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5. Simulation of Lidar signal with DART for the development of LEAF, a spaceborne Lidar mission for forest ecosystem monitoring

Author

Durrieu, S., de Boissieu, F., Gastellu-Etchegorry, Jean-Philippe, Vincent, G., Lavalley, C., Couderc, G., Mpili, S., Heuschmidt, F., Costeraste, J., Feret, J.B., Ebengo, D., Lauret, Nicolas, Lefèvre Fonollosa, M.J., Yin, T., Territoires, Environnement, Télédétection et Information Spatiale (UMR TETIS), Centre de Coopération Internationale en Recherche Agronomique pour le Développement (Cirad)-AgroParisTech-Institut national de recherche en sciences et technologies pour l'environnement et l'agriculture (IRSTEA)-Centre National de la Recherche Scientifique (CNRS), Centre d'études spatiales de la biosphère (CESBIO), Centre National de la Recherche Scientifique (CNRS)-Institut de Recherche pour le Développement (IRD)-Institut National de Recherche pour l’Agriculture, l’Alimentation et l’Environnement (INRAE)-Université Toulouse III - Paul Sabatier (UT3), Université Fédérale Toulouse Midi-Pyrénées-Université Fédérale Toulouse Midi-Pyrénées-Institut national des sciences de l'Univers (INSU - CNRS)-Observatoire Midi-Pyrénées (OMP), Météo France-Centre National d'Études Spatiales [Toulouse] (CNES)-Université Fédérale Toulouse Midi-Pyrénées-Centre National de la Recherche Scientifique (CNRS)-Institut de Recherche pour le Développement (IRD)-Météo France-Centre National d'Études Spatiales [Toulouse] (CNES)-Centre National de la Recherche Scientifique (CNRS), Institut National de la Recherche Agronomique (INRA), Centre National d'Études Spatiales [Toulouse] (CNES), NASA GSFC GREENBELT USA, Partenaires IRSTEA, and Institut national de recherche en sciences et technologies pour l'environnement et l'agriculture (IRSTEA)-Institut national de recherche en sciences et technologies pour l'environnement et l'agriculture (IRSTEA)

Subjects
STRUCTURE FORESTIERE, LIDAR SPATIAL, [SDE]Environmental Sciences, DART, TRANSFERT RADIATIF, SIMULATION SIGNAL
Abstract

Understanding the Global Climate Change and the way it will affect the Earth and preserving biodiversity are two major challenges of the 21st century. Forests cover 30% of continental surfaces and are a major contributor to the carbon cycle. Sequestration of carbon in forest biomass appears as an important mechanism - in conjunction with reduced emissions - for mitigating climate change. Adequate management of forest resources could strengthen the action of forests as a carbon sink. Forests also play a key role for biodiversity conservation and energy supply. Sustainable management of forest ecosystems is thus critical for the future of mankind. However, the lack of consistent information on forest structure and biomass and on their dynamics at global scale hampers the development of ecological models and of earth-vegetation-atmosphere interaction global models that are essential to improve knowledge on forest ecosystem functioning and to address the challenge of forest sustainable management. By its ability to measure the vertical structure of land cover, airborne Lidar technology is highly qualified for forest applications. NASA's ICESat1 mission (2003-2009) paved the way for Earth observation from space with Lidar systems. ICESat2, launched in September 2018, although primarily designed for ice monitoring will also provide vegetation height measurements worldwide. Vegetation profiles with high vertical resolution should also become soon available with GEDI (NASA) and MOLI (JAXA) missions that will be installed on the ISS at the end of 2018 and in 2019 or 2020, respectively. Although data coverage will be limited from 52°S to 52°N, both these missions will contribute to ecosystem structure observation from space in conjunction with radar missions, especially the BIOMASS ESA's mission. Combined with Sentinel 2 imagery, which provides spectral information with high spatial and temporal resolutions, they will also enable to evaluate the complementarity between information on 3D structure, composition and phenology for a comprehensive monitoring of forest ecosystem conditions. LEAF (Lidar For Earth and Forests) mission has been under study at CNES since 2008 and could contribute in the future to the international effort to sustain global carbon and biodiversity monitoring systems. The system under study combines a NIR full-waveform Lidar profiler and a very high resolution multispectral imager. CNES has supported scientific projects in order to refine instrument specifications and design a system that will meet user requirements. Due to the high cost associated with the development of an airborne prototype, priority has been given to simulation approaches. The aim of this contribution is to present LEAF mission concept and to focus on the recent "LEAF ExpeVal" experiment, designed to consolidate and validate the simulation approaches developed to model a realistic Lidar signal on various forest types, including complex tropical forests. These approaches rely on DART, a radiative transfer model developed at CESBIO. A Lidar module was introduced into DART in the early 2010s and has undergone constant improvement since then. However, simulating a realistic signal also requires to work on model inputs and to develop methods to build detailed forest scenes. The objective of the LEAF-Expeval experiment was twofold: first, to validate the simulations by comparing simulated and experimental Lidar waveforms on a tropical forest; second, to develop a new approach to simulate spaceborne Lidar data from small footprint airborne Lidar data (ALS data). Achieving the first objective is a key step to refine LEAF system specifications in order to ensure that the system will provide accurate height measurements and vegetation profiles on tropical forests, which are the most constraining environment for a space Lidar. Field and airborne data were collected in Paracou experimental forest in French Guiana. The processing and analysis steps include (1) the construction of forest scenes from TLS (Terrestrial Lidar Scanner) and reflectance measurements on a dense forest plot, (2) the estimation of the calibration coefficient of the airborne system, coefficient that is used to convert digital count into physical units, (3) the simulation of airborne Lidar data on the forest scene using DART and (4) the comparison of simulated and real waveforms. As ALS data are now widely available, achieving the second objective would enable the simulation and evaluation of LEAF data on a variety of forest ecosystems. This part of the study relies on Lidar simulations realized on temperate broadleaved forest scenes created using Allostand (Amap) and Genesis software. Small footprint lidar point clouds were simulated using DART and were in turn used to simulate large footprint lidar waveforms. The resulting waveforms were compared to reference data, i.e. large footprint waveforms obtained directly with DART on the same forest scenes. First results are encouraging and showed that large footprint waveforms obtained from the processing of small footprint data were very similar to reference waveforms, even with a change of waveband between lidar point clouds and large footprint waveform.

Published
2019

10. Structural Relaxation in Nanometer Thin Layers of Glycerol

Author

Capponi, Simona, Napolitano, Simone, Behrnd, N., Couderc, G., Hulliger, J., Wübbenhorst, Michael, Capponi, Simona, Napolitano, Simone, Behrnd, N., Couderc, G., Hulliger, J., and Wübbenhorst, Michael

Abstract

info:eu-repo/semantics/published

Published
2010

11. Alignment and relaxation dynamics of dye molecules in host-guest inclusion compounds as probed by dielectric spectroscopy

Author

Tsuwi J., Berger R., Labat G., Couderc G., Behrnd N.-R., Ottiger P., Cucinotta F., Schürmann K., Bertoni M., Viani L., Gierschner, Johannes, Cornil J., Prodi-Schwab A., De Cola L., Wübbenhorst M., Hulliger J., Tsuwi J., Berger R., Labat G., Couderc G., Behrnd N.-R., Ottiger P., Cucinotta F., Schürmann K., Bertoni M., Viani L., Gierschner, Johannes, Cornil J., Prodi-Schwab A., De Cola L., Wübbenhorst M., and Hulliger J.

Published
2010

23. Delineation of the roles of paracrine and autocrine interleukin-6 (IL-6) in myeloma cell lines in survival versus cell cycle. A possible model for the cooperation of myeloma cell growth factors

Author

Jourdan M, Mahtouk K, Jl, Veyrune, Couderc G, Fiol G, Redal N, Christophe Duperray, De Vos J, Klein B, Immunopathologie des maladies tumorales et autoimmunes, Université Montpellier 1 (UM1)-IFR76-Institut National de la Santé et de la Recherche Médicale (INSERM), Unité de thérapie cellulaire, Centre Hospitalier Régional Universitaire [Montpellier] (CHRU Montpellier)-Hôpital Saint Eloi (CHRU Montpellier), Centre Hospitalier Régional Universitaire [Montpellier] (CHRU Montpellier), and Frei, Monique

Subjects
MESH: Neoplasm Proteins, MESH: Cell Line, Tumor, Cell Survival, MESH: Cell Cycle, MESH: Multiple Myeloma, MESH: Antibodies, Monoclonal, Cell Line, Tumor, Paracrine Communication, [SDV.BBM] Life Sciences [q-bio]/Biochemistry, Molecular Biology, Humans, [SDV.BBM]Life Sciences [q-bio]/Biochemistry, Molecular Biology, MESH: Paracrine Communication, IL-6, MESH: Humans, Interleukin-6, MESH: Apoptosis, apoptosis, Antibodies, Monoclonal, MESH: Interleukin-6, Neoplasm Proteins, Autocrine Communication, myeloma, Proto-Oncogene Proteins c-bcl-2, MESH: Proto-Oncogene Proteins c-bcl-2, MESH: Cell Survival, Myeloid Cell Leukemia Sequence 1 Protein, cell cycle, MESH: Autocrine Communication, Multiple Myeloma
Abstract

Primary myeloma cells rapidly apoptose as soon as they are removed from their bone-marrow environment. A likely explanation is that the tumor environment produces survival factors that may counteract a spontaneous activation of pro-apoptotic program. Additional factors may trigger cell cycling in surviving myeloma cells. Interleukin-6 (IL-6) is a well recognized myeloma cell growth factor produced mainly by the tumor environment. However, myeloma cells themselves may produce low levels of autocrine IL-6. The respective roles of paracrine versus autocrine IL-6 are a matter of debate. We investigated these roles using the XG-6 myeloma cell line whose growth is dependent on addition of exogenous IL-6, despite its weak IL-6 mRNA and protein expression. The apoptosis induced by exogenous IL-6 deprivation was blocked by transferring the Mcl-1 gene coding for an anti-apoptotic protein in XG-6 cells. An XG-6Mcl-1 cell line which can survive and grow without adding IL-6 was obtained. We show that anti-IL-6 or anti-gp130 antibodies abrogated cell cycling whereas they did not affect cell survival. These data indicate that the weak autocrine IL-6 produced by myeloma cells is sufficient to trigger cell cycling whereas their survival requires large exogenous IL-6 concentrations. This important role of autocrine IL-6 has to be considered when evaluating the mechanism of action of myeloma cell growth factors. These factors may actually block an activated pro-apoptotic program, making possible a weak production of autocrine IL-6 to promote cell cycling.

25. Addressing the quality challenge of a human biospecimen biobank through the creation of a quality management system.

Author

Servais MD, Galtier F, Nouvel A, Rebuffat S, Laget J, Géan A, Provost N, Lorcy F, Rigau V, Couderc G, Géraud P, Nocca D, Builles N, De Préville N, and Lajoix AD

Subjects
Humans, Reproducibility of Results, Preservation, Biological, Specimen Handling methods, DNA, Biological Specimen Banks, RNA
Abstract

Background: The objective of the COMET (COllection of MEtabolic Tissues) biobank project is to create a high-quality collection of insulin-sensitive tissues (liver, muscle, adipose tissues, and epiploic artery) and blood sample derivatives (plasma, serum, DNA and RNA), collected from 270 grade 2-3 obese patients undergoing bariatric surgery. Relevant data on patient such as clinical/biological characteristics and sample handling are also collected. For this, our aim was to establish a Quality Management System (QMS) to meet the reliability and quality requirements necessary for its scientific exploitation., Materials and Methods: The COMET QMS includes: (1) Quality Assurance to standardize all stages of the biobanking process, (2) Quality Controls on samples from the first patients included in order to validate the sample management process and ensure reproducible quality; and 3) "in process" Quality Controls to ensure the reliability of the storage procedures and the stability of the samples over time., Results: For serum and plasma, several corrective actions, such as temperature handling and centrifugation conditions, were made to the protocol and led to improvement of the volume and quality of samples. Regarding DNA, all samples evaluated achieved a satisfactory level of purity and integrity and most of them yielded the required DNA quantity. All frozen tissue samples had RNAs of good purity. RNA quality was confirmed by RIN, achieving values in most cases over 7 and efficient amplification of housekeeping genes by RT-qPCR, with no significant differences among samples from the same tissue type. In the "in process" Quality Controls, DNA, RNA, and histological integrity of tissues showed no differences among samples after different preservation times., Conclusion: Quality Control results have made it possible to validate the entire biobank process and confirm the utility of implementing QMS to guarantee the quality of a biospecimen collection., Competing Interests: The authors have declared that no competing interests exist., (Copyright: © 2022 Servais et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.)

Published
2022
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26. Risk factors of rejection after penetrating keratoplasty: a retrospective monocentric study.

Author

Debourdeau E, Builles N, Couderc G, Boulhic J, Chamard C, Villain M, Babeau F, and Daien V

Subjects
Humans, Male, Middle Aged, Female, Keratoplasty, Penetrating methods, Retrospective Studies, Graft Survival, Graft Rejection diagnosis, Graft Rejection etiology, Graft Rejection surgery, Risk Factors, Corneal Diseases diagnosis, Corneal Diseases surgery, Keratoconus surgery, Keratitis
Abstract

Purpose: To assess risk factors of rejection after penetrating keratoplasty (PKP)., Methods: This retrospective monocentric study assessed risk factors for rejection in patients who underwent PKP at Montpellier University Hospital between June 2005 and September 2018. Graft and donor data were obtained from our tissue bank in Montpellier. Clinical data of recipients were recorded from medical files. Survival was estimated by the Kaplan-Meir method. Potential risk factors of rejection were assessed by multivariate Cox proportional hazards analysis, estimating hazard ratios (HR) and 95% confidence intervals (CI)., Results: Among the 316 consecutive patients (59% male, mean SD] age 52 [17]), 360 eyes underwent PKP. Indications for PKP were bullous keratopathy (27%), infectious keratitis (20%), and keratoconus (15%). The median follow-up was 44 months (IQR 22-73). The overall graft survival and irreversible rejection rate at 5 years were 70% and 29%, respectively. Factors associated with risk of rejection were prior indication for graft rejection (SHR [CI 95%] = 7.8 [2.6-23.1]), trauma (SHR [CI 95%] = 3.6 [1.1-11.7]), and infectious keratitis (SHR [CI 95%] = 2.7 [1.2-11.1]), history of corneal neovascularization (SHR [CI 95%] = 2.1 [1.2-3.8]), hypertonia (SHR [CI 95%] = 2.8 [1.8-4.3]), and mixed sex matching (SHR [CI 95%] = 2.0 [1.01-4.0])., Conclusion: The significant risk factors of graft rejection after PKP found in this study agree with those from major international cohorts: prior indication for graft rejection, history of neovascularization and high intraocular pressure. Sex matching donor-recipient is a most recent parameter in the literature confirmed by the present analysis., Trial Registration: ClinicalTrials.gov Identifier: NCT04791696., (© 2022. The Author(s), under exclusive licence to Springer-Verlag GmbH Germany, part of Springer Nature.)

