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2. Toxicity and genotoxicity of antimalarial alkaloid rich extracts derived fromMitragyna inermis O. Kuntze andNauclea latifolia

Author

Michèle Laget, P. Timon-David, C. Di Giorgio, H. Guiraud, F. Traore, O. Doumbo, Monique Gasquet, and Nadine Azas

Subjects
Pharmacology, Rubiaceae, Nauclea, biology, Traditional medicine, Alkaloid, Mutagen, Pharmacognosy, biology.organism_classification, medicine.disease_cause, In vivo, medicine, Medicinal plants, Genotoxicity
Abstract

The toxicity and the genotoxicity of antimalarial alkaloid rich extracts derived from two plants used in traditional medicine in Mali (Mitragyna inermis (Willd.) O. Kuntze Rubiaceae and Nauclea latifolia (Sm.) Rubiaceae) were evaluated on in vitro and in vivo systems. The results demonstrated that an alkaloid rich extract derived from M. inermis induced a strong inhibition of protein synthesis in mammalian cells but did not exhibit mutagenic or genotoxic activity. An alkaloid rich extract derived from N. latifolia could interact in vitro with DNA of bacteria and mammalian cells, leading to G2-M cell cycle arrest and herita­ ble DNA-damage, as well as inducing in vivo single-strand breaks in liver, kidney and blood cells. Copy­ right © 2000 John Wiley & Sons, Ltd.

Published
2000
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3. The protective activity of α-hederine against H2O2 genotoxicity in HepG2 cells by alkaline comet assay

Author

M De Méo, C Mba Gachou, Michèle Laget, H. Guiraud-Dauriac, Gérard Duménil, and R. Elias

Subjects
Antioxidant, Health, Toxicology and Mutagenesis, medicine.medical_treatment, Protective Agents, medicine.disease_cause, chemistry.chemical_compound, Tumor Cells, Cultured, Genetics, medicine, Humans, Oleanolic Acid, Electrophoresis, Agar Gel, Dose-Response Relationship, Drug, biology, Mutagenicity Tests, Cell Membrane, Proteins, DNA, Neoplasm, Hydrogen Peroxide, Glutathione, Saponins, Carbohydrate, Catalase, Molecular biology, Comet assay, chemistry, Biochemistry, Toxicity, biology.protein, Oxidation-Reduction, Antimutagen, Genotoxicity, DNA Damage
Abstract

This study was designed to evaluate the protective effect of alpha-hederine (alpha-hed) against H2O2-mediated DNA damage on HepG2 cell line by the alkaline comet assay. For the protective effect of alpha-hed study, cells were treated according to three protocols: pre-treatment, simultaneous treatment and post-treatment. The effect of alpha-hed on catalase activity was evaluated after treating the cells with 3.36 mg/ml of 3-amino-1,2,4-triazole (AMT) singly or in combination with alpha-hed (1.5 or 3 microg/ml) and H2O2 (8.8 microM) during 1 h. The catalase activity was also biochemically measured after treating cells with alpha-hed at 1.5, 3, or 15 microg/ml during 1 h. Additionally, the influence of alpha-hed on membrane RedOx potential, pool of reduced glutathione and total protein content was evaluated by flow cytometry. In the pre-treatment, the two concentrations of alpha-hed (1.5 and 3 microg/ml) decreased the lesions induced by H2O2 (8.8 microM) significantly. This decrease was about 57.2% and 66.1%, respectively. Similar results were observed when cells were treated with alpha-hed and H2O2 simultaneously. The decrease of H2O2-induced lesions was about 78.2% and 83.2% (alpha-hed 1.5 and 3 microg/ml, respectively). In the post-treatment protocol, this decrease was not significant. The combination of AMT and H2O2 induced more DNA damage than H2O2 alone (tail moment (TM) means was 31.4% and 21.8%, respectively). When alpha-hed was added to this mixture, TM means were reduced significantly (17.4% for alpha-hed 1. 5 microg/ml and 15.5% for alpha-hed 3 microg/ml). Up to 6.9 microg/ml, alpha-hed enhanced catalase activity (60.5%), followed by a decrease of the activity. Total protein content and membrane RedOx potential were slightly increased up to 11 microg/ml (14% and 3.6%, respectively) followed by a drop and a plateau. Pool of reduced glutathione remained unchanged up to 10 microg/ml then dropped and reached a plateau. In conclusion, alpha-hed could exert its protective effect against H2O2-mediated DNA damage by scavenging free radicals or by enhancing the catalase activity.

Published
1999
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4. Evaluation of the mutagenicity and antimutagenicity of forty-two 3-substituted flavones in the Ames test

Author

C. Beudot, Michèle Laget, Guy Balansard, M De Méo, R. Elias, Gérard Duménil, D. Dauzonne, and H. Guiraud

Subjects
Flavonoids, Salmonella typhimurium, chemistry.chemical_classification, endocrine system, Mutagenicity Tests, Chemistry, Stereochemistry, Health, Toxicology and Mutagenesis, fungi, Mutagenesis, food and beverages, Antimutagenic Agents, Flavones, Ames test, Toxicology, Nitroreductase, chemistry.chemical_compound, Polyphenol, Acetyltransferase, Genetics, Pyrene, Antimutagen, Mutagens
Abstract

The mutagenic and antimutagenic activities of forty-two synthetic flavones were assessed by the Ames test. The tested flavones included twenty-three 3-nitroflavones, eighteen 3-aminoflavones and the 3-chloroflavone. The mutagenicity was evaluated with Salmonella typhimurium TA100 and YG1042 (an overproducing nitroreductase and O -acetyltransferase TA100 strain) with and without metabolic activation (S9 mix). The antimutagenicity of the non mutagenic derivatives was evaluated against 11 known reference mutagens. A total of 39 synthetic flavones were mutagenic. The mutagenic activities ranged from 0.1 rev/nmole (4′-chloro-6-methoxy-3-nitroflavone) to 6240 rev/nmole (4′-methoxy-3,3′-diaminoflavone). Two differences were found between the 3-amino and the 3-nitroflavones: (i) the mutagenicity of the 3-aminoflavones required the presence of the metabolic activation; (ii) the 3-amino derivatives were more mutagenic than their 3-nitro counterparts. Increased mutagenicity, as assessed with strain YG1042, was limited to 17/39 derivatives. The mutagenic activity was induced by the presence of the double bond at the 2,3-position for conjugation of the lone-pair electron with the carbonyl group on the `C' ring. This mutagenicity was modulated by substituents at the 2′-position. Additional mutagenicity was brought by the aminoaromatic and nitroaromatic group reduction by bacterial nitroreductases and by the S9 mix; it was modulated by different substituents on the aromatic rings of the flavones. Three flavones: 3-chloroflavone ( 1C ), 4′-hydroxy-3-nitroflavone ( 23N ) and 2′,3-diaminoflavone ( 2A ) showed antimutagenic properties. Compound 1C was efficient against benzo( a )pyrene (BaP), 2-aminofluorene (2AF), 2-aminoanthracene (2AA), 4-nitroquinoline-1-oxide (4NQO) and 1-methyl-3′-nitro-1-nitrosoguanidine (MNNG). Compound 23N inhibited the mutagenicity of BaP and MNNG. The antimutagenic activity of 2A was limited to MNNG.

