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1. RAT INTERLEUKIN-2 IMMUNOGLOBULIN M FUSION PROTEINS ARE CYTOTOXIC IN VITRO FOR CELLS EXPRESSING THE IL-2 RECEPTOR AND CAN ABOLISH CELL-MEDIATED IMMUNITY IN VIVO

Author

Parker Ke, Ignacio Anegon, Lang F, J. P. Soulillou, Le Mauff B, Yannick Jacques, and Bogers Wm

Subjects
Cytotoxicity, Immunologic, Interleukin 2, Recombinant Fusion Proteins, T cell, Molecular Sequence Data, CHO Cells, Cell Line, Mice, Cricetinae, Rats, Inbred BN, medicine, Animals, Cytotoxic T cell, Hypersensitivity, Delayed, IL-2 receptor, Immunity, Cellular, Transplantation, Base Sequence, biology, Chemistry, Chinese hamster ovary cell, Receptors, Interleukin-2, Fusion protein, Molecular biology, Rats, Raji cell, medicine.anatomical_structure, Immunoglobulin M, Antibody Formation, biology.protein, Interleukin-2, Antibody, medicine.drug
Abstract

A hybrid cDNA coding for a fusion protein between rat interleukin 2 (IL-2) and a truncated heavy chain from rat immunoglobulin M (IgM) was constructed. The rat IL-2 and rat IgM CH2-3-4 hybrid gene was subcloned into a vector (PKCR6) for expression of the fusion molecule in Chinese hamster ovary (CHO) cells. Cells transfected with the hybrid cDNA secrete multimeric forms of the fusion protein (IL-2-Mu). Size analysis of the construct revealed that the majority (95%) of the secreted proteins have a high mw (> 500 kDa). The IL-2-Mu construct bind specifically to cells bearing the IL-2 receptors (IL-2R) with a binding affinity around 5 nM. The specific binding to IL-2R leads to T cell proliferation or, if rabbit complement is added, to T cell lysis. Multimeric forms (> 500 kDa) of the fusion protein mediate complement-dependent lysis but trigger only weak proliferation when compared with the low-mw forms (< 500 kDa). In contrast, the latter only efficiently mediate T cell proliferation without inducing complement-dependent lysis. After intravenous administration of CHO supernatant containing IL-2-Mu, or purified IL-2-Mu proteins into rats, the fusion proteins disappeared from the circulation with a t1/2 of 1 hr. The circulating IL-2-Mu constructs in the rat serum retained their capacity to induce complement-dependent lysis of IL-2R-bearing T cells in vitro. Furthermore, the IL-2-Mu construct was able to suppress the delayed-type hypersensitivity (DTH) reaction (an IL-2R, T helper cell-dependent event) in mice. A weak immune response (antirat IL-2-Mu antibodies) was observed when rats received multiple daily injections of the construct.

Published
1994

2. PREVENTION OF ACUTE REJECTION EPISODES WITH AN ANTI-INTERLEUKIN 2 RECEPTOR MONOCLONAL ANTIBODY

Author

J. P. Soulillou, Georges Karam, Jacques Dantal, Yannick Jacques, Diego Cantarovich, R. Baatard, Le Mauff B, Denis M, and M. Hourmant

Subjects
Transplantation, medicine.medical_specialty, Kidney, biology, medicine.drug_class, business.industry, medicine.medical_treatment, Azathioprine, Immunosuppression, medicine.disease, Monoclonal antibody, Gastroenterology, medicine.anatomical_structure, Internal medicine, Monoclonal, Immunology, medicine, biology.protein, Antibody, business, Kidney transplantation, medicine.drug
Abstract

The focus of progress in transplantation immunosuppression is to achieve more specific immunosuppression with monoclonal antibodies. We have already shown that the efficacy of 33B3.1, a rat monoclonal Ig2A directed against the human IL-2 receptor, was similar to that of rabbit antithymocyte globulin in the prevention of acute rejection in first kidney transplants. A similar comparative analysis has been made in 40-sec renal transplants. ATG (1 mg/kg/day) or 33B3.1 (10 mg/day) was administered during the first 10 days postgrafting in association with corticosteroids and azathioprine. Cyclosporine was introduced on day 9 and azathioprine/CsA constituted the patient's maintenance treatment after day 45. Rejection treatment consisted of equine antilymphocyte globulin in both cases and of steroid boluses when patients were under Cyclosporine. One patient in each group died. Graft survival was 90%, 85%, and 79% in the ATG group (n = 20) and 100%, 89%, and 89% in the 33B3.1 group (n = 20) at 3, 12, and 24 months, respectively. Of the ATG group patients, 45% and 40% in the 33B3.1 group had at least one rejection episode, half the episodes in the MoAb cohort occurring under 33B3.1, vs. none in the ATG group. Transplant function was similar in both groups. Viral infections appeared to be more frequent with ATG (60%) than with 33B3.1 (12%), with CMV accounting for half of these in the ATG group, and none in the MoAb group. Tolerance of both agents was good. Of the 33B3.1 recipients, 70% developed anti-33B3.1 antibodies. From these data, we conclude that this anti-IL-2 receptor MoAb seems less effective than rabbit ATG as induction treatment in second kidney transplant patients.