Published
2022
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28. Characterization of immortalized human islet stromal cells reveals a MSC-like profile with pancreatic features.

Author

Villard O, Armanet M, Couderc G, Bony C, Moreaux J, Noël D, De Vos J, Klein B, Veyrune JL, and Wojtusciszyn A

Subjects
Bone Marrow Cells, Cell Differentiation, Cell Proliferation, Cells, Cultured, Chondrogenesis, Humans, Leukocytes, Mononuclear, Islets of Langerhans, Mesenchymal Stem Cells
Abstract

Background: Mesenchymal stromal cells (MSCs) represent an interesting tool to improve pancreatic islet transplantation. They have immunomodulatory properties and secrete supportive proteins. However, the functional properties of MSCs vary according to many factors such as donor characteristics, tissue origin, or isolation methods. To counteract this heterogeneity, we aimed to immortalize and characterize adherent cells derived from human pancreatic islets (hISCs), using phenotypic, transcriptomic, and functional analysis., Methods: Adherent cells derived from human islets in culture were infected with a hTERT retrovirus vector and then characterized by microarray hybridization, flow cytometry analysis, and immunofluorescence assays. Osteogenic, adipogenic, and chondrogenic differentiation as well as PBMC proliferation suppression assays were used to compare the functional abilities of hISCs and MSCs. Extracellular matrix (ECM) gene expression profile analysis was performed using the SAM (Significance Analysis of Microarrays) software, and protein expression was confirmed by western blotting., Results: hISCs kept an unlimited proliferative potential. They exhibited several properties of MSCs such as CD73, CD90, and CD105 expression and differentiation capacity. From a functional point of view, hISCs inhibited the proliferation of activated peripheral blood mononuclear cells. The transcriptomic profile of hISCs highly clusterized with bone marrow (BM)-MSCs and revealed a differential enrichment of genes involved in the organization of the ECM. Indeed, the expression and secretion profiles of ECM proteins including collagens I, IV, and VI, fibronectin, and laminins, known to be expressed in abundance around and within the islets, were different between hISCs and BM-MSCs., Conclusion: We generated a new human cell line from pancreatic islets, with MSCs properties and retaining some pancreatic specificities related to the production of ECM proteins. hISCs appear as a very promising tool in islet transplantation by their availability (as a source of inexhaustible source of cells) and ability to secrete a supportive "pancreatic" microenvironment.

Published
2020
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29. Microbial contamination and tissue procurement location: A conventional operating room is not mandatory. An observational study.

Author

Louart B, Charles C, Nguyen TL, Builles N, Roger C, Lefrant JY, Vachiery-Lahaye F, De Vos J, Couderc G, and Muller L

Subjects
Adult, Aged, Female, France, Humans, Intensive Care Units standards, Male, Middle Aged, Morgue standards, Operating Rooms standards, Patient Transfer standards, Practice Guidelines as Topic, Retrospective Studies, Tissue Banks statistics & numerical data, Tissue and Organ Harvesting adverse effects, Tissue and Organ Harvesting methods, Air Microbiology standards, Allografts microbiology, Tissue and Organ Harvesting standards, Tissue and Organ Procurement standards
Abstract

Background: Standard operating rooms (SOR) are assumed to be the best place to prevent microbial contamination when performing tissue procurement. However, mobilizing an operating room is time and cost consuming if no organ retrieval is performed. In such case, non-operating dedicated rooms (NODR) are usually recommended by European guidelines for tissue harvesting. Performing the tissue retrieval in the Intensive care unit (ICU) when possible might be considered as it allows a faster and simpler procedure., Objective: Our primary objective was to study the relationship between the risk of microbial contamination and the location (ICU, SOR or NODR) of the tissue retrieval in heart-beating and non-heart-beating deceased donors., Materials and Method: We retrospectively reviewed all deceased donors' files of the local tissue banks of Montpellier and Marseille from January 2007 to December 2014. The primary endpoint was the microbial contamination of the grafts. We built a multivariate regression model and used a GEE (generalized estimating equations) allowing us to take into account the clustered structure of our data., Results: 2535 cases were analyzed involving 1027 donors. The retrieval took place for 1189 in a SOR, for 996 in a hospital mortuary (NODR) and for 350 in an ICU. 285 (11%) microbial contaminations were revealed. The multivariate analysis found that the location in a hospital mortuary was associated with a lower risk of contamination (OR 0.43, 95% CI [0.2-0.91], p = 0.03). A procurement performed in the ICU was not associated with a significant increased risk (OR 0.62, 95% CI [0.26-1.48], p = 0.4)., Conclusion: According to our results, performing tissue procurement in dedicated non-sterile rooms could decrease the rate of allograft tissue contamination. This study also suggests that in daily clinical practice, transferring patients from ICU to SOR for tissue procurement could be avoided as it does not lead to less microbial contamination., Competing Interests: The authors have declared that no competing interests exist.