Published
1998
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5. Evaluation of a flow cytofluorometric method for rapid determination of amphotericin B susceptibility of yeast isolates

Author

Christiane Chastin, F Peyron, H. Guiraud-Dauriac, P Regli, M El Mzibri, A Favel, and Gérard Duménil

Subjects
Antifungal Agents, Time Factors, Microbial Sensitivity Tests, Microbiology, Flow cytometry, Amphotericin B, medicine, Pharmacology (medical), IC50, Candida, Pharmacology, Reproducibility, Chromatography, biology, medicine.diagnostic_test, Computers, Fungi imperfecti, Flow Cytometry, biology.organism_classification, Yeast, Fluorescence intensity, Infectious Diseases, Evaluation Studies as Topic, Candida spp, Regression Analysis, Research Article, medicine.drug
Abstract

A rapid-flow cytofluorometric susceptibility test for in vitro amphotericin B testing of yeasts was evaluated and compared to the National Committee for Clinical Laboratory Standards (NCCLS) M27-T reference broth macrodilution method. The flow cytofluorometric method is based on the detection of decreased green fluorescence intensity of cells stained with DiOC5(3), a membrane potential-sensitive cationic dye, after drug treatment. Testing was performed on 134 clinical isolates (Candida spp. and Torulopsis glabrata). From the dose-response curve obtained for each isolate, three endpoints were calculated by computer analysis (the concentrations at which the fluorescence intensity was reduced by 50, 80, and 90%, i.e., 50% inhibitory concentration [IC50], IC80, and IC90, respectively). A regression analysis correlating these endpoints with the M27-T MICs showed that the best agreement was obtained with IC80. The flow cytofluorometric method showed good reproducibility with control strains. These initial results suggest that the flow cytofluorometric method is a valid alternative to the NCCLS reference method.

Published
1997
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6. [Untitled]

Author

Gérard Duménil, M. De Méo, H. Guiraud-Dauriac, C. Beudot, Michèle Laget, and M. El Mzibri

Subjects
Salmonella, Reporter gene, medicine.diagnostic_test, Mutagen, Biology, medicine.disease_cause, biology.organism_classification, Applied Microbiology and Biotechnology, Biochemistry, Enterobacteriaceae, Molecular biology, Flow cytometry, Flow cytometry technique, medicine, Carcinogen, Bacteria
Abstract

The Salmonella sulA-test using Salmonella typhimurium TA1538/pEM1968 ( sulA:: lacZ) is a new SOS-repair inducing system that detects mutagens and carcinogens. The b-galactosidase activity, currently detected by colorimetric dosage, can be measured by flow cytometry using a fluorescent substrate (fluorescein-di-b-D-galactopyranoside). Comparison of the dose-response relationships of eight chemicals determined by the two techniques showed that the Salmonella sulA-test combined with the flow cytometry technique was accurate and reliable as it covered a large number of cells in a short time.

Published
1997
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7. Adsorption of phage λ to Salmonella typhimurium lamB + requires the presence of lipopolysaccharide in the outer membrane

Author

Michèle Laget, H. Guiraud, C. Beudot, M. El Mzibri, M. De Méo, and Gérard Duménil

Subjects
Expression vector, Strain (chemistry), biology, Lipopolysaccharide, Bioengineering, General Medicine, Lambda phage, biology.organism_classification, Applied Microbiology and Biotechnology, Enterobacteriaceae, Molecular biology, Bacteriophage, chemistry.chemical_compound, chemistry, Membrane protein, Bacterial outer membrane, Biotechnology
Abstract

Two S. typhimurium strains TA1534 (rfa+) and TA1538 (rfaE) were transformed with the lamB expression plasmid pAMH70. Transposition events with λplacMu55 hybrid phage were successful only with TA1534/pAMH70 strain. Using SDS-PAGE, the LamB protein was present in the total cell proteins but not in the outer membrane proteins of the TA1538/pAMH70 strain. The LamB protein must linked to the LPS of the outer membrane to allow adsorption of λ phage in S. typhimurium.

Published
1996
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8. Optimization of the Salmonella/mammalian microsome assay for urine mutagenesis by experimental designs

Author

Alain Botta, Marcel Castegnaro, H. Guiraud, Michèle Laget, C. Di Giorgio, M. De Meo, and Gérard Duménil

Subjects
Salmonella typhimurium, Salmonella, Chromatography, Dose-Response Relationship, Drug, Mutagenicity Tests, Chemistry, Smoking, Fractional factorial design, Urine, Toxicology, medicine.disease_cause, Ames test, Dose–response relationship, Volume (thermodynamics), Predictive Value of Tests, Research Design, Microsomes, Liver, Genetics, medicine, Microsome, Humans, Factor Analysis, Statistical, Incubation, Mutagens
Abstract

Assessing urine mutagenicity with the Salmonella mutagenicity test is often limited by the volumes of the samples. Optimization of the assay was performed with factorial and Doehlert designs. Two fractional factorial designs 2(3-1) (3 factors, 4 experiments) were used to estimate the main effects of the percent S9 in the mix, the time of liquid incubation, the inoculum size and the growth conditions. A Doehlert design (3 factors, 13 experiments) was used to study the main effects and the interactions of the NADP, G6P and S9 in the mix. The positive markers were benzo[a]pyrene (BaP, 0.3 microgram/plate) and a pool of smokers' urine (SU, 1.25 ml equivalent/plate). The response was limited to the induction factor (IF, number of induced revertants/number of spontaneous revertants) with Salmonella typhimurium TA98. The optimal conditions for BaP were: a 60 min period of liquid incubation and a volume of 0.1 ml (approx. 10(8) cells/plate) of an overnight culture grown in 50 ml of Nutrient Broth No. 2 from a 250 ml flask. The S9 mix (0.1 ml, final volume) included 1.5% of S9, 1.0 mM NADP and 4.4 mM G6P. The maximal IF was 15.79. The optimal conditions for SU were: a 60 min period of liquid incubation and a volume of 0.1 ml (approx. 10(8) cells/plate) of an overnight culture grown in 7 ml of Nutrient Broth No. 2 from a 20 x 180 mm tube. The S9 mix (0.1 ml, final volume) included: 4% S9, 4.2 mM NADP and 5.2 mM G6P. The maximal IF was 10.95. These optimal conditions did not modify the spontaneous frequencies of the tester strains: TA97a, TA98, TA100 and TA102. The dose-response curves of mutagenic urine samples were found to be non-linear. This micromethod required 8-fold less urine sample and 12.5-fold less liver homogenate as compared to the standard plate incorporation assay and was from 6.2- to 11.8-fold more sensitive to evaluate urine mutagenicity. The sensitivity of this technique was found to be limited to individuals smoking more than approx. 5 cigarettes/day by the standard extraction-concentration procedure.

Published
1996
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9. The microstructure of dry concrete products

Author

Sidney Diamond, H. Guiraud, Michel Pigeon, H. Hornain, and J. Marchand

Subjects
Materials science, Silica fume, Optical microscope, Scanning electron microscope, law, Fly ash, General Materials Science, Building and Construction, Composite material, Mercury intrusion porosimetry, Microstructure, Cement paste, law.invention
Abstract

In North America, the use of dry concrete products has significantly expanded over the past decades. Despite the growing interest in these materials, little is known of their microstructure. In order to obtain more information on the subject, the microstructure of various dry concretes was investigated by means of optical microscopy, scanning electron microscopy, and mercury intrusion porosimetry, and compared to that of ordinary concretes. The results indicate that the cement paste fraction of most dry concretes is generally much more heterogeneous than that of ordinary concretes. High-energy mixing and the use of mineral additives, such as silica fume and fly ash, were found to significantly enhance the homogeneity of the cement paste. Considerable improvements of the engineering properties of dry concretes can be achieved by using these additives.

