Your search keyword '"Laurent Chevalet"' showing total 8 results

1. Demonstration of physicochemical and functional similarity between the proposed biosimilar adalimumab MSB11022 and Humira®

Author

Fabio D'Amici, Christèle Fremaux, Mara Rossi, Angelo Palmese, Mariagrazia Terlizzese, Laurent Chevalet, and Laurent Magnenat

Subjects

0301 basic medicine, Glycan, Stereochemistry, Immunology, MSB11022, TNF, FcR, 03 medical and health sciences, 0302 clinical medicine, Report, adalimumab, Site occupancy, Adalimumab, medicine, Animals, Humans, Immunology and Allergy, biosimilars, Biosimilar Pharmaceuticals, Functional similarity, biology, Chemistry, Humira®, Disulfide bond, Biosimilar, analytical similarity, Reference product, 030104 developmental biology, Biochemistry, Antirheumatic Agents, 030220 oncology & carcinogenesis, biology.protein, Higher Order Structure, medicine.drug

Abstract

Biosimilars are biological products that are highly similar to existing products approved by health authorities. Demonstration of similarity starts with the comprehensive analysis of the reference product and its proposed biosimilar at the physicochemical and functional levels. Here, we report the results of a comparative analysis of a proposed biosimilar adalimumab MSB11022 and its reference product, Humira®. Three batches of MSB11022 and up to 23 batches of Humira® were analyzed by a set of state-of-the-art orthogonal methods. Primary and higher order structure analysis included N/C-terminal modifications, molecular weight of heavy and light chains, C-terminal lysine truncation, disulfide bridges, secondary and tertiary structures, and thermal stability. Purity ranged from 98.4%–98.8% for MSB11022 batches (N = 3) and from 98.4%–99.6% for Humira® batches (N = 19). Isoform analysis showed 5 isoform clusters within the pI range of 7.94–9.14 and 100% glycan site occupancy for both MSB11022 and Humira®. Functional analysis included Fab-dependent inhibition of tumor necrosis factor (TNF)-induced cytotoxicity in L929-A9 cell line and affinity to soluble and transmembrane forms of TNF, as well as Fc-dependent binding to Fcγ and neonatal Fc receptors and C1q complement proteins. All tested physicochemical and functional parameters demonstrated high similarity of MSB11022 and Humira®, with lower variability between MSB11022 and Humira® batches compared with variability within individual batches of Humira®. Based on these results, MSB11022 is anticipated to have safety and efficacy comparable to those of Humira®.

Published

2016

2. A high-throughput protein refolding screen in 96-well format combined with design of experiments to optimize the refolding conditions

Author

Bruno Antonsson, Aurelie Hermant, Frédéric Borlat, Laurent Magnenat, Nicolas Barrillat, Mikael Paquet, Vincent Dechavanne, and Laurent Chevalet

Subjects

Inclusion Bodies, Anaphylatoxins, Chromatography, Chemistry, Design of experiments, Interleukin-17, Protein Renaturation, Chemokine CXCL13, Chemokine CXCL12, Recombinant Proteins, High-Throughput Screening Assays, Reducing Agents, Research Design, Protein refolding, Granulocyte Colony-Stimulating Factor, Interleukin 17F, Escherichia coli, Humans, Biological Assay, Cloning, Molecular, Throughput (business), Biotechnology

Abstract

Production of correctly folded and biologically active proteins in Escherichiacoli can be a challenging process. Frequently, proteins are recovered as insoluble inclusion bodies and need to be denatured and refolded into the correct structure. To address this, a refolding screening process based on a 96-well assay format supported by design of experiments (DOE) was developed for identification of optimal refolding conditions. After a first generic screen of 96 different refolding conditions the parameters that produced the best yield were further explored in a focused DOE-based screen. The refolding efficiency and the quality of the refolded protein were analyzed by RP-HPLC and SDS-PAGE. The results were analyzed by the DOE software to identify the optimal concentrations of the critical additives. The optimal refolding conditions suggested by DOE were verified in medium-scale refolding tests, which confirmed the reliability of the predictions. Finally, the refolded protein was purified and its biological activity was tested in vitro. The screen was applied for the refolding of Interleukin 17F (IL-17F), stromal-cell-derived factor-1 (SDF-1α/CXCL12), B cell-attracting chemokine 1 (BCA-1/CXCL13), granulocyte macrophage colony stimulating factor (GM-CSF) and the complement factor C5a. This procedure identified refolding conditions for all the tested proteins. For the proteins where refolding conditions were already available, the optimized conditions identified in the screening process increased the yields between 50% and 100%. Thus, the method described herein is a useful tool to determine the feasibility of refolding and to identify high-yield scalable refolding conditions optimized for each individual protein.

Published

2011

3. In vivo processing of CXCL12α/SDF-1α after intravenous and subcutaneous administration to mice

Author

Vincent Dechavanne, Bruno Antonsson, Laurent Chevalet, Patricia de Lys, and Ursula Boschert

Subjects

Ratón, Injections, Subcutaneous, medicine.medical_treatment, Lysine, Biology, Biochemistry, Mice, chemistry.chemical_compound, In vivo, medicine, Animals, Humans, Molecular Biology, chemistry.chemical_classification, Methionine, Protease, Molecular biology, Chemokine CXCL12, In vitro, Amino acid, Mice, Inbred C57BL, chemistry, Injections, Intravenous, biology.protein, Female, Antibody

Abstract

CXCL12α has been shown to be selectively processed at the N- and C-termini in blood and plasma in vitro. In order to study the processing in vivo, several versions of CXCL12α were expressed and purified. The protein was administered either iv or sc to mice, and at different time points postadministration plasma was collected and analyzed. To detect modifications of the CXCL12α molecule in crude plasma a SELDI TOF-MS-based method was developed. Anti-CXCL12 antibodies were immobilized on the SELDI chip and CXCL12α binding to the antibodies was detected by SELDI-TOF-MS. The protein was found to be processed both at the C- and N-termini. The same processed CXCL12α forms as detected in vitro were found; however, in addition further processing was detected at the N-terminus, where altogether seven amino acids were removed. At the C-terminus the lysine was removed as has been seen in vitro, and no further processing was detected. The full-length CXCL12α disappeared within minutes after administration, whereas the processed forms of the protein were detectable for up to 6-8 h postadministration. The same processed forms appeared after iv and sc administration, only the kinetics was different. When the shortest processed form detected in plasma, 7ΔN1ΔC-CXCL12α, was administered directly, no further processed forms were detected. Interestingly, a version of CXCL12α containing a N-terminal methionine was protected against N-terminal processing in plasma in vitro; however, in vivo no protection was seen, the protein was processed in the same way as full-length CXCL12α.

Published

2010

4. CD4+T-Cell-Mediated Antiviral Protection of the Upper Respiratory Tract in BALB/c Mice following Parenteral Immunization with a Recombinant Respiratory Syncytial Virus G Protein Fragment

Author

Claire-Anne Siegrist, Hélène Plotnicky-Gilquin, Alain Robert, Ultan F. Power, Jean-François Haeuw, Jean-Yves Bonnefoy, Thien Ngoc Nguyen, Christian Brandt, Alain Beck, and Laurent Chevalet

Subjects

CD4-Positive T-Lymphocytes, Adoptive cell transfer, G protein, Recombinant Fusion Proteins, T-Lymphocytes, Immunology, Mice, SCID, Respiratory Syncytial Virus Infections, Biology, Microbiology, Virus, Epitope, BALB/c, Mice, Viral Proteins, Viral Envelope Proteins, Pregnancy, Virology, medicine, Animals, Respiratory Tract Infections, B-Lymphocytes, Mice, Inbred BALB C, HN Protein, T helper cell, biology.organism_classification, Adoptive Transfer, Respiratory Syncytial Viruses, medicine.anatomical_structure, Insect Science, biology.protein, Pathogenesis and Immunity, Female, Immunization, Antibody, Immunity, Maternally-Acquired, CD8

Abstract

We analyzed the protective mechanisms induced against respiratory syncytial virus subgroup A (RSV-A) infection in the lower and upper respiratory tracts (LRT and URT) of BALB/c mice after intraperitoneal immunization with a recombinant fusion protein incorporating residues 130 to 230 of RSV-A G protein (BBG2Na). Mother-to-offspring antibody (Ab) transfer and adoptive transfer of BBG2Na-primed B cells into SCID mice demonstrated that Abs are important for LRT protection but have no effect on URT infection. In contrast, RSV-A clearance in the URT was achieved in a dose-dependent fashion after adoptive transfer of BBG2Na-primed T cells, while it was abolished in BBG2Na-immunized mice upon in vivo depletion of CD4+, but not CD8+, T cells. Furthermore, the conserved RSV-A G protein cysteines and residues 193 and 194, overlapping the recently identified T helper cell epitope on the G protein (P. W. Tebbey et al., J. Exp. Med. 188:1967–1972, 1998), were found to be essential for URT but not LRT protection. Taken together, these results demonstrate for the first time that CD4+T cells induced upon parenteral immunization with an RSV G protein fragment play a critical role in URT protection of normal mice against RSV infection.

Published

2000

5. Differences in the glycosylation of recombinant proteins expressed in HEK and CHO cells

Author

Laurent Chevalet, Flavie Robert, Francis Vilbois, Bruno Antonsson, Christian Arod, Laurence Delafosse, Amelie Croset, Ana Krstanovic, Christophe Losberger, Loic Glez, Damien Begue, and Jean-Philippe Gaudry

Subjects

Glycosylation, Bioengineering, CHO Cells, Biology, Transfection, Applied Microbiology and Biotechnology, Mass Spectrometry, chemistry.chemical_compound, Protein structure, N-linked glycosylation, Polysaccharides, Cricetinae, Animals, Humans, Peptide-N4-(N-acetyl-beta-glucosaminyl) Asparagine Amidase, chemistry.chemical_classification, Glycobiology, Isoelectric focusing, Chinese hamster ovary cell, HEK 293 cells, Electrophoresis, Capillary, Reproducibility of Results, General Medicine, Reference Standards, Recombinant Proteins, carbohydrates (lipids), Molecular Weight, HEK293 Cells, chemistry, Biochemistry, lipids (amino acids, peptides, and proteins), Electrophoresis, Polyacrylamide Gel, Isoelectric Focusing, Glycoprotein, Biotechnology