Published
2019
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30. Corrective GUSB transfer to the canine mucopolysaccharidosis VII cornea using a helper-dependent canine adenovirus vector.

Author

Serratrice N, Cubizolle A, Ibanes S, Mestre-Francés N, Bayo-Puxan N, Creyssels S, Gennetier A, Bernex F, Verdier JM, Haskins ME, Couderc G, Malecaze F, Kalatzis V, and Kremer EJ

Subjects
Adenoviruses, Human genetics, Animals, Cheirogaleidae, Corneal Opacity enzymology, Corneal Opacity pathology, Corneal Stroma pathology, Corneal Stroma ultrastructure, Disease Models, Animal, Dogs, Genetic Therapy, Genetic Vectors, Glycosaminoglycans metabolism, Helper Viruses, Humans, In Vitro Techniques, Lysosomes enzymology, Mice, Mice, Inbred C57BL, Microscopy, Confocal, Microscopy, Electron, Transmission, Mucopolysaccharidosis VII enzymology, Mucopolysaccharidosis VII pathology, Species Specificity, Adenoviruses, Canine genetics, Corneal Opacity therapy, Corneal Stroma enzymology, Gene Transfer Techniques, Glucuronidase genetics, Mucopolysaccharidosis VII therapy
Abstract

Corneal transparency is maintained, in part, by specialized fibroblasts called keratocytes, which reside in the fibrous lamellae of the stroma. Corneal clouding, a condition that impairs visual acuity, is associated with numerous diseases, including mucopolysaccharidosis (MPS) type VII. MPS VII is due to deficiency in β-glucuronidase (β-glu) enzymatic activity, which leads to accumulation of glycosaminoglycans (GAGs), and secondary accumulation of gangliosides. Here, we tested the efficacy of canine adenovirus type 2 (CAV-2) vectors to transduce keratocyte in vivo in mice and nonhuman primates, and ex vivo in dog and human corneal explants. Following efficacy studies, we asked if we could treat corneal clouding by the injection a helper-dependent (HD) CAV-2 vector (HD-RIGIE) harboring the human cDNA coding for β-glu (GUSB) in the canine MPS VII cornea. β-Glu activity, GAG content, and lysosome morphology and physiopathology were analyzed. We found that HD-RIGIE injections efficiently transduced coxsackievirus adenovirus receptor-expressing keratocytes in the four species and, compared to mock-injected controls, improved the pathology in the canine MPS VII cornea. The key criterion to corrective therapy was the steady controlled release of β-glu and its diffusion throughout the collagen-dense stroma. These data support the continued evaluation of HD CAV-2 vectors to treat diseases affecting corneal keratocytes., (Copyright © 2014 Elsevier B.V. All rights reserved.)

Published
2014
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31. Wetting properties and critical micellar concentration of benzalkonium chloride mixed in sodium hypochlorite.

Author

Bukiet F, Couderc G, Camps J, Tassery H, Cuisinier F, About I, Charrier A, and Candoni N

Subjects
Analysis of Variance, Anti-Infective Agents, Local chemistry, Benzalkonium Compounds toxicity, Chlorine analysis, Enterococcus faecalis drug effects, Fibroblasts drug effects, Humans, Sodium Hypochlorite toxicity, Statistics, Nonparametric, Surface Tension, Wettability, Wetting Agents chemistry, Wetting Agents toxicity, Benzalkonium Compounds chemistry, Micelles, Root Canal Preparation, Sodium Hypochlorite chemistry, Therapeutic Irrigation
Abstract

Introduction: The purposes of the present study were to (1) assess the effect of the addition of benzalkonium chloride to sodium hypochlorite on its wetting properties, contact angle, and surface energy; (2) determine the critical micellar concentration of benzalkonium chloride in sodium hypochlorite; and (3) investigate the influence of addition of benzalkonium chloride on the free chlorine level, cytotoxicity, and antiseptic properties of the mixture., Methods: Solutions of benzalkonium chloride, with concentrations ranging from 0%-1%, were mixed in 2.4% sodium hypochlorite and tested as follows. The wetting properties were investigated by measuring the contact angle of the solutions on a nondehydrated dentin surface by using the static sessile drop method. The pending drop technique was subsequently used to determine the surface energy of the solutions. The critical micellar concentration of benzalkonium chloride mixed in sodium hypochlorite was calculated from the data. When 2.4% NaOCl was mixed with benzalkonium chloride at the critical micellar concentration, 3 parameters were tested: free chloride content, cytotoxicity, and antibacterial effects against Enterococcus faecalis., Results: The contact angle (P < .001) as well as the surface energy (P < .001) significantly decreased with increasing benzalkonium chloride concentrations. The critical micellar concentration of benzalkonium chloride in sodium hypochlorite was 0.008%. At this concentration, the addition of benzalkonium chloride had no effect on the free chlorine content, cytotoxicity, or antibacterial efficiency of the mixture., Conclusions: The addition of benzalkonium chloride to sodium hypochlorite at the critical micellar concentration reduced the contact angle by 51.2% and the surface energy by 53.4%, without affecting the free chloride content, cytotoxicity, or antibacterial properties of the mixture., (Copyright © 2012 American Association of Endodontists. Published by Elsevier Inc. All rights reserved.)

Published
2012
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32. Use of the ditramax system to communicate esthetic specifications to the laboratory.

Author

Margossian P, Laborde G, Koubi S, Couderc G, and Mariani P

Subjects
Cuspid anatomy & histology, Dental Technicians, Dentists, Equipment Design, Esthetics, Face anatomy & histology, Humans, Incisor anatomy & histology, Interprofessional Relations, Jaw Relation Record instrumentation, Models, Dental, Communication, Dental Prosthesis Design instrumentation, Esthetics, Dental, Laboratories, Dental, Prescriptions
Abstract

Prosthetic restoration of the anterior teeth is a major esthetic challenge. Esthetic treatment consists of creating pleasantly proportioned teeth and integrating them harmoniously into the patient's gingiva, lips, and face. The communication of clinical data to the laboratory is critical to the success of any esthetic treatment. The purpose here is to present a straightforward, efficient, and reproducible means of communicating esthetic specifications to ceramists, allowing them to work as though the patient was actually in front of them, with access to all of the major facial esthetic criteria.

Published
2011

33. Alignment and relaxation dynamics of dye molecules in host-guest inclusion compounds as probed by dielectric spectroscopy.

Author

Tsuwi J, Berger R, Labat G, Couderc G, Behrnd NR, Ottiger P, Cucinotta F, Schürmann K, Bertoni M, Viani L, Gierschner J, Cornil J, Prodi-Schwab A, De Cola L, Wübbenhorst M, and Hulliger J

Abstract

The alignment and relaxation dynamics of a polar dye molecule, N,N-dimethyl-4(4-nitrophenylazo)aniline (DNAA), in zeolite L and perhydrotriphenylene (PHTP) channels were investigated by means of a combination of optical, dielectric, and quantum-chemical methods. Both the zeolite L and PHTP channels enable the dye molecules to align along the channel axis. An amplified net dipole moment of DNAA in PHTP is observed and attributed to enhanced 1D close alignment of dye molecules. In zeolite L channels, a concentration gradient is found with aggregation at the channel entrances. The dynamics of the dye in zeolite L channels reveals localized conical rotational fluctuation modes following Arrhenius-type activation with energy of 0.31 eV, which we assign to small noninteracting fluctuating polar units of the dyes being loosely aligned or isolated. Unlike zeolite L, relaxations in PHTP are characterized by cooperative wobbling motions interpreted as increased intermolecular dipole interaction due to a closely packed one-dimensional array. Temperature-dependent activation energies of 0.25 eV below 0 degrees C and 0.37 eV at ambient temperature reflect the role of the soft channel walls in the activation process.

Published
2010
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34. Delineation of the roles of paracrine and autocrine interleukin-6 (IL-6) in myeloma cell lines in survival versus cell cycle. A possible model for the cooperation of myeloma cell growth factors.

Author

Jourdan M, Mahtouk K, Veyrune JL, Couderc G, Fiol G, Redal N, Duperray C, De Vos J, and Klein B

Subjects
Antibodies, Monoclonal pharmacology, Apoptosis, Autocrine Communication, Cell Line, Tumor, Humans, Interleukin-6 genetics, Interleukin-6 pharmacology, Myeloid Cell Leukemia Sequence 1 Protein, Neoplasm Proteins genetics, Neoplasm Proteins metabolism, Paracrine Communication, Proto-Oncogene Proteins c-bcl-2 genetics, Proto-Oncogene Proteins c-bcl-2 metabolism, Cell Cycle, Cell Survival, Interleukin-6 metabolism, Multiple Myeloma metabolism, Multiple Myeloma pathology
Abstract