Published
1996
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10. Antimutagenic activities of 24 synthetic flavones with theSalmonella microsomal assay

Author

H. Guiraud, Gérard Duménil, J. C. Wallet, E. M. Gaydou, Michèle Laget, and M. De Méo

Subjects
chemistry.chemical_classification, Chromatography, Stereochemistry, Chlorophyllin, Organic Chemistry, Mutagen, Urine, medicine.disease_cause, Flavones, Ames test, chemistry.chemical_compound, chemistry, Drug Discovery, medicine, Microsome, Molecular Medicine, Pyrene, Incubation
Abstract

Twenty-four flavones were synthesized with various hydroxyl and/or methoxyl groups on A and B rings. Their antimutagenic properties were evaluated against benzo(a)pyrene (BaP) and a pool of mutagenic urine concentrate (U) using a modified liquid incubation method of Ames test. The tester strain wasSalmonella typhimurium TA98+S9 Mix. The antimutagenic activities were calculated by non linear regression analysis and the doses of flavones (in nmoles) required for a 50% reduction of induced revertants with BaP and U were defined as the inhibition doses (ID50B and ID50U respectively). Seventeen flavones possessed significant antimutagenic activity against BaP. ID50B ranged from 15.1 nmoles (F22) to 1000.6 nmoles (F13). Eighteen flavones showed significant antimutagenic activity against U. ID50U ranged from 23.5 nmoles (F22) to 354.6 nmoles (F3). The 2′, 3′, 4′-trihydroxyflavone (F22, ID50B=15.1 nmoles, ID50U=23.5 nmoles) and the 2′,3′,4′,7-tetrahydroxyflavone (F20, ID50B=37.8 nmoles; ID50U=62.3 nmoles) had antimutagenic activities similar to those of chlorophyllin (ID50B=19.6 nmoles and ID50U=44.2 nmoles) and were evaluated against B(a)P 7,8-dihydrodiol-9,10-epoxide. Against this last mutagen, the flavones which included three OH in B ring showed the highest activity and this property seemed independent of the substitutent groups on A ring.

Published
1995
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11. Monitoring exposure of hospital personnel handling cytostatic drugs and contaminated materials

Author

Michèle Laget, A. Botta, G. Duménil, M. P. DeMéo, H. Guiraud, A. D. DeBaille, and S. Mérono

Subjects
Adult, Male, endocrine system, medicine.medical_specialty, Antineoplastic Agents, Mutagen, Urine, medicine.disease_cause, Medical Waste, Ames test, Toxicology, Occupational medicine, Salmonella, Occupational Exposure, Humans, Medicine, Mutagenicity Tests, business.industry, Smoking, fungi, Public Health, Environmental and Occupational Health, food and beverages, Contamination, Personnel, Hospital, Cytostatic drugs, Female, Occupational exposure, business
Abstract

A study was undertaken to evaluate the urine mutagenicity of 63 individuals working in four hospital departments. The exposed group included 38 subjects who were exposed to various cytostatic drugs and/or contaminated material from treated patients. The control group included 25 individuals of the hospital personnel. Urine mutagenicity was monitored by the Ames test using tester strains TA 98 + S9 Mix and TA 102 — S9 Mix. Urine samples were collected before and after the working periods. A total of 29/116 (25%) urine samples were mutagenic for either strain. Among the mutagenic samples, 24/29 were mutagenic for tester strain TA 98 exclusively. No significant correlation could be found between occupational exposure to cytostatic drugs and urine mutagenicity evaluated by the strain TA 98 + S9 Mix. Smoking was the main environmental factor that modulated urine mutagenicity with TA 98. Three subjects in the exposed group had mutagenic urine samples at the end of the working period with strain TA 102 — S9 Mix. This mutagenicity was related to occupational exposure to cisplatin. In the control group, one individual had mutagenic samples before and after the working period. Assessing occupational exposure to cytostatic drugs with strain TA 102 requires additional studies to determine environmental mutagens which can be detected by this strain.

Published
1995
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12. [Difficulty in nursing patients with profound deficits]

Author

H, Guiraud

Subjects
Psychotic Disorders, Intellectual Disability, Nursing, Team, Humans, Nurse-Patient Relations, Nurse's Role, Self-Injurious Behavior, Patient Care Planning, Regression, Psychology
Published
2002

13. Toxicity and genotoxicity of antimalarial alkaloid rich extracts derived from Mitragyna inermis O. Kuntze and Nauclea latifolia

Author

F, Traore, M, Gasquet, M, Laget, H, Guiraud, C, Di Giorgio, N, Azas, O, Doumbo, and P, Timon-David

Subjects
Salmonella typhimurium, Plants, Medicinal, Mutagenicity Tests, Plant Extracts, Carbocyanines, Flow Cytometry, Kidney, Mali, Monocytes, Membrane Potentials, Antimalarials, Kinetics, Mice, Alkaloids, Liver, Microscopy, Fluorescence, Animals, Humans, Comet Assay, Lymphocytes, Medicine, African Traditional, DNA Damage
Abstract

The toxicity and the genotoxicity of antimalarial alkaloid rich extracts derived from two plants used in traditional medicine in Mali (Mitragyna inermis (Willd.) O. Kuntze Rubiaceae and Nauclea latifolia (Sm.) Rubiaceae) were evaluated on in vitro and in vivo systems. The results demonstrated that an alkaloid rich extract derived from M. inermis induced a strong inhibition of protein synthesis in mammalian cells but did not exhibit mutagenic or genotoxic activity. An alkaloid rich extract derived from N. latifolia could interact in vitro with DNA of bacteria and mammalian cells, leading to G2-M cell cycle arrest and heritable DNA-damage, as well as inducing in vivo single-strand breaks in liver, kidney and blood cells.

Published
2000

14. Formation of nitrogen-containing metabolites from the main iridoids of Harpagophytum procumbens and H. zeyheri by human intestinal bacteria

Author

Evelyne Ollivier, Guy Balansard, Béatrice Baghdikian, Annie N'Guyen, H. Guiraud-Dauriac, and Gérard Duménil

Subjects
Iridoid Glycosides, Magnetic Resonance Spectroscopy, Iridoid, Coumaric Acids, medicine.drug_class, Nitrogen, Pyridines, Monoterpene, Pharmaceutical Science, Pharmacognosy, Harpagophytum, Analytical Chemistry, Alkaloids, Drug Discovery, medicine, Humans, Glycosides, Pyrans, Pharmacology, chemistry.chemical_classification, biology, Bacteria, Alkaloid, Organic Chemistry, Glycoside, Plants, biology.organism_classification, Intestines, Complementary and alternative medicine, Biochemistry, chemistry, Molecular Medicine
Abstract

The study of the metabolism of iridoid glycosides from Harpagophytum procumbens and Harpagophytum zeyheri by human intestinal bacteria, was realized in order to elucidate compounds responsible for the pharmacological activities of Harpagophytum. Harpagide, harpagoside and 8-O-p-coumaroyl-harpagide were transformed into the pyridine monoterpene alkaloid aucubinine B by human fecal flora and by bacteria isolated from this flora. Aucubinine B was also prepared from harpagide, harpagoside and 8-O-p-coumaroylharpagide, by beta-glucosidase in the presence of NH4+.

Published
1999

15. Evaluation of the genotoxic activity of metronidazole and dimetridazole in human lymphocytes by the comet assay

Author

Patrice Vanelle, H. Guiraud, J.L. Re, Marcel Castegnaro, Michèle Laget, Gérard Duménil, and M.P. De Méo

Subjects
Male, DNA damage, Health, Toxicology and Mutagenesis, DNA Mutational Analysis, medicine.disease_cause, Superoxide dismutase, Rats, Sprague-Dawley, Metronidazole, Genetics, medicine, Animals, Humans, Lymphocytes, Molecular Biology, Electrophoresis, Agar Gel, biology, Vitamin C, Chemistry, Mutagenicity Tests, Superoxide Dismutase, Molecular biology, Dimetridazole, Rats, Comet assay, Biochemistry, Catalase, Toxicity, biology.protein, Microsomes, Liver, Genotoxicity, medicine.drug, DNA Damage, Mutagens
Abstract

The genotoxicity of metronidazole (MZ) and dimetridazole (DZ) has been evaluated in human lymphocytes using the comet assay. The test has been performed using 3 doses (58.4, 175.2 and 292.1 microM for MZ; and 70.9, 212.6 and 354.3 microM for DZ) under 3 experimental protocols: aerobiosis, anaerobiosis (90% N2, 10% CO2) and with the presence of the microsomal fraction S9 mix. The effects of 4 antioxidants (8-hydroxyquinoline (8HQ), vitamin C (VitC), catalase (CAT) and superoxide dismutase (SOD), have been investigated on DNA damage generated by fixed concentrations of MZ (292.1 microM) and DZ (354.4 microM). In aerobic conditions, MZ and DZ produced significant dose-response relationships. The dose-related effects of both drugs decreased or were abolished in anaerobic conditions or in presence of S9 mix. 8HQ, VitC, CAT and SOD induced dose-related protective responses against DNA damage due to MZ and DZ. These findings suggest that MZ and DZ induce DNA damage in human lymphocytes through the futile cycle. The one-electron reduction of the drugs leads to the production of nitro radical anions. In the presence of oxygen, these radicals are reoxidized and generate oxygen-activated species.