Published
1994

3. Xenoreactivity in the pig islet to human combination: feasibility of adenovirus-mediated gene transfer into pig islets

Author

Mirenda V, Beatrice CHARREAU, Sigalla J, Cassard A, Jm, Huvelin, David A, Jp, Soulillou, Le Mauff B, and Anegon I

Subjects
Adult, Swine, Adenoviruses, Human, Genetic Vectors, Transplantation, Heterologous, Infant, Newborn, Islets of Langerhans Transplantation, Antibodies, Heterophile, CD59 Antigens, Fetal Blood, Transfection, beta-Galactosidase, Islets of Langerhans, Antigens, Heterophile, Lectins, Animals, Feasibility Studies, Humans, Rabbits, Cells, Cultured
Published
1996

4. A dose-searching trial of an anti-LFA1 monoclonal antibody in first kidney transplant recipients

Author

Le Mauff B, Yannick Le Meur, Hourmant M, Debray M, Boeffard F, Alberici G, Jp, Soulillou, and Jm, Scherrmann

Subjects
Adult, Graft Rejection, Male, Adolescent, Dose-Response Relationship, Drug, Antibodies, Monoclonal, Humans, Female, Pilot Projects, Middle Aged, Kidney Transplantation, Lymphocyte Function-Associated Antigen-1
Abstract

25.3, a mouse IgG1 monoclonal antibody (MoAb), directed at the alpha chain of the LFA1 molecule (CD11a) has been used in prophylaxis of rejection in recipients of cadaveric kidney graft. Promising clinical results have been obtained for both tolerance and efficacy [1]. The aim of this trial was to determine the optimal dosage, base on a pharmacokinetic-pharmacodynamic analysis of the data obtained from the 15 patients included in this dose-searching study. Biological parameters, such as circulating levels and functional inhibition (as detected in an adhesion assay of patient lymphocytes), were measured during and after treatment. A Hill relation was calculated between the effect and the concentration measured and led us to select a 15 mg/day dose for further clinical trials, with a loading dose of 30 mg. An additional group receiving this protocol was submitted to the same calculation, and the results from this last group were in agreement with this previous analysis.

Published
1996

6. Permanent expression of human CD59 and/or decay-accelerating factor by rat endothelial cells confers protection from human complement-mediated lysis

Author

Beatrice CHARREAU, Cassard A, Tesson L, Le Mauff B, Blanchard D, Lublin D, Jp, Soulillou, and Anegon I

Subjects
Complement Inactivator Proteins, Membrane Glycoproteins, CD55 Antigens, Cell Survival, CD59 Antigens, Complement System Proteins, Flow Cytometry, Transfection, Recombinant Proteins, Rats, Rats, Sprague-Dawley, Antigens, CD, Animals, Humans, Endothelium, Vascular, Aorta
Published
1995

8. Protection of rat endothelial cells from primate complement-mediated lysis by expression of human CD59 and/or decay-accelerating factor

Author

Beatrice CHARREAU, Cassard A, Tesson L, Le Mauff B, Jm, Navenot, Blanchard D, Lublin D, Jp, Soulillou, and Anegon I

Subjects
Cytotoxicity, Immunologic, Transplantation, Membrane Glycoproteins, CD55 Antigens, Cell Survival, Transplantation, Heterologous, Gene Transfer Techniques, Gene Expression, CD59 Antigens, Complement Membrane Attack Complex, Simian virus 40, Cell Transformation, Viral, Transfection, Fluorescence, Rats, Rats, Sprague-Dawley, Macaca fascicularis, Antigens, CD, Animals, Humans, Endothelium, Vascular
Abstract

The present study analyzed the ability of human decay-accelerating factor (DAF) and CD59 to protect rat endothelial cell (EC) clones from human and primate complement-mediated lysis. By flow cytometry and Scatchard analysis, we show that human DAF and/or CD59 cDNAs under the transcriptional control of elongation factor 1-alpha promoter were expressed at levels similar to or higher than that of a human EC line. Human DAF and CD59 were released from the surface of transfected rat cells by phosphatidylinositol phospholipase C, demonstrating that the two molecules were linked to the cell membrane by means of a glycolipid anchor. The functional activity of the two human C regulatory proteins expressed on rat EC lines was studied using an in vitro assay of C-dependent cytotoxic in which rat EC were incubated with human or nonhuman primate sera as sources of xenogeneic natural antibodies and C. We demonstrate that human and monkey xenogeneic natural antibodies bind to rat cells and induce lysis by a C-dependent mechanism involving mainly the C direct activation pathway. Our data indicate that human DAF and CD59, expressed either alone or in combination, abrogated all EC cytotoxicity, even in the presence of 50% human serum. This protective phenotype was correlated with decreased membrane attack complex (CD59 and/or DAF transfectants) and C3 deposition (DAF transfectants) on EC surface. Antibodies against the transfected molecules abolished the protection against C-mediated lysis.

Published
1994

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