Primary myeloma cells rapidly apoptose as soon as they are removed from their bone-marrow environment. A likely explanation is that the tumor environment produces survival factors that may counteract a spontaneous activation of pro-apoptotic program. Additional factors may trigger cell cycling in surviving myeloma cells. Interleukin-6 (IL-6) is a well recognized myeloma cell growth factor produced mainly by the tumor environment. However, myeloma cells themselves may produce low levels of autocrine IL-6. The respective roles of paracrine versus autocrine IL-6 are a matter of debate. We investigated these roles using the XG-6 myeloma cell line whose growth is dependent on addition of exogenous IL-6, despite its weak IL-6 mRNA and protein expression. The apoptosis induced by exogenous IL-6 deprivation was blocked by transferring the Mcl-1 gene coding for an anti-apoptotic protein in XG-6 cells. An XG-6Mcl-1 cell line which can survive and grow without adding IL-6 was obtained. We show that anti-IL-6 or anti-gp130 antibodies abrogated cell cycling whereas they did not affect cell survival. These data indicate that the weak autocrine IL-6 produced by myeloma cells is sufficient to trigger cell cycling whereas their survival requires large exogenous IL-6 concentrations. This important role of autocrine IL-6 has to be considered when evaluating the mechanism of action of myeloma cell growth factors. These factors may actually block an activated pro-apoptotic program, making possible a weak production of autocrine IL-6 to promote cell cycling.

Published
2005

35. A major role for Mcl-1 antiapoptotic protein in the IL-6-induced survival of human myeloma cells.

Author

Jourdan M, Veyrune JL, De Vos J, Redal N, Couderc G, and Klein B

Subjects
Antibodies immunology, Antigens, CD immunology, Antigens, CD metabolism, Apoptosis physiology, Cytokine Receptor gp130, Genetic Vectors, Humans, In Vitro Techniques, Membrane Glycoproteins immunology, Membrane Glycoproteins metabolism, Multiple Myeloma pathology, Myeloid Cell Leukemia Sequence 1 Protein, Proto-Oncogene Proteins c-bcl-2 biosynthesis, Proto-Oncogene Proteins c-bcl-2 genetics, Proto-Oncogene Proteins c-bcl-2 metabolism, Retroviridae, Transduction, Genetic, Tumor Cells, Cultured, Cell Survival physiology, Interleukin-6 metabolism, Multiple Myeloma metabolism, Neoplasm Proteins metabolism
Abstract

Interleukin-6 (IL-6) is a major survival factor for malignant plasma cells involved in multiple myeloma. Using an RNase protection assay, we looked for gene expression of 10 anti- and proapoptotic Bcl-2-family proteins in 12 IL-6-dependent human myeloma cell lines (HMCL). A high Mcl-1 gene expression was found in all HMCLs and the other genes were variably expressed. Out of the 10 Bcl-2-family members, only the Mcl-1 gene was regulated by IL-6. Upon starvation of IL-6, Mcl-1 gene expression decreased in association with myeloma cell apoptosis and was upregulated after adding IL-6 again in association with myeloma cell survival. A constitutive Mcl-1 expression was induced with an Mcl-1-GFP retrovirus in two IL-6-dependent HMCLs. The Mcl-1 HMCLs have a marked reduced apoptosis upon IL-6 starvation compared to HMCLs transduced with control GFP retrovirus and may grow without adding IL-6. These data emphasize the major role of Mcl-1 antiapoptotic protein in the IL-6-induced survival of human myeloma cells.

Published
2003
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36. Cooperation between heparin-binding EGF-like growth factor and interleukin-6 in promoting the growth of human myeloma cells.

Author

Wang YD, De Vos J, Jourdan M, Couderc G, Lu ZY, Rossi JF, and Klein B

Subjects
Antigens, CD metabolism, Apoptosis, Autocrine Communication, Cell Division drug effects, Cell Survival drug effects, Dose-Response Relationship, Drug, Drug Synergism, ErbB Receptors genetics, ErbB Receptors metabolism, Heparin-binding EGF-like Growth Factor, Humans, Intercellular Signaling Peptides and Proteins, Kinetics, Models, Biological, Multiple Myeloma metabolism, RNA, Neoplasm biosynthesis, Tetraspanin 29, Tumor Cells, Cultured, Epidermal Growth Factor pharmacology, Interleukin-6 pharmacology, Membrane Glycoproteins, Multiple Myeloma pathology
Abstract