Published
1997

16. The Salmonella sulA-test: a new in vitro system to detect genotoxins

Author

Y. Barra, Eric Seree, Michèle Laget, Gérard Duménil, H. Guiraud, M. El Mzibri, and M. De Méo

Subjects
Salmonella typhimurium, Salmonella, Ethyl methanesulfonate, Molecular Sequence Data, Mutagen, Biology, Toxicology, medicine.disease_cause, Ames test, Microbiology, chemistry.chemical_compound, Bacterial Proteins, Genetics, medicine, SOS response, SOS Response, Genetics, Base Sequence, Mutagenicity Tests, Escherichia coli Proteins, Gene Expression Regulation, Bacterial, biology.organism_classification, Molecular biology, Enterobacteriaceae, SOS chromotest, chemistry, Evaluation Studies as Topic, Sodium azide, Mutagens
Abstract

The Salmonella sulA -test is a newly developed colorimetric assay to detect genotoxins. This technique is based on the ability of DNA-damaging agents to induce the sulA gene, one of the SOS response genes. A constructed plasmid, pEM1968, carrying a fused sulA′::′lacZ was introduced into Salmonella typhimurium TA1538. Monitoring sulA gene expression was performed by assaying the s-galactosidase activity in the transformed strain S. typhimurium TA1538/pEM1968. A simple, fast and sensitive liquid incubation procedure has been developed after optimization of the S9 mix composition and s-galactosidase assay. The SOS-inducing potency (SOSIP, μM −1 ) was defined as the slopes of the non-linear dose-response relationships. Twenty-one chemicals with different modes of action were examined for a preliminary evaluation of the test. Nineteen chemicals were genotoxic in the Salmonella sulA -test. The SOSIP ranged from 1.2 · 10 −4 μM −1 (ethyl methanesulfonate) to 419.9 μM −1 (bleomycin). Sodium azide and 5-fluoroucil were not genotoxic. Frameshift, base-pair and oxidative genotoxins were detected by the tester strain. The calculated SOSIP and the minimum concentrations detected (MCD) in the Salmonella sulA -test were compared to the reported values obtained with two similar assays: the SOS Chromotest and umu -test. The SOSIP values of 12 compounds were the highest in this new assay. Five chemicals tested in the Salmonella sulA -test gave similar SOSIP values with those of one of the two other tests. ICR-191 had the highest SOSIP with the SOS Chromotest and 3-methylchloranthrene showed the highest SOSIP with the umu -test. Similarly, the lowest MCD values were found for 12 compounds in the Salmonella sulA -test. Four compounds had close MCD values in this assay and one of the two other techniques. The SOS Chromotest remained the most sensitive assay for cisplatin and ICR 191. The umu -test was the technique of choice for 3-methylchloranthrene.

Published
1996

17. [A new mode of expression for the assessment of capacities of DNA repair by flow cytometry]

Author

M, Laget, H, Guiraud-Dauriac, M P, de Méo, C, di Giorgio, E, Roth, and G, Duménil

Subjects
Antibiotics, Antineoplastic, Carcinoma, Hepatocellular, DNA Repair, Doxorubicin, Depression, Chemical, Mitomycin, Liver Neoplasms, Tumor Cells, Cultured, Humans, DNA, Neoplasm, In Vitro Techniques, Flow Cytometry, Cell Division
Abstract

Flow cytometry technic was used to study DNA synthesis of Hep G2 cells following mitomycin C and adriblastine treatments during 24 hours. DNA synthesis was expressed by 2 methods: the new expression global DNA synthesis (S+G2)/G1 that considered the cells during scheduled and unscheduled DNA syntheses of S and G2 phases and the cell cycle (Fox program) that evaluated the cells during scheduled DNA synthesis by the terms G1 = 2n, S = 2n+x and G2 = 4n which excluded unscheduled DNA synthesis. The experimental data treated with this new expression led to the determination of threshold concentrations for the two tested compounds where the DNA repair mechanisms were overloaded, leading to cell death. This term was shown to be more accurate to describe the genotoxic action of compounds. Furthermore, these threshold concentrations of DNA damages was found to be linked with significant increase of micronuclei in the micronucleus test.

Published
1995

18. The micronucleus assay in human lymphocytes: screening for inter-individual variability and application to biomonitoring

Author

Gérard Duménil, Alain Botta, Michèle Laget, C. Di Giorgio, M. De Meo, and H. Guiraud

Subjects
Adult, Male, Cancer Research, Lymphocyte, Physiology, Biology, Age and sex, Toxicology, Reference Values, Occupational Exposure, Biomonitoring, medicine, Humans, Lymphocytes, Micronucleus Tests, General Medicine, Middle Aged, Investigation methods, medicine.anatomical_structure, Micronucleus test, Mann–Whitney U test, Female, Occupational exposure, Micronucleus, Environmental Monitoring, Mutagens
Abstract

Micronuclei levels were assessed in cytokinesis-blocked lymphocytes of 200 male and female healthy donors not occupationally exposed to genotoxic risks and of 33 male industrial painters handling genotoxic substances. Frequency of micronucleated cells was 9.87 +/- 3.1 per 1000 in the control population and was shown to have a large inter-individual variability. The study of factors contributing to this variability showed that only smoking could affect micronucleated cell rate, inducing an increase of 25%, whereas age and sex had no effect. Among the industrial painters, frequency of micronucleated cells averaged 18.30 +/- 7.39 per 1000: the difference between the two populations studied was shown to be statistically significant by the Mann-Whitney rank sum test (one-sided U test) and indicated that exposed painters need preventive measures.

Published
1994

19. Flow cytometry to evaluate the parasitemia of Plasmodium falciparum

Author

V, Kadjoian, M, Gasquet, F, Delmas, H, Guiraud, M, De Meo, M, Laget, and P, Timon-David

Subjects
Ethidium, Humans, Malaria, Falciparum, Flow Cytometry
Abstract

The resistance of plasmodiums to the current antimalarial agents has spurred the search for new active molecules of vegetal origin or chemical synthesis. The screening of antimalarial molecules "in vitro" was done by simple but tedious techniques such as quantification of parasitemia through optical microscopy or by using radioactive markers. We have developed a new method to evaluate parasitemia by using the ODAM ATC 3000 flow cytometer and biological cell sorter. We selected the ethidium bromide for labelling the nucleic acids of Plasmodium falciparum, and we optimised the method by using a mathematical model: the design of Hadamar. This simple technique presents the advantage of being an objective and rapid count of large number of red cells (10(6) x 10(7)). This method is rapid, reliable, reproducible, devoid of subjectivity and provides more precise results than those of optical microscopy. The good correlation between paraitemia measured by optical microscopy and fluorescence obtained by flow cytometry allows us to recommend this technic for the screening of new antimalarial molecules.

Published
1992

24. Activité d'une mousse antiseptique sur la flore normale des mains

Author

G. Dumenil, A. Cremieux, and H. Guiraud-Dauriac

Subjects
Infectious Diseases, media_common.quotation_subject, Art, Humanities, Hand disinfection, media_common
Abstract

Resume L'activite bactericide d'un nouvel antiseptique presente sous forme de mousse a ete determinee apres une seule application sur les mains. La reduction de la flore totale aerobie, exprimee en logarithme du nombre de bacteries par main, a pu etre appreciee quantitativement, apres 5 minutes, et apres 60 minutes avec port de gants : elle est de 1,39 et de 1,52 respectivement. Cette activite bactericide est obtenue avec une faible teneur en triclosan ; la formulation a base d'ethanol et donnant une mousse stable nous parait jouer un role important dans l'efficacite de cet antiseptique.

Published
1980
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26. [Multicenter study in actual situations of the activity of an antiseptic in the surgical washing of hands]

Author

A, Crémieux, H, Guiraud-Dauriac, J, Duval, G, Otterbein, J, Guilbaud, B, Epardeau, and A, Guillemart

Subjects
Anti-Infective Agents, Local, Humans, Hand, Surgery Department, Hospital, Hand Disinfection
Abstract

Results of a collaborative study carried out in three different hospitals by nine surgeons are reported. Activity of a new scrub applied according to a standardized protocol was compared with that of the different scrubs and/or antiseptics customarily used by participating surgeons with their habitual method. Activity of products was evaluated by bacterial counts in gloves. Statistical analysis of results demonstrates the value of this trial design which compares scrubs under real conditions of use.

Published
1984

28. [Inactivation of disinfectants by proteins and calcium ions as a function of their chemical constitution and bacterial species]

Author

H, Guiraud-Dauriac and A, Crémieux

Subjects
Chemistry, Bacteria, Chemical Phenomena, Species Specificity, Proteins, Water, Calcium, Microbial Sensitivity Tests, Disinfectants
Abstract

Activity of nine disinfectants was evaluated with interfering substances (albumin-yeast mixture and hard water), by two methods (NFT. 72 170, NFT. 72 171 and without interfering substance NFT. 72 150, NFT 72 151 respectively). Interference indexes were defined as the ratio of bactericidal concentration without interfering substances to bactericidal concentration with interfering substances. Five different ratings of interference effects were arbitrarily defined (no effect, moderate, average, strong, very strong). Proteins and hard water significantly inactivate aldehydes and quaternary ammonium salts : interference index is usually 25 but may reach 100-500. Inactivation of phenolic products by these two interfering substances is either lacking or inconsiderable. Conversely to Gram negative bacteria, activity of disinfectants on Gram positive bacteria is not significantly affected by proteins or hard water. P. aeruginosa can survive despite high concentrations of disinfectant in the presence of proteins and calcium ions. This finding may be a reason why this microorganism is difficult to eliminate from hospital wards.

Published
1984

30. [Multicenter study of the antimicrobial activity of antiseptics on the hands. Protocols and results]

Author

C, Savage, H, Leclerc, M E, Reverdy, J, Fleurette, H, Guiraud-Dauriac, A, Cremieux, B, Joly, R, Cluzel, and G, Garrigue

Subjects
Anti-Infective Agents, Local, Humans, Hand, Hand Disinfection
Abstract

Quantitative evaluation of in vivo activity of antiseptics in surgical-type handwashing is achieved by comparing bacterial counts on one hand after disinfection and on the other untreated hand. Handwashing, bacterial recovery and bacterial counts must be performed according to strictly standardized methods. A large number of participants is required.

Published
1984

34. [Homogeneous suspensions of mycobacteria: application to the evaluation of bactericidal activity (author's transl)]

Author

A, Crémieux, H, Guiraud, G, Duménil, and J, Chevalier

Subjects
Species Specificity, Suspensions, Virulence, Microbial Sensitivity Tests, Culture Media, Disinfectants, Mycobacterium
Abstract

This work describes a technique of emulsification of mycobacterial cells (including tubercle bacilli) in order to obtain homogeneous suspensions containing up to 10(8) cells/ml. The suspensions are used in a modified AFNOR method for the evaluation of bacterial activity: within five min virulent strains are more resistant than are avirulent ones but, within 30 min and in the presence of proteins, the behaviour of all strains is quite similar.

Published
1978

35. Links between organized visual search and reading ability in French primary school children.

Author

Guilbert A and Guiraud-Vinatea H

Subjects
Achievement, Child, Cognition, Humans, Schools, Dyslexia epidemiology, Reading
Abstract

Visual search skills develop substantially during the primary school years, and in parallel with children's reading achievement. Reading requires an efficient visual search and exposure to reading from the left to the right could also influence the way we explore space. No study, however, made links between visual search strategies and reading ability. In this study, 70 primary school children performed a cancellation task (Bells test) and reading tests. Our results showed that reading was closely linked to visual search accuracy but also to visual search organization, even after controlling for age for some measures. Along with the development of reading abilities, children made fewer revisitation, moved more to the nearest unmarked targets than to the farthest ones and explored more in lines. It appears, therefore, essential to take more into account the visual search organization of children with reading impairments such as dyslexia., (© 2021 John Wiley & Sons Ltd.)

Published
2022
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36. Neural oscillations track natural but not artificial fast speech: Novel insights from speech-brain coupling using MEG.

Author

Hincapié Casas AS, Lajnef T, Pascarella A, Guiraud-Vinatea H, Laaksonen H, Bayle D, Jerbi K, and Boulenger V

Subjects
Adolescent, Adult, Female, Humans, Language, Male, Middle Aged, Motor Cortex physiology, Young Adult, Auditory Perception physiology, Brain physiology, Magnetoencephalography methods, Speech physiology
Abstract

Neural oscillations contribute to speech parsing via cortical tracking of hierarchical linguistic structures, including syllable rate. While the properties of neural entrainment have been largely probed with speech stimuli at either normal or artificially accelerated rates, the important case of natural fast speech has been largely overlooked. Using magnetoencephalography, we found that listening to naturally-produced speech was associated with cortico-acoustic coupling, both at normal (∼6 syllables/s) and fast (∼9 syllables/s) rates, with a corresponding shift in peak entrainment frequency. Interestingly, time-compressed sentences did not yield such coupling, despite being generated at the same rate as the natural fast sentences. Additionally, neural activity in right motor cortex exhibited stronger tuning to natural fast rather than to artificially accelerated speech, and showed evidence for stronger phase-coupling with left temporo-parietal and motor areas. These findings are highly relevant for our understanding of the role played by auditory and motor cortex oscillations in the perception of naturally produced speech., (Copyright © 2021. Published by Elsevier Inc.)

Published
2021
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37. Visual search strategies in children: A reflection of working memory processes?

Author

Guilbert A, Perguilhem S, and Guiraud-Vinatea H

Subjects
Child, Female, Humans, Male, Attention physiology, Child Development physiology, Memory, Short-Term physiology, Space Perception physiology, Visual Perception physiology
Abstract

Visual search is not only less accurate but also less organized in children than in adults. However, visual search strategies in children have not been extensively studied and they are not evaluated in clinical practice. Working memory could play a critical role for the execution and the maintaining of a visual search strategy. Few studies if any have explored the links between visual search organization and working memory in children. In the present study, 54 primary school children performed a cancellation task (Bells test) and working memory tests (span tasks). Our results suggested that, contrary to visual search accuracy, visual search organization was significantly linked to working memory and, more specifically, to the efficiency of the central executive component. There is, thus, a real need to better understand the visual search process and to improve its assessment with cancellation tests in clinical practice.

Published
2020
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38. Don't speak too fast! Processing of fast rate speech in children with specific language impairment.

