Your search keyword '"Amigorena S"' showing total 267 results

251. Deficient antigen processing of a protein quaternary structure can be overcome by receptor-mediated uptake.

Author

Rouas-Freiss N, Housseau F, Bidart JM, Bonnerot C, Amigorena S, Guillet JG, and Bellet D

Subjects

Animals, Antigen-Presenting Cells physiology, Cell Line, Female, Glycoprotein Hormones, alpha Subunit metabolism, Hybridomas metabolism, Mice, Mice, Inbred BALB C, Protein Biosynthesis, Protein Conformation, Antigen Presentation, Receptors, IgG physiology

Abstract

Human chorionic gonadotropin (hCG) is a dimer of non-covalently associated alpha (hCG-alpha) and beta (hCG-beta) subunits. This molecule was used to study whether receptor-mediated uptake influences the presentation of a protein quaternary structure. Unprimed splenocytes and a B cell lymphoma were capable of presenting only the free (hCG-alpha) but not the combined (hCG) alpha subunit to hCG-alpha T cell hybridomas, while hCG-alpha-primed lymph node cells (LNC) responded to both hCG-alpha and hCG. As antigen (Ag)-specific antigen-presenting cells (APC) present in the hCG-alpha-primed LNC population may be potentially effective for presenting hCG, we investigated the role of specific Ag capture, through mIg and Fc gamma R, in the processing and presentation of hCG and hCG-alpha to HAG5, a T cell hybridoma directed against the immunodominant region (amino acids 61-81) of hCG-alpha. Results showed that only B cells bearing membrane immunoglobulin capable of recognizing hCG-alpha and hCG, and present in hCG-alpha-primed mice, were extremely effective in presenting the free as well as the combined alpha subunit. The effect of FcR-mediated uptake was analyzed using a B cell line transfected with the Fc gamma RII-B2 gene to present immune complexes of either hCG-alpha or hCG. We found that hCG-alpha and hCG were presented equally well, whatever the Ag-binding site of each antibody to hCG or its alpha subunit. Using HBG 6, an hCG-beta T cell hybridoma, we performed similar experiments with the Fc gamma RII-B2 cell line and determined that the potentiation of hCG presentation to HBG 6 was similar to that observed with HAG 5. Then kinetic experiments were performed to examine the effect of Ag uptake through FcR on processing. Results demonstrated that the uptake pathway drastically influenced the expression of alpha T cell determinants in the alpha/beta dimer. In addition, treatment with cycloheximide, a protein synthesis inhibitor, only impaired the ability of APC to present specifically captured Ag. Thus, the processing pathway for specifically captured Ag might be different from the pathway used to process nonspecifically captured Ag. This observation might explain why receptor-enhanced uptake bypasses the inefficient processing of the hCG quaternary structure and enables similar efficiency in the presentation of alpha and beta T cell specificities. These findings provide new insight into the antigenicity of oligomeric molecules, which is modified whether antigen capture is specific or not.

Published

1993

252. Murine low-affinity receptors for the Fc portion of IgG. Roles in cell activation and ligand internalization.

Author

Bonnerot C and Amigorena S

Subjects

Amino Acid Sequence, Animals, Antigen-Antibody Complex metabolism, Humans, Immune System cytology, Immune System metabolism, Ligands, Mice, Molecular Sequence Data, Receptors, IgG classification, Receptors, IgG genetics, Receptors, IgG metabolism

Abstract

The low-affinity receptors for the Fc portion of IgG (Fc gamma R) are expressed on most of the cells of the immune system. They bind immune complexes but not monomeric IgG. These receptors are a family of surface glycoproteins with homologous extracellular domains and different transmembrane and cytoplasmic portions. This paper review the biological activities of Fc gamma R and focus on the molecular analysis done for the murine receptors involved in cell activation and ligand internalization.