Interleukin-6 (IL-6) is a major survival and proliferation factor of human malignant plasma cells and IL-6 dependent myeloma cell lines can be obtained from patients with terminal disease. We show here that mutated diphtheria toxin, a specific inhibitor of heparin-binding epidermal growth factor-like growth factor (HB-EGF), blocked the IL-6-induced growth of two myeloma cell lines (XG-1 and XG-14) and did not significantly affect that of two other cell lines (XG-6 and XG-13). The IL-6 mediated growth of myeloma cells was also inhibited by antibodies to ErbB1, a receptor for HB-EGF. The XG-1 and XG-14 cell lines that are sensitive to HB-EGF inhibitors overexpressed HB-EGF and EGF receptor (ErbB1) genes. They also overexpressed CD9, a tetraspanin that binds to the heparin-binding domain of HB-EGF and is critical for promoting ErbB1 activation by HB-EGF. The XG-6 and XG-13 myeloma cells that were not significantly sensitive to HB-EGF antagonists, poorly expressed HB-EGF, ErbB1 and CD9 genes or proteins. We demonstrated that recombinant HB-EGF supported the long-term growth of myeloma cells, as did IL-6. The myeloma cell growth factor activity of HB-EGF was completely inhited by antibodies to ErbB1, but also by antibodies to gp130 IL-6 transducer or to IL-6. These data indicate that in the XG-1 and XG-14 IL-6-dependent myeloma cell lines, the CD9/HB-EGF/erbB1 and the IL-6/IL-6R/gp130 pathways cooperate synergistically to trigger myeloma cell growth. They suggest that inhibitors of the EGF receptor or HB-EGF may be useful for inducing myeloma cell apoptosis in patients with multiple myeloma.

Published
2002
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37. Identifying intercellular signaling genes expressed in malignant plasma cells by using complementary DNA arrays.

Author

De Vos J, Couderc G, Tarte K, Jourdan M, Requirand G, Delteil MC, Rossi JF, Mechti N, and Klein B

Subjects
B-Lymphocytes metabolism, Cell Division drug effects, Epidermal Growth Factor metabolism, Flow Cytometry, Gene Expression genetics, Heparin-binding EGF-like Growth Factor, Humans, Intercellular Signaling Peptides and Proteins, Multiple Myeloma genetics, Multiple Myeloma pathology, Neoplasm Proteins genetics, Neoplasm Proteins metabolism, Plasma Cells pathology, Reverse Transcriptase Polymerase Chain Reaction, Tumor Cells, Cultured, Multiple Myeloma metabolism, Oligonucleotide Array Sequence Analysis methods, Plasma Cells metabolism, Signal Transduction genetics
Abstract

In multiple myeloma (MM), the growth of primary plasma cells depends not only on interleukin-6 (IL-6), but also on additional unidentified signals delivered by the bone marrow environment. Using Atlas complementary DNA (cDNA) arrays comprising 268 genes coding for intercellular signaling molecules, this study identified genes that are overexpressed in myeloma cells compared to autologous B-lymphoblastoid cell lines. These genes encode the oncogenic Tyro3 tyrosine kinase receptor, the heparin-binding epidermal growth factor-like growth factor (HB-EGF) that is an epithelial autocrine tumor growth factor, the thrombin receptor (TR) that is linked to HB-EGF and syndecan-1 processing and to cell invasion, chemokine receptors CCR1 and CCR2, the Wnt pathway actor Frizzled-related protein (FRZB), and the Notch receptor ligand Jagged 2. These data, obtained with the Atlas cDNA array, were confirmed by reverse transcriptase-polymerase chain reaction or protein analysis or both. Furthermore, Tyro3, HB-EGF, TR, and FRZB gene expression was documented in purified primary malignant plasma cells from patients with plasma cell leukemia or MM. HB-EGF and FRZB were poorly expressed in purified polyclonal plasma cells. Finally, HB-EGF was proved to be an essential autocrine growth factor for the XG-1 myeloma cells. This study shows the potency and the biologic relevance of cDNA arrays used to analyze simultaneously a large panel of intercellular signaling genes and, by identifying several genes overexpressed in malignant plasma cells, opens new fields of investigation in MM biology. (Blood. 2001;98:771-780)

Published
2001
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38. CD4+ T cell surface CCR5 density as a determining factor of virus load in persons infected with human immunodeficiency virus type 1.

Author

Reynes J, Portales P, Segondy M, Baillat V, André P, Réant B, Avinens O, Couderc G, Benkirane M, Clot J, Eliaou JF, and Corbeau P

Subjects
Acquired Immunodeficiency Syndrome virology, Adult, HLA-DR Antigens analysis, Humans, Acquired Immunodeficiency Syndrome immunology, CD4-Positive T-Lymphocytes chemistry, HIV-1 isolation & purification, Receptors, CCR5 analysis, Viremia virology
Abstract

The intensity of expression of the chemokine receptor CCR5 is involved in in vitro cell infectability by human immunodeficiency virus (HIV)-1 R5 isolates. Because CCR5 expression varies among individuals, the hypothesis that this expression could determine virus load in HIV-1-infected persons was tested. The mean number of CCR5 molecules per cell was measured on peripheral blood CD4+ T lymphocytes (CCR5 density) from HIV-1-infected, asymptomatic, nontreated adults. There was a strong correlation between HIV RNA plasma level and CCR5 density (P=.009) that was independent of cell activation and was not due to an HIV-induced CCR5 up-regulation. These data are compatible with the hypothesis that CCR5 density is a key factor governing cell infectability and in vivo virus production and explain the protective effect of the Delta32CCR5 deletion, which results in low CCR5 expression. CCR5 density might be of critical predictive value in HIV infection.

Published
2000
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