Author

Guiraud H, Bedoin N, Krifi-Papoz S, Herbillon V, Caillot-Bascoul A, Gonzalez-Monge S, and Boulenger V

Subjects
Adolescent, Case-Control Studies, Child, Comprehension physiology, Cues, Female, Humans, Language Tests, Male, Neuropsychological Tests, Reaction Time physiology, Speech Acoustics, Speech Intelligibility physiology, Language Development Disorders physiopathology, Language Development Disorders psychology, Speech Perception physiology
Abstract

Background: Perception of speech rhythm requires the auditory system to track temporal envelope fluctuations, which carry syllabic and stress information. Reduced sensitivity to rhythmic acoustic cues has been evidenced in children with Specific Language Impairment (SLI), impeding syllabic parsing and speech decoding. Our study investigated whether these children experience specific difficulties processing fast rate speech as compared with typically developing (TD) children., Method: Sixteen French children with SLI (8-13 years old) with mainly expressive phonological disorders and with preserved comprehension and 16 age-matched TD children performed a judgment task on sentences produced 1) at normal rate, 2) at fast rate or 3) time-compressed. Sensitivity index (d') to semantically incongruent sentence-final words was measured., Results: Overall children with SLI perform significantly worse than TD children. Importantly, as revealed by the significant Group × Speech Rate interaction, children with SLI find it more challenging than TD children to process both naturally or artificially accelerated speech. The two groups do not significantly differ in normal rate speech processing., Conclusion: In agreement with rhythm-processing deficits in atypical language development, our results suggest that children with SLI face difficulties adjusting to rapid speech rate. These findings are interpreted in light of temporal sampling and prosodic phrasing frameworks and of oscillatory mechanisms underlying speech perception.

Published
2018
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39. [Difficulty in nursing patients with profound deficits].

Author

Guiraud H

Subjects
Humans, Intellectual Disability psychology, Nurse's Role psychology, Patient Care Planning, Psychotic Disorders psychology, Self-Injurious Behavior psychology, Intellectual Disability nursing, Nurse-Patient Relations, Nursing, Team, Psychotic Disorders nursing, Regression, Psychology, Self-Injurious Behavior nursing
Published
2001

40. Toxicity and genotoxicity of antimalarial alkaloid rich extracts derived from Mitragyna inermis O. Kuntze and Nauclea latifolia.

Author

Traore F, Gasquet M, Laget M, Guiraud H, Di Giorgio C, Azas N, Doumbo O, and Timon-David P

Subjects
Animals, Carbocyanines chemistry, Comet Assay, Flow Cytometry, Humans, Kidney chemistry, Kinetics, Liver chemistry, Lymphocytes chemistry, Mali, Medicine, African Traditional, Membrane Potentials, Mice, Microscopy, Fluorescence, Monocytes cytology, Mutagenicity Tests, Salmonella typhimurium drug effects, Salmonella typhimurium genetics, Alkaloids toxicity, Antimalarials toxicity, DNA Damage, Monocytes drug effects, Plant Extracts toxicity, Plants, Medicinal toxicity
Abstract

The toxicity and the genotoxicity of antimalarial alkaloid rich extracts derived from two plants used in traditional medicine in Mali (Mitragyna inermis (Willd.) O. Kuntze Rubiaceae and Nauclea latifolia (Sm.) Rubiaceae) were evaluated on in vitro and in vivo systems. The results demonstrated that an alkaloid rich extract derived from M. inermis induced a strong inhibition of protein synthesis in mammalian cells but did not exhibit mutagenic or genotoxic activity. An alkaloid rich extract derived from N. latifolia could interact in vitro with DNA of bacteria and mammalian cells, leading to G2-M cell cycle arrest and heritable DNA-damage, as well as inducing in vivo single-strand breaks in liver, kidney and blood cells.

Published
2000
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41. The protective activity of alpha-hederine against H2O2 genotoxicity in HepG2 cells by alkaline comet assay.

Author

Mba Gachou C, Laget M, Guiraud-Dauriac H, De Méo M, Elias R, and Duménil G

Subjects
Catalase drug effects, Catalase metabolism, Cell Membrane drug effects, Cell Membrane metabolism, DNA, Neoplasm drug effects, Dose-Response Relationship, Drug, Electrophoresis, Agar Gel methods, Glutathione drug effects, Glutathione metabolism, Humans, Mutagenicity Tests, Oxidation-Reduction drug effects, Proteins drug effects, Proteins metabolism, Tumor Cells, Cultured, DNA Damage drug effects, Hydrogen Peroxide toxicity, Oleanolic Acid analogs & derivatives, Protective Agents pharmacology, Saponins pharmacology
Abstract

This study was designed to evaluate the protective effect of alpha-hederine (alpha-hed) against H2O2-mediated DNA damage on HepG2 cell line by the alkaline comet assay. For the protective effect of alpha-hed study, cells were treated according to three protocols: pre-treatment, simultaneous treatment and post-treatment. The effect of alpha-hed on catalase activity was evaluated after treating the cells with 3.36 mg/ml of 3-amino-1,2,4-triazole (AMT) singly or in combination with alpha-hed (1.5 or 3 microg/ml) and H2O2 (8.8 microM) during 1 h. The catalase activity was also biochemically measured after treating cells with alpha-hed at 1.5, 3, or 15 microg/ml during 1 h. Additionally, the influence of alpha-hed on membrane RedOx potential, pool of reduced glutathione and total protein content was evaluated by flow cytometry. In the pre-treatment, the two concentrations of alpha-hed (1.5 and 3 microg/ml) decreased the lesions induced by H2O2 (8.8 microM) significantly. This decrease was about 57.2% and 66.1%, respectively. Similar results were observed when cells were treated with alpha-hed and H2O2 simultaneously. The decrease of H2O2-induced lesions was about 78.2% and 83.2% (alpha-hed 1.5 and 3 microg/ml, respectively). In the post-treatment protocol, this decrease was not significant. The combination of AMT and H2O2 induced more DNA damage than H2O2 alone (tail moment (TM) means was 31.4% and 21.8%, respectively). When alpha-hed was added to this mixture, TM means were reduced significantly (17.4% for alpha-hed 1. 5 microg/ml and 15.5% for alpha-hed 3 microg/ml). Up to 6.9 microg/ml, alpha-hed enhanced catalase activity (60.5%), followed by a decrease of the activity. Total protein content and membrane RedOx potential were slightly increased up to 11 microg/ml (14% and 3.6%, respectively) followed by a drop and a plateau. Pool of reduced glutathione remained unchanged up to 10 microg/ml then dropped and reached a plateau. In conclusion, alpha-hed could exert its protective effect against H2O2-mediated DNA damage by scavenging free radicals or by enhancing the catalase activity.

Published
1999
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42. Formation of nitrogen-containing metabolites from the main iridoids of Harpagophytum procumbens and H. zeyheri by human intestinal bacteria.

Author

Baghdikian B, Guiraud-Dauriac H, Ollivier E, N'Guyen A, Dumenil G, and Balansard G

Subjects
Coumaric Acids chemistry, Humans, Iridoid Glycosides, Magnetic Resonance Spectroscopy, Nitrogen chemistry, Pyrans chemistry, Alkaloids chemical synthesis, Bacteria metabolism, Coumaric Acids metabolism, Glycosides, Intestines microbiology, Plants metabolism, Pyrans metabolism, Pyridines chemical synthesis
Abstract

The study of the metabolism of iridoid glycosides from Harpagophytum procumbens and Harpagophytum zeyheri by human intestinal bacteria, was realized in order to elucidate compounds responsible for the pharmacological activities of Harpagophytum. Harpagide, harpagoside and 8-O-p-coumaroyl-harpagide were transformed into the pyridine monoterpene alkaloid aucubinine B by human fecal flora and by bacteria isolated from this flora. Aucubinine B was also prepared from harpagide, harpagoside and 8-O-p-coumaroylharpagide, by beta-glucosidase in the presence of NH4+.

