Your search keyword '"Jacquier, Hervé"' showing total 7 results

1. Massive Increase, Spread, and Exchange of Extended Spectrum β-Lactamase—Encoding Genes Among Intestinal Enterobacteriaceae in Hospitalized Children With Severe Acute Malnutrition in Niger

Author

Woerther, Paul-Louis, Angebault, Cécile, Jacquier, Hervé, Hugede, Henri-Charles, Janssens, Ann-Carole, Sayadi, Sani, Mniai, Assiya El, Armand-Lefèvre, Laurence, Ruppé, Etienne, Barbier, François, Raskine, Laurent, Page, Anne-Laure, de Rekeneire, Nathalie, and Andremont, Antoine

Published

2011

2. Emergence and Dissemination of Extended-Spectrum β-Lactamase—Producing Escherichia coli in the Community: Lessons from the Study of a Remote and Controlled Population

Author

Woerther, Paul-Louis, Angebault, Cécile, Lescat, Mathilde, Ruppé, Etienne, Skurnik, David, Mniai, Assiya El, Clermont, Olivier, Jacquier, Hervé, Costa, Anaelle Da, Renard, Magaly, Bettinger, Régis Marc, Epelboin, Loïc, Dupont, Claire, Guillemot, Didier, Rousset, François, Arlet, Guillaume, Denamur, Erick, Djossou, Félix, and Andremont, Antoine

Published

2010

3. Performance of commercial methods for linezolid susceptibility testing of Enterococcus faecium and Enterococcus faecalis.

Author

Dejoies, Loren, Boukthir, Sarrah, Péan de Ponfilly, Gauthier, Le Guen, Ronan, Zouari, Asma, Potrel, Sophie, Collet, Anaïs, Auger, Gabriel, Jacquier, Hervé, Fihman, Vincent, Dortet, Laurent, and Cattoir, Vincent

Subjects

RESEARCH, ENTEROCOCCUS faecium, RESEARCH methodology, MEDICAL cooperation, EVALUATION research, GRAM-positive bacterial infections, COMPARATIVE studies, ENTEROCOCCUS, DRUG resistance in microorganisms, ANTIBIOTICS, MICROBIAL sensitivity tests, PHARMACODYNAMICS

Abstract

Background: Linezolid-resistant enterococci (LRE) causing infections that are challenging to treat are rising, highlighting the need for reliable screening of LRE clinical isolates.Objectives: To evaluate the ability of the broth microdilution (BMD) method for LRE detection and to assess the performance of seven commercially available techniques for linezolid susceptibility testing.Methods: A collection of 100 clinical isolates (80 Enterococcus faecium and 20 Enterococcus faecalis), including 20 optrA-positive isolates, 17 poxtA-positive isolates and 1 optrA/poxtA-positive E. faecium isolate, were studied. MICs were determined after 18 h [Day 1 (D1)] and 42 h [Day 2 (D2)] of incubation and interpreted following EUCAST and CLSI guidelines, which currently provide different interpretative breakpoints. Performance of commercial techniques was compared with BMD results.Results: MIC50/D1 and MIC50/D2 were both 8 mg/L, while MIC90/D1 and MIC90/D2 were 16 and 32 mg/L, respectively. MICD1 values for poxtA-positive isolates were lower than those for optrA-positive isolates. Proportions of susceptible isolates at D1 and D2 were 48% and 41%, respectively, according to EUCAST breakpoints and 35% and 13%, respectively, according to CLSI criteria (the proportions of isolates categorized as intermediate following CLSI recommendations were 13% and 28% at D1 and D2, respectively). Percentage susceptibility assessed by the commercially available techniques was always higher. The four commercial methods allowing MIC determination provided an overall essential agreement of ≥90% at D1. Categorical agreement and error rates were generally improved at D2.Conclusions: Non-automated methods (Sensititre and UMIC) and, to a lesser extent, gradient strip Etest appear to show an acceptable correlation with the BMD reference method for the detection of isolates with low MICs of linezolid after prolonged incubation. [ABSTRACT FROM AUTHOR]

Published

2020

4. Genomic characterization of 16S rRNA methyltransferase-producing Escherichia coli isolates from the Parisian area, France.

Author

Caméléna, François, Morel, Florence, Merimèche, Manel, Decousser, Jean-Winoc, Jacquier, Hervé, Clermont, Olivier, Darty, Mélanie, Mainardis, Mary, Cambau, Emmanuelle, Tenaillon, Olivier, Denamur, Erick, Berçot, Béatrice, Group, the IAME Resistance, and IAME Resistance Group

Subjects

ESCHERICHIA coli, RESEARCH, BIOLOGICAL evolution, RESEARCH methodology, RNA, MEDICAL cooperation, EVALUATION research, HYDROLASES, COMPARATIVE studies, GENOMICS, GENES, TRANSFERASES, DRUG resistance in microorganisms, MICROBIAL sensitivity tests, ANTIBIOTICS, PHARMACODYNAMICS

Abstract

Background: The resistance to all aminoglycosides (AGs) conferred by 16S rRNA methyltransferase enzymes (16S-RMTases) is a major public health concern.Objectives: To characterize the resistance genotype, its genetic environment and plasmid support, and the phylogenetic relatedness of 16S-RMTase-producing Escherichia coli from France.Methods: We screened 137 E. coli isolates resistant to all clinically relevant AGs from nine Parisian hospitals for 16S-RMTases. WGS was performed on clinical isolates with high-level AG resistance (MIC ≥256 mg/L) and their transformants.Results: Thirty of the 137 AG-resistant E. coli produced 16S-RMTases: 11 ArmA, 18 RmtB and 1 RmtC. The 16S-RMTase producers were also resistant to third-generation cephalosporins (90% due to a blaCTX-M gene), co-trimoxazole, fluoroquinolones and carbapenems (blaNDM and blaVIM genes) in 97%, 83%, 70% and 10% of cases, respectively. Phylogenomic diversity was high in ArmA producers, with 10 different STs, but a similar genetic environment, with the Tn1548 transposon carried by a plasmid closely related to pCTX-M-3 in 6/11 isolates. Conversely, RmtB producers belonged to 12 STs, the most frequent being ST405 and ST complex (STc) 10 (four and four isolates, respectively). The rmtB gene was carried by IncF plasmids in 10 isolates and was found in different genetic environments. The rmtC gene was carried by the pNDM-US plasmid.Conclusions: ArmA and RmtB are the predominant 16S-RMTases in France, but their spread follows two different patterns: (i) dissemination of a conserved genetic support carrying armA in E. coli with high levels of genomic diversity; and (ii) various genetic environments surrounding rmtB in clonally related E. coli. [ABSTRACT FROM AUTHOR]

Published

2020

5. Molecular epidemiology and mechanisms of resistance of azithromycin-resistant Neisseria gonorrhoeae isolated in France during 2013-14.

Author

Belkacem, Anna, Jacquier, Hervé, Goubard, Agathe, Mougari, Faiza, La Ruche, Guy, Patey, Olivier, Micaëlo, Maïté, Semaille, Caroline, Cambau, Emmanuelle, and Bercot, Béatrice

Subjects

*DISEASE prevalence, *AZITHROMYCIN, *DRUG resistance in microorganisms, *NEISSERIA gonorrhoeae, *DISEASE susceptibility, *ANTIBIOTICS, *CLUSTER analysis (Statistics), *GONORRHEA, *MOLECULAR epidemiology, *GENETIC mutation, *NEISSERIA, *POLYMERASE chain reaction, *SEQUENCE analysis, *GENOTYPES, *PHARMACODYNAMICS

Abstract

Objectives: The objective of this study was to determine the prevalence and mechanisms of azithromycin resistance of Neisseria gonorrhoeae French isolates from 2013 to 2014.Methods: N. gonorrhoeae samples isolated in a network of laboratories were tested for susceptibility to azithromycin between April 2013 and March 2014. Fifty-four isolates that were non-susceptible to azithromycin and 18 susceptible isolates were characterized for molecular mechanisms of resistance by PCR/sequencing and genotyped using N. gonorrhoeae multiantigen sequence typing (NG-MAST).Results: Among the 970 N. gonorrhoeae isolates, 54 (5.56%) were non-susceptible to azithromycin, 9 (1%) were resistant and 45 (4.6%) showed intermediate resistance. Azithromycin-non-susceptible isolates harboured a C2599T mutation in the rrl gene encoding the 23S rRNA alleles (5.5%), a C substitution in the mtrR promoter (5.5%), an A deletion in the mtrR promoter (53.7%) and mutations in the L4 ribosomal protein (14.8%) and in the MtrR repressor (25.9%). No isolates showed an L22 mutation or carried an erm, ere, mef(A)/(E) or mphA gene. Thirty different STs were highlighted using the NG-MAST technique. The predominant genogroups non-susceptible to azithromycin were G21 (31%), G1407 (20%) and G2400 (15%). Genogroup G2400 (15%) was revealed to be a novel cluster prevalent in the south of France and resistant to azithromycin, ciprofloxacin and tetracycline.Conclusions: Our study highlights that the prevalence of resistance of N. gonorrhoeae to azithromycin in France is low and essentially due to multiple genetic mutations. Its dissemination occurs through three major genogroups including a novel one in France (G2400). [ABSTRACT FROM AUTHOR]

Published

2016

6. Capturing the mutational landscape of the beta-lactamase TEM-1.

Author

Jacquier, Hervé, Birgy, André, Le Nagard, Hervé, Mechulam, Yves, Schmitt, Emmanuelle, Glodt, Jérémy, Bercot, Beatrice, Petit, Emmanuelle, Poulain, Julie, Barnaud, Guilène, Gros, Pierre-Alexis, and Tenaillon, Olivier

Subjects

*GENETIC mutation, *BETA lactamases, *TRANSMISSION electron microscopy, *ENZYMES, *ANTIBIOTICS, *AMOXICILLIN

Abstract

Adaptation proceeds through the selection of mutations. The distribution of mutant fitness effect and the forces shaping this distribution are therefore keys to predict the evolutionary fate of organisms and their constituents such as enzymes. Here, by producing and sequencing a comprehensive collection of 10,000 mutants, we explore the mutational landscape of one enzyme involved in the spread of antibiotic resistance, the beta-lactamase TEM-1. We measured mutation impact on the enzyme activity through the estimation of amoxicillin minimum inhibitory concentration on a subset of 990 mutants carrying a unique missense mutation, representing 64% of possible amino acid changes in that protein reachable by point mutation. We established that mutation type, solvent accessibility of residues, and the predicted effect of mutations on protein stability primarily determined alone or in combination changes in minimum inhibitory concentration of mutants. Moreover, we were able to capture the drastic modification of the mutational landscape induced by a single stabilizing point mutation (M182T) by a simple model of protein stability. This work thereby provides an integrated framework to study mutation effects and a tool to understand/define better the epistatic interactions. [ABSTRACT FROM AUTHOR]

Published

2013

7. Genetic and Phenotypic Study of the Pectobacterium versatile Beta-Lactamase, the Enzyme Most Similar to the Plasmid-Encoded TEM-1.

Author

Royer, Guilhem, Dixit, Zoya, Pédron, Jacques, Pierrat, Gautier, Demontant, Vanessa, Berçot, Béatrice, Rodriguez, Christophe, Barny, Marie-Anne, Jacquier, Hervé, and Woerther, Paul-Louis

Subjects

*ERWINIA, *PHENOTYPES, *GENETIC distance, *BETA lactamases, *ENZYMES, *ANTIBIOTICS

Abstract

Genus Pectobacterium bacteria include important agricultural pathogens. Pectobacterium versatile isolates contain a chromosome-borne beta-lactamase, PEC-1. This enzyme is the closest relative of TEM-1, a plasmid-borne beta-lactamase widespread in the Enterobacterales. We performed bioinformatics and phenotypic analyses to investigate the genetic and phenotypic features of PEC-1 and its frequency and ability to spread within genus Pectobacterium. We also compared the characteristics of PEC-1 and TEM-1 and evaluated the likelihood of transfer. We found that blaPEC-1 was present principally in a small number of genetic environments in P. versatile. Identical blaPEC-1 genetic environments were present in closely related species, consistent with the high frequency of genetic exchange within the genus Pectobacterium. Despite the similarities between PEC-1 and TEM-1, their genetic environments displayed no significant identity, suggesting an absence of recent transfer. Phenotypic analyses on clonal constructs revealed similar hydrolysis spectra. Our results suggest that P. versatile is the main reservoir of PEC-1, which seems to transfer to closely related species. The genetic distance between PEC-1 and TEM-1, and the lack of conserved elements in their genetic environments, suggest that any transfer that may have occurred must have taken place well before the antibiotic era. [ABSTRACT FROM AUTHOR]

Published

2022