Abstract

Glycosylation is one of the most common posttranslational modifications of proteins. It has important roles for protein structure, stability and functions. In vivo the glycostructures influence pharmacokinetics and immunogenecity. It is well known that significant differences in glycosylation and glycostructures exist between recombinant proteins expressed in mammalian, yeast and insect cells. However, differences in protein glycosylation between different mammalian cell lines are much less well known. In order to examine differences in glycosylation in mammalian cells we have expressed 12 proteins in the two commonly used cell lines HEK and CHO. The cells were transiently transfected, and the expressed proteins were purified. To identify differences in glycosylation the proteins were analyzed on SDS-PAGE, isoelectric focusing (IEF), mass spectrometry and released glycans on capillary gel electrophoresis (CGE-LIF). For all proteins significant differences in the glycosylation were detected. The proteins migrated differently on SDS-PAGE, had different isoform patterns on IEF, showed different mass peak distributions on mass spectrometry and showed differences in the glycostructures detected in CGE. In order to verify that differences detected were attributed to glycosylation the proteins were treated with deglycosylating enzymes. Although, culture conditions induced minor changes in the glycosylation the major differences were between the two cell lines.

Published

2012

6. Design of Experiment in CHO and HEK transient transfection condition optimization

Author

Laurent Chevalet, Frederic Bollin, and Vincent Dechavanne

Subjects

Cell Survival, Cell Count, CHO Cells, Biology, Transfection, Antibodies, law.invention, chemistry.chemical_compound, Plasmid, Cricetulus, law, Cricetinae, Gene expression, Animals, Humans, Polyethyleneimine, Cloning, Molecular, Chinese hamster ovary cell, HEK 293 cells, Molecular biology, Recombinant Proteins, HEK293 Cells, chemistry, Cell culture, Research Design, Recombinant DNA, DNA, Biotechnology

Abstract

Transient gene expression (TGE) is a well-established enabling technology for rapid generation of recombinant proteins, with Human Embryonic Kidney (HEK) and Chinese Hamster Ovary (CHO) cell lines and polyethyleneimine (PEI) as the transfection reagent being its most popular components. However, despite considerable progress made in the field, volumetric titers can still be a limiting factor causing the manipulation of increasing quantities of culture media and DNA. Here, we report a systematic analysis of TGE conditions and their influence on yields and protein quality. Guided by Design of Experiments (DoE), we conclude that TGE yields with one test antibody can be maximized by a parallel increase of cell density - 2.4 to 3.0 × 10(6)cells/mL - and PEI concentration - 24 to 30 mg/L - while maintaining a 1:1 ratio of heavy chain and light chain encoding plasmids. Interestingly, we also show that in these conditions, DNA concentration can be maintained in the 1mg/L range, thereby limiting the need for large DNA preparations. Our optimized settings for PEI-mediated TGE in HEK and CHO cells evaluated on several proteins are generally applicable to recombinant antibodies and proteins.

Published

2010

7. Transformation of Aspergillus flavus: construction of urate oxidase-deficient mutants by gene disruption

Author

Bruno Cabane, Gérard Loison, Gérard Tiraby, and Laurent Chevalet

Subjects

Urate Oxidase, Restriction Mapping, Mutant, Aspergillus flavus, Biology, medicine.disease_cause, Nitrate Reductase, Transformation, Genetic, Nitrate Reductases, Genetics, medicine, Cloning, Molecular, Gene, Mutation, Genetic Complementation Test, Urate oxidase, General Medicine, biology.organism_classification, Uric Acid, Complementation, Blotting, Southern, Transformation (genetics), Biochemistry, Plasmids, Transformation efficiency

Abstract

A transformation procedure based on the complementation of a genetic defect was developed using a nitrate reductase-deficient mutant of Aspergillus flavus. The initial transformation efficiency was improved 40-fold by combining factors in a planned experimental program. Although low, this transformation rate was sufficient to obtain transformants in which the urate oxidase-encoding gene (uaZ) was disrupted in a gene replacement experiment. These new uaZ- strains were unable to utilize uric acid as the unique nitrogen source and could be reversed directly to the wild-type phenotype in second order transformation experiments using a urate oxidase-expressing vector.

Published

1992

8. Air-lift Bioreactor Improvement of Scale-up Linearity Between Shake Flasks and 25-L Scale in the Insect Cells—baculovirus Expression System

Author

Christophe Losberger, Laurent Chevalet, Frederic Bollin, and Thierry Battle

Subjects

Lift (force), Shake flask, Chromatography, Insect cell, Materials science, Scale (chemistry), SCALE-UP, Baculovirus expression, Bioreactor, Linearity

Published

2007