Published
1999
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43. Evaluation of the mutagenicity and antimutagenicity of forty-two 3-substituted flavones in the Ames test.

Author

Beudot C, De Méo MP, Dauzonne D, Elias R, Laget M, Guiraud H, Balansard G, and Duménil G

Subjects
Mutagenicity Tests, Salmonella typhimurium drug effects, Salmonella typhimurium genetics, Antimutagenic Agents pharmacology, Flavonoids pharmacology, Flavonoids toxicity, Mutagens toxicity
Abstract

The mutagenic and antimutagenic activities of forty-two synthetic flavones were assessed by the Ames test. The tested flavones included twenty-three 3-nitroflavones, eighteen 3-aminoflavones and the 3-chloroflavone. The mutagenicity was evaluated with Salmonella typhimurium TA100 and YG1042 (an overproducing nitroreductase and O-acetyltransferase TA100 strain) with and without metabolic activation (S9 mix). The antimutagenicity of the non mutagenic derivatives was evaluated against 11 known reference mutagens. A total of 39 synthetic flavones were mutagenic. The mutagenic activities ranged from 0.1 rev/nmole (4'-chloro-6-methoxy-3-nitroflavone) to 6240 rev/nmole (4'-methoxy-3, 3'-diaminoflavone). Two differences were found between the 3-amino and the 3-nitroflavones: (i) the mutagenicity of the 3-aminoflavones required the presence of the metabolic activation; (ii) the 3-amino derivatives were more mutagenic than their 3-nitro counterparts. Increased mutagenicity, as assessed with strain YG1042, was limited to 17/39 derivatives. The mutagenic activity was induced by the presence of the double bond at the 2,3-position for conjugation of the lone-pair electron with the carbonyl group on the 'C' ring. This mutagenicity was modulated by substituents at the 2'-position. Additional mutagenicity was brought by the aminoaromatic and nitroaromatic group reduction by bacterial nitroreductases and by the S9 mix; it was modulated by different substituents on the aromatic rings of the flavones. Three flavones: 3-chloroflavone (1C), 4'-hydroxy-3-nitroflavone (23N) and 2',3-diaminoflavone (2A) showed antimutagenic properties. Compound 1C was efficient against benzo(a)pyrene (BaP), 2-aminofluorene (2AF), 2-aminoanthracene (2AA), 4-nitroquinoline-1-oxide (4NQO) and 1-methyl-3'-nitro-1-nitrosoguanidine (MNNG). Compound 23N inhibited the mutagenicity of BaP and MNNG. The antimutagenic activity of 2A was limited to MNNG., (Copyright 1998 Elsevier Science B.V.)

Published
1998
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44. Evaluation of a flow cytofluorometric method for rapid determination of amphotericin B susceptibility of yeast isolates.

Author

Peyron F, Favel A, Guiraud-Dauriac H, El Mzibri M, Chastin C, Dumenil G, and Regli P

Subjects
Computers, Evaluation Studies as Topic, Flow Cytometry, Microbial Sensitivity Tests, Regression Analysis, Time Factors, Amphotericin B pharmacology, Antifungal Agents pharmacology, Candida drug effects
Abstract

A rapid-flow cytofluorometric susceptibility test for in vitro amphotericin B testing of yeasts was evaluated and compared to the National Committee for Clinical Laboratory Standards (NCCLS) M27-T reference broth macrodilution method. The flow cytofluorometric method is based on the detection of decreased green fluorescence intensity of cells stained with DiOC5(3), a membrane potential-sensitive cationic dye, after drug treatment. Testing was performed on 134 clinical isolates (Candida spp. and Torulopsis glabrata). From the dose-response curve obtained for each isolate, three endpoints were calculated by computer analysis (the concentrations at which the fluorescence intensity was reduced by 50, 80, and 90%, i.e., 50% inhibitory concentration [IC50], IC80, and IC90, respectively). A regression analysis correlating these endpoints with the M27-T MICs showed that the best agreement was obtained with IC80. The flow cytofluorometric method showed good reproducibility with control strains. These initial results suggest that the flow cytofluorometric method is a valid alternative to the NCCLS reference method.

Published
1997
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45. Evaluation of the genotoxic activity of metronidazole and dimetridazole in human lymphocytes by the comet assay.

Author

Ré JL, De Méo MP, Laget M, Guiraud H, Castegnaro M, Vanelle P, and Duménil G

Subjects
Animals, Electrophoresis, Agar Gel methods, Humans, Male, Microsomes, Liver metabolism, Rats, Rats, Sprague-Dawley, Superoxide Dismutase metabolism, DNA Damage, DNA Mutational Analysis, Dimetridazole pharmacology, Lymphocytes drug effects, Metronidazole pharmacology, Mutagenicity Tests methods, Mutagens pharmacology
Abstract

The genotoxicity of metronidazole (MZ) and dimetridazole (DZ) has been evaluated in human lymphocytes using the comet assay. The test has been performed using 3 doses (58.4, 175.2 and 292.1 microM for MZ; and 70.9, 212.6 and 354.3 microM for DZ) under 3 experimental protocols: aerobiosis, anaerobiosis (90% N2, 10% CO2) and with the presence of the microsomal fraction S9 mix. The effects of 4 antioxidants (8-hydroxyquinoline (8HQ), vitamin C (VitC), catalase (CAT) and superoxide dismutase (SOD), have been investigated on DNA damage generated by fixed concentrations of MZ (292.1 microM) and DZ (354.4 microM). In aerobic conditions, MZ and DZ produced significant dose-response relationships. The dose-related effects of both drugs decreased or were abolished in anaerobic conditions or in presence of S9 mix. 8HQ, VitC, CAT and SOD induced dose-related protective responses against DNA damage due to MZ and DZ. These findings suggest that MZ and DZ induce DNA damage in human lymphocytes through the futile cycle. The one-electron reduction of the drugs leads to the production of nitro radical anions. In the presence of oxygen, these radicals are reoxidized and generate oxygen-activated species.

Published
1997
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46. The Salmonella sulA-test: a new in vitro system to detect genotoxins.

Author

el Mzibri M, De Méo MP, Laget M, Guiraud H, Séree E, Barra Y, and Duménil G

Subjects
Base Sequence, Evaluation Studies as Topic, Gene Expression Regulation, Bacterial, Molecular Sequence Data, SOS Response, Genetics, Bacterial Proteins, Escherichia coli Proteins, Mutagenicity Tests, Mutagens toxicity, Salmonella typhimurium drug effects
Abstract

The Salmonella sulA-test is a newly developed colorimetric assay to detect genotoxins. This technique is based on the ability of DNA-damaging agents to induce the sulA gene, one of the SOS response genes. A constructed plasmid, pEM1968, carrying a fused sulA'::'lacZ was introduced into Salmonella typhimurium TA1538. Monitoring sulA gene expression was performed by assaying the beta-galactosidase activity in the transformed strain S. typhimurium TA1538/pEM1968. A simple, fast and sensitive liquid incubation procedure has been developed after optimization of the S9 mix composition and beta-galactosidase assay. The SOS-inducing potency (SOSIP, microM-1) was defined as the slopes of the non-linear dose-response relationships. Twenty-one chemicals with different modes of action were examined for a preliminary evaluation of the test. Nineteen chemicals were genotoxic in the Salmonella sulA-test. The SOSIP ranged from 1.2 x 10(-4) microM-1 (ethyl methanesulfonate) to 419.9 microM-1 (bleomycin). Sodium azide and 5-fluorouracil were not genotoxic. Frameshift, base-pair and oxidative genotoxins were detected by the tester strain. The calculated SOSIP and the minimum concentrations detected (MCD) in the Salmonella sulA-test were compared to the reported values obtained with two similar assays: the SOS Chromotest and umu-test. The SOSIP values of 12 compounds were the highest in this new assay. Five chemicals tested in the Salmonella sulA-test gave similar SOSIP values with those of one of the two other tests. ICR-191 had the highest SOSIP with the SOS Chromotest and 3-methylchloranthrene showed the highest SOSIP with the umu-test. Similarly, the lowest MCD values were found for 12 compounds in the Salmonella sulA-test. Four compounds had close MCD values in this assay and one of the two other techniques. The SOS Chromotest remained the most sensitive assay for cisplatin and ICR 191. The umu-test was the technique of choice for 3-methylchloranthrene.

Published
1996
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47. Optimization of the Salmonella/mammalian microsome assay for urine mutagenesis by experimental designs.

Author

De Méo M, Laget M, Di Giorgio C, Guiraud H, Botta A, Castegnaro M, and Duménil G

Subjects
Dose-Response Relationship, Drug, Factor Analysis, Statistical, Humans, Mutagenicity Tests statistics & numerical data, Mutagens pharmacology, Predictive Value of Tests, Smoking adverse effects, Microsomes, Liver metabolism, Mutagenicity Tests methods, Research Design statistics & numerical data, Salmonella typhimurium genetics, Smoking urine
Abstract

Assessing urine mutagenicity with the Salmonella mutagenicity test is often limited by the volumes of the samples. Optimization of the assay was performed with factorial and Doehlert designs. Two fractional factorial designs 2(3-1) (3 factors, 4 experiments) were used to estimate the main effects of the percent S9 in the mix, the time of liquid incubation, the inoculum size and the growth conditions. A Doehlert design (3 factors, 13 experiments) was used to study the main effects and the interactions of the NADP, G6P and S9 in the mix. The positive markers were benzo[a]pyrene (BaP, 0.3 microgram/plate) and a pool of smokers' urine (SU, 1.25 ml equivalent/plate). The response was limited to the induction factor (IF, number of induced revertants/number of spontaneous revertants) with Salmonella typhimurium TA98. The optimal conditions for BaP were: a 60 min period of liquid incubation and a volume of 0.1 ml (approx. 10(8) cells/plate) of an overnight culture grown in 50 ml of Nutrient Broth No. 2 from a 250 ml flask. The S9 mix (0.1 ml, final volume) included 1.5% of S9, 1.0 mM NADP and 4.4 mM G6P. The maximal IF was 15.79. The optimal conditions for SU were: a 60 min period of liquid incubation and a volume of 0.1 ml (approx. 10(8) cells/plate) of an overnight culture grown in 7 ml of Nutrient Broth No. 2 from a 20 x 180 mm tube. The S9 mix (0.1 ml, final volume) included: 4% S9, 4.2 mM NADP and 5.2 mM G6P. The maximal IF was 10.95. These optimal conditions did not modify the spontaneous frequencies of the tester strains: TA97a, TA98, TA100 and TA102. The dose-response curves of mutagenic urine samples were found to be non-linear. This micromethod required 8-fold less urine sample and 12.5-fold less liver homogenate as compared to the standard plate incorporation assay and was from 6.2- to 11.8-fold more sensitive to evaluate urine mutagenicity. The sensitivity of this technique was found to be limited to individuals smoking more than approx. 5 cigarettes/day by the standard extraction-concentration procedure.

Published
1996
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48. [A new mode of expression for the assessment of capacities of DNA repair by flow cytometry].

Author

Laget M, Guiraud-Dauriac H, de Méo MP, di Giorgio C, Roth E, and Duménil G

Subjects
Antibiotics, Antineoplastic pharmacology, Carcinoma, Hepatocellular genetics, Cell Division drug effects, Depression, Chemical, Humans, In Vitro Techniques, Liver Neoplasms genetics, Tumor Cells, Cultured cytology, Tumor Cells, Cultured drug effects, DNA Repair drug effects, DNA, Neoplasm drug effects, Doxorubicin pharmacology, Flow Cytometry methods, Mitomycin pharmacology
Abstract

Flow cytometry technic was used to study DNA synthesis of Hep G2 cells following mitomycin C and adriblastine treatments during 24 hours. DNA synthesis was expressed by 2 methods: the new expression global DNA synthesis (S+G2)/G1 that considered the cells during scheduled and unscheduled DNA syntheses of S and G2 phases and the cell cycle (Fox program) that evaluated the cells during scheduled DNA synthesis by the terms G1 = 2n, S = 2n+x and G2 = 4n which excluded unscheduled DNA synthesis. The experimental data treated with this new expression led to the determination of threshold concentrations for the two tested compounds where the DNA repair mechanisms were overloaded, leading to cell death. This term was shown to be more accurate to describe the genotoxic action of compounds. Furthermore, these threshold concentrations of DNA damages was found to be linked with significant increase of micronuclei in the micronucleus test.

Published
1995

49. Monitoring exposure of hospital personnel handling cytostatic drugs and contaminated materials.

Author

DeMéo MP, Mérono S, DeBaille AD, Botta A, Laget M, Guiraud H, and Duménil G

Subjects
Adult, Antineoplastic Agents pharmacokinetics, Antineoplastic Agents pharmacology, Female, Humans, Male, Medical Waste, Mutagenicity Tests, Salmonella drug effects, Salmonella genetics, Smoking, Antineoplastic Agents urine, Occupational Exposure analysis, Personnel, Hospital
Abstract

A study was undertaken to evaluate the urine mutagenicity of 63 individuals working in four hospital departments. The exposed group included 38 subjects who were exposed to various cytostatic drugs and/or contaminated material from treated patients. The control group included 25 individuals of the hospital personnel. Urine mutagenicity was monitored by the Ames test using tester strains TA 98 + S9 Mix and TA 102-S9 Mix. Urine samples were collected before and after the working periods. A total of 29/116 (25%) urine samples were mutagenic for either strain. Among the mutagenic samples, 24/29 were mutagenic for tester strain TA 98 exclusively. No significant correlation could be found between occupational exposure to cytostatic drugs and urine mutagenicity evaluated by the strain TA 98 + S9 Mix. Smoking was the main environmental factor that modulated urine mutagenicity with TA 98. Three subjects in the exposed group had mutagenic urine samples at the end of the working period with strain TA 102-S9 Mix. This mutagenicity was related to occupational exposure to cisplatin. In the control group, one individual had mutagenic samples before and after the working period. Assessing occupational exposure to cytostatic drugs with strain TA 102 requires additional studies to determine environmental mutagens which can be detected by this strain.

Published
1995
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50. The micronucleus assay in human lymphocytes: screening for inter-individual variability and application to biomonitoring.

Author

Di Giorgio C, De Méo MP, Laget M, Guiraud H, Botta A, and Duménil G

Subjects
Adult, Female, Humans, Lymphocytes ultrastructure, Male, Micronucleus Tests, Middle Aged, Reference Values, Environmental Monitoring, Lymphocytes drug effects, Mutagens toxicity, Occupational Exposure
Abstract

Micronuclei levels were assessed in cytokinesis-blocked lymphocytes of 200 male and female healthy donors not occupationally exposed to genotoxic risks and of 33 male industrial painters handling genotoxic substances. Frequency of micronucleated cells was 9.87 +/- 3.1 per 1000 in the control population and was shown to have a large inter-individual variability. The study of factors contributing to this variability showed that only smoking could affect micronucleated cell rate, inducing an increase of 25%, whereas age and sex had no effect. Among the industrial painters, frequency of micronucleated cells averaged 18.30 +/- 7.39 per 1000: the difference between the two populations studied was shown to be statistically significant by the Mann-Whitney rank sum test (one-sided U test) and indicated that exposed painters need preventive measures.

Published
1994
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