María, Bou, Germán, and Rodríguez-Baño, Jesús

Subjects
Acinetobacter baumannii, Male, Cross Infection, Colistin, Incidence, Colony Count, Microbial, biochemical phenomena, metabolism, and nutrition, Middle Aged, bacterial infections and mycoses, Article, Anti-Bacterial Agents, Bacterial Typing Techniques, Electrophoresis, Gel, Pulsed-Field, Cohort Studies, Carbapenems, Spain, Drug Resistance, Bacterial, Humans, Female, Acinetobacter Infections, Aged
Abstract

Acinetobacter baumannii is one of the most important antibiotic-resistant nosocomial bacteria. We investigated changes in the clinical and molecular epidemiology of A. baumannii over a 10-year period. We compared the data from 2 prospective multicenter cohort studies in Spain, one performed in 2000 (183 patients) and one in 2010 (246 patients), which included consecutive patients infected or colonized by A. baumannii. Molecular typing was performed by repetitive extragenic palindromic polymerase chain reaction (REP-PCR), pulsed-field gel electrophoresis (PFGE), and multilocus sequence typing (MLST). The incidence density of A. baumannii colonization or infection increased significantly from 0.14 in 2000 to 0.52 in 2010 in medical services (p

Published
2014

240. Analysis of the role of the LH92_11085 gene of a biofilm hyper-producingAcinetobacter baumanniistrain on biofilm formation and attachment to eukaryotic cells

Author

Álvarez-Fraga, Laura, primary, Pérez, Astrid, additional, Rumbo-Feal, Soraya, additional, Merino, María, additional, Vallejo, Juan Andrés, additional, Ohneck, Emily J., additional, Edelmann, Richard E., additional, Beceiro, Alejandro, additional, Vázquez-Ucha, Juan C., additional, Valle, Jaione, additional, Actis, Luis A., additional, Bou, Germán, additional, and Poza, Margarita, additional

Published
2016
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241. Comprehensive clinical and epidemiological assessment of colonisation and infection due to carbapenemase-producing Enterobacteriaceae in Spain

Author

Palacios-Baena, Zaira R., primary, Oteo, Jesús, additional, Conejo, Carmen, additional, Larrosa, M. Nieves, additional, Bou, Germán, additional, Fernández-Martínez, Marta, additional, González-López, Juan José, additional, Pintado, Vicente, additional, Martínez-Martínez, Luis, additional, Merino, María, additional, Pomar, Virginia, additional, Mora-Rillo, Marta, additional, Rivera, María Alba, additional, Oliver, Antonio, additional, Ruiz-Carrascoso, Guillermo, additional, Ruiz-Garbajosa, Patricia, additional, Zamorano, Laura, additional, Bautista, Verónica, additional, Ortega, Adriana, additional, Morales, Isabel, additional, Pascual, Álvaro, additional, Campos, José, additional, Rodríguez-Baño, Jesús, additional, Zaballos, Ángel, additional, Cantón, Rafael, additional, Martínez-García, Laura, additional, Fleites, Ana María, additional, Rodríguez-Lucas, Carlos, additional, Sánchez-Romero, Ma Isabel, additional, García-Picazo, Luisa, additional, Aznar, Esteban, additional, Campelo, Carolina, additional, González-Praetorius, Alejandro, additional, Solís, Sonia, additional, Giner, Salvador, additional, Salavert, Miguel, additional, Hernández, Juan Manuel, additional, Pujals, Josep Vilaró, additional, Bastarras, Anna Vilamala, additional, Orellana, Ma Ángeles, additional, Cercenado, Emilia, additional, Espasa, Mateu, additional, Fontanals, Dionisia, additional, García-López, Ma Victoria, additional, Hernández-Almaraz, José Luis, additional, Martí-Sala, Carmina, additional, Gimeno, Adelina, additional, Alarcón, Teresa, additional, Llorca, Laura, additional, Segura, Concepción, additional, Clivillé-Abad, Raquel, additional, Motjé, Montse, additional, Garcia i Parés, Delia, additional, de la Iglesia, Pedro, additional, Iglesias, Beatriz, additional, Castón, Juanjo, additional, Romero, María Dolores, additional, Rodríguez-Polo, José Antonio, additional, Trujillo, Gloria, additional, Morta, Montserrat, additional, Setas, Alberto Gil, additional, Ezpeleta, Carmen, additional, Miguel-Martínez, Ma Dolores, additional, Sánchez-Porto, Antonio, additional, Casas, Javier, additional, Molina, David, additional, Garduño, Eugenio, additional, Alados, Juan Carlos, additional, Pérez-Jové, Pepa, additional, Sauca, Goretti, additional, Gallés, Carmen, additional, Galánand, Fátima, additional, Guerrero, Francisca, additional, Brezmes, Ma Fe, additional, Ortega, Ma Pilar, additional, Castillo, Francisco Javier, additional, Seral, Cristina, additional, Delgado-Iribarren, Alberto, additional, Yagüe, Alberto, additional, Aspiroz, Carmen, additional, Fernández-Natal, Ma Isabel, additional, Wilhelmi, Isabel, additional, Reyes, Pilar, additional, Pérez-Ramírez, Ma Dolores, additional, Cuesta, Inocente, additional, Pérez Moreno, Mar Olga, additional, García, Amparo, additional, Ballester, Frederic, additional, Pujol, Isabel, additional, Sierra, Montserrat, additional, González-Cuevas, Araceli, additional, García, Pilar López, additional, Saladrigas, Lluís Carbó, additional, Martínez-López, Jesús, additional, Martínez-Lamas, Lucía, additional, Cabrera, Jorge Julio, additional, de Cruz, Susana García, additional, Raya, Carmen, additional, Campo, Ana Belén, additional, de Benito, Inés, additional, Canut, Andrés, additional, Berdonces, Pilar, additional, Lecaroz Agara, María Concepción, additional, Real, Susana Hernando, additional, Hernández, Belén, additional, Ledo, Ma Teresa, additional, El Knaichi, Firdaous, additional, Tejero, Carlos García, additional, Azcona, Jose Manuel, additional, Ferrer, Isabel, additional, Lamata, Marta, additional, Pazos, Carmen, additional, Chocarro, Ma Pilar, additional, Murillas, Javier, additional, Miró, Elisenda, additional, Navarro, Ferrán, additional, and Bartolomé, Rosa M., additional

Published
2016
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244. Mobile genetic elements related to the diffusion of plasmid-mediated AmpC β-lactamases or carbapenemases from enterobacteriaceae: Findings from a multicenter study in Spain

Author

Universidad de Sevilla. Departamento de Microbiología, Conejo Gonzalo, Mª Carmen, Zamorano, Laura, Miró, Elisenda, Juan, Carlos, Gómez Martínez, Laura E., Bou, Germán, González López, Juan José, Martínez Martínez, Luis, Universidad de Sevilla. Departamento de Microbiología, Conejo Gonzalo, Mª Carmen, Zamorano, Laura, Miró, Elisenda, Juan, Carlos, Gómez Martínez, Laura E., Bou, Germán, González López, Juan José, and Martínez Martínez, Luis

Abstract

We examined the genetic context of 74 acquired ampC genes and 17 carbapenemase genes from 85 of 640 Enterobacteriaceae isolates collected in 2009. Using S1 pulsed-field gel electrophoresis and Southern hybridization, 37 of 74 blaAmpC genes were located on large plasmids of different sizes belonging to six incompatibility groups. We used sequencing and PCR mapping to investigate the regions flanking the acquired ampC genes. The blaCMY-2-like genes were associated with ISEcp1; the surrounding blaDHA genes were similar to Klebsiella pneumoniae plasmid pTN60013 associated with IS26 and the psp and sap operons; and the blaACC-1 genes were associated with IS26 elements inserted into ISEcp1. All of the carbapenemase genes (blaVIM-1, blaIMP-22, and blaIMP-28) were located in class 1 integrons. Therefore, although plasmids are the main cause of the rapid dissemination of ampC genes among Enterobacteriaceae, we need to be aware that other mobile genetic elements, such as insertion sequences, transposons, or integrons, can be involved in the mobilization of these genes of chromosomal origin. Additionally, three new integrons (In846 to In848) are described in this study.

Published
2015

245. Prospective multicenter study of carbapenemase-producing Enterobacteriaceae from 83 hospitals in Spain reveals high in vitro susceptibility to colistin and meropenem

Author

Universidad de Sevilla. Departamento de Microbiología, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (MINECO). España, Conejo Gonzalo, Mª Carmen, Pascual Hernández, Álvaro, Otero, Jesús, Ortega, Adriana, Bartolomé, Rosa M., Bou, Germán, Fernández Martínez, Marta, González López, Juan José, Universidad de Sevilla. Departamento de Microbiología, Instituto de Salud Carlos III, Ministerio de Economía y Competitividad (MINECO). España, Conejo Gonzalo, Mª Carmen, Pascual Hernández, Álvaro, Otero, Jesús, Ortega, Adriana, Bartolomé, Rosa M., Bou, Germán, Fernández Martínez, Marta, and González López, Juan José

Abstract

The aim of this study was to determine the impact of carbapenemase-producing Enterobacteriaceae (CPE) in Spain in 2013 by describing the prevalence, dissemination, and geographic distribution of CPE clones, and their population structure and antibiotic susceptibility. From February 2013 to May 2013, 83 hospitals (about 40,000 hospital beds) prospectively collected nonduplicate Enterobacteriaceae using the screening cutoff recommended by EUCAST. Carbapenemase characterization was performed by phenotypic methods and confirmed by PCR and sequencing. Multilocus sequencing types (MLST) were determined for Klebsiella pneumoniae and Escherichia coli. A total of 702 Enterobacteriaceae isolates met the inclusion criteria; 379 (54%) were CPE. OXA-48 (71.5%) and VIM-1 (25.3%) were the most frequent carbapenemases, and K. pneumoniae (74.4%), Enterobacter cloacae (10.3%), and E. coli (8.4%) were the species most affected. Susceptibility to colistin, amikacin, and meropenem was 95.5%, 81.3%, and 74.7%, respectively. The most prevalent sequence types (STs) were ST11 and ST405 for K. pneumoniae and ST131 for E. coli. Forty-five (54.1%) of the hospitals had at least one CPE case. For K. pneumoniae, ST11/OXA-48, ST15/OXA-48, ST405/OXA-48, and ST11/VIM-1 were detected in two or more Spanish provinces. ST11 isolates carried four carbapenemases (VIM-1, OXA-48, KPC-2, and OXA-245), but ST405 isolates carried OXA-48 only. A wide interregional spread of CPE in Spain was observed, mainly due to a few successful clones of OXA-48-producing K. pneumoniae (e.g., ST11 and ST405). The dissemination of OXA-48-producing E. coli is a new finding of public health concern. According to the susceptibilities determined in vitro, most of the CPE (94.5%) had three or more options for antibiotic treatment

Published
2015

246. N-acetylcysteine selectively antagonizes the activity of imipenem in Pseudomonas aeruginosa by an OprD-mediated mechanism

Author

Universidad de Sevilla. Departamento de Microbiología, Ministerio de Ciencia e Innovación (MICIN). España, Rodríguez Beltrán, Jerónimo, Cabot, Gabriel, Ynés Valencia, Estela, Costas, Coloma, Bou, Germán, Oliver, Antonio, Blázquez, Jesús, Universidad de Sevilla. Departamento de Microbiología, Ministerio de Ciencia e Innovación (MICIN). España, Rodríguez Beltrán, Jerónimo, Cabot, Gabriel, Ynés Valencia, Estela, Costas, Coloma, Bou, Germán, Oliver, Antonio, and Blázquez, Jesús

Abstract

The modulating effect of N-acetylcysteine (NAC) on the activity of different antibiotics has been studied in Pseudomonas aeruginosa. Our results demonstrate that, in contrast to previous reports, only the activity of imipenem is clearly affected by NAC. MIC and checkerboard determinations indicate that the NAC-based modulation of imipenem activity is dependent mainly on OprD. SDS-PAGE of outer membrane proteins (OMPs) after NAC treatments demonstrates that NAC does not modify the expression of OprD, suggesting that NAC competitively inhibits the uptake of imipenem through OprD. Similar effects on imipenem activity were obtained with P. aeruginosa clinical isolates. Our results indicate that imipenem-susceptible P. aeruginosa strains become resistant upon simultaneous treatment with NAC and imipenem. Moreover, the generality of the observed effects of NAC on antibiotic activity was assessed with two additional bacterial species, Escherichia coli and Acinetobacter baumannii. Caution should be taken during treatments, as the activity of imipenem may be modified by physiologically attainable concentrations of NAC, particularly during intravenous and nebulized regimes.

Published
2015

249. Epidemiological and Clinical Complexity of Amoxicillin-Clavulanate- Resistant Escherichia coli

Author

Rodríguez-Baño, Jesús, Oteo, Jesús, Ortega, Adriana, Villar, Macarena, Conejo Gonzalo, Mª Carmen, Bou, Germán, Aranzamendi-Zaldumbide, Maitane, Cercenado, Emilia, Gurguí, Mercè, Martínez-Martínez, Luis, Merino, María, Rivera, Alba, Oliver, Antonio, Weber, Irene, Pascual Hernández, Álvaro, Bartolomé, Rosa M., Gónzalez López, Juan José, Campos, José, Universidad de Sevilla. Departamento de Medicina, and Universidad de Sevilla. Departamento de Microbiología

Subjects
musculoskeletal diseases, Estudio Multicéntrico, Antibacterianos, Infección Hospitalaria, Resistencia beta-Lactámica, polycyclic compounds, Escherichia coli, bacteria, biochemical phenomena, metabolism, and nutrition, Infecciones Urinarias
Abstract

Two hundred twelve patients with colonization/infection due to amoxicillin-clavulanate (AMC)-resistant Escherichia coli were studied. OXA-1- and inhibitor-resistant TEM (IRT)-producing strains were associated with urinary tract infections, while OXA-1 producers and chromosomal AmpC hyperproducers were associated with bacteremic infections. AMC resistance in E. coli is a complex phenomenon with heterogeneous clinical implications.

Published
2013

250. First Report of an OXA-23 Carbapenemase-Producing Acinetobacter baumannii Clinical Isolate Related to Tn2006 in Spain

Author

Espinal, P., Macià, M. D., Roca, I., Fernández-Cuenca, Felipe, Oliver, A., Rodríguez-Baño, Jesús, Bou, Germán, Tomás, M., Villa, J., and Universidad de Sevilla. Departamento de Medicina

Subjects
polycyclic compounds, bacteria, biochemical phenomena, metabolism, and nutrition, bacterial infections and mycoses
Abstract

A carbapenem-resistant Acinetobacter baumannii clinical isolate belonging to European clone II and sequence type 2 was recov-ered from a patient in the Son Espases hospital in Mallorca, Spain. Genetic analysis showed the presence of the bla OXA-23 gene in association with the widely disseminated transposon Tn2006. This is the first reported identification of A. baumannii carrying bla OXA-23 in Spain.

Published
2013

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