Published

1993

253. Cytoplasmic domain heterogeneity and functions of IgG Fc receptors in B lymphocytes.

Author

Amigorena S, Bonnerot C, Drake JR, Choquet D, Hunziker W, Guillet JG, Webster P, Sautes C, Mellman I, and Fridman WH

Subjects

Amino Acid Sequence, Antigen-Antibody Complex metabolism, Antigen-Antibody Reactions genetics, Antigen-Antibody Reactions immunology, Antigens, CD genetics, Antigens, Differentiation genetics, Calcium metabolism, Dose-Response Relationship, Immunologic, Endocytosis genetics, Endocytosis immunology, Humans, Immunohistochemistry, Lymphocyte Activation immunology, Microscopy, Electron, Molecular Sequence Data, Receptors, Fc genetics, Receptors, IgG, Repressor Proteins pharmacology, Transcription Factors pharmacology, Transfection, Viral Proteins, Viral Regulatory and Accessory Proteins, Antigens, CD immunology, Antigens, Differentiation immunology, B-Lymphocytes immunology, DNA-Binding Proteins, Receptors, Fc immunology

Abstract

B lymphocytes and macrophages express closely related immunoglobulin G (IgG) Fc receptors (Fc gamma RII) that differ only in the structures of their cytoplasmic domains. Because of cell type-specific alternative messenger RNA splicing, B-cell Fc gamma RII contains an insertion of 47 amino acids that participates in determining receptor function in these cells. Transfection of an Fc gamma RII-negative B-cell line with complementary DNA's encoding the two splice products and various receptor mutants indicated that the insertion was responsible for preventing both Fc gamma RII-mediated endocytosis and Fc gamma RII-mediated antigen presentation. The insertion was not required for Fc gamma RII to modulate surface immunoglobulin-triggered B-cell activation. Instead, regulation of activation involved a region of the cytoplasmic domain common to both the lymphocyte and macrophage receptor isoforms. In contrast, the insertion did contribute to the formation of caps in response to receptor cross-linking, consistent with suggestions that the lymphocyte but not macrophage form of the receptor can associate with the detergent-insoluble cytoskeleton.

Published

1992

254. Structural bases of Fc gamma receptor functions.

Author

Fridman WH, Bonnerot C, Daeron M, Amigorena S, Teillaud JL, and Sautes C

Subjects

Amino Acid Sequence, Animals, Antigens, CD chemistry, Antigens, Differentiation genetics, Cell Line, Fibroblasts immunology, Humans, Leukemia, Basophilic, Acute immunology, Lymphoma, B-Cell immunology, Membrane Proteins chemistry, Molecular Sequence Data, Mutagenesis, Receptors, Fc genetics, Receptors, IgG, Solubility, Structure-Activity Relationship, Tumor Cells, Cultured, Antigens, Differentiation chemistry, Immunoglobulin G chemistry, Receptors, Fc chemistry

Published

1992

255. In vitro inhibition of tumor B cell growth by IgG-BF-producing Fc gamma RII+ T cell hybridoma and by immunoglobulin G-binding factors.

Author

Mathiot C, Amigorena S, Moncuit J, Sautès C, Fridman WH, and Teillaud JL

Subjects

Animals, B-Lymphocytes pathology, Cell Division, Down-Regulation, Hybridomas immunology, Mice, Suppressor Factors, Immunologic biosynthesis, T-Lymphocytes immunology, Tumor Cells, Cultured immunology, Tumor Cells, Cultured pathology, B-Lymphocytes immunology, Lymphokines biosynthesis, Prostatic Secretory Proteins, Receptors, IgG metabolism

Abstract

The growth-modulating effect on mouse hybridoma B cells of IgG-BF-producing Fc gamma RII+ mouse T cell hybridomas and of the IgG-BF isolated from the culture supernatants of these cells has been examined. Cocultures of IgG-secreting hybridoma B cells with IgG-BF-producing T hybridomas or with partially purified IgG-BF demonstrated a reproducible inhibition of the tumor B cell growth. The inhibition was due to a cytostatic and not to a cytotoxic effect. Hybridoma B cells cultured in liquid medium in the presence of soluble IgG-BF, or cocultured in semisolid agarose assays with IgG-BF-producing hybridoma T cells did not undergo immediate cytolysis but were prevented from proliferating. Thus, our data indicate that IgG-BF-producing Fc gamma RII+ T cells interfere with the proliferation of transformed B cells, possibly through soluble IgG-BF.

Published

1992

256. Murine soluble Fc gamma receptors/IgG-binding factors (IgG-BF): analysis of the relation to Fc gamma RII and production of milligram quantities of biologically active recombinant IgG-BF.

Author

Sautès C, Mazières N, Galinha A, Tartour E, Bonnerot C, Amigorena S, Teillaud C, Spagnoli R, and Fridman WH

Subjects

Amino Acid Sequence, Animals, Cell Line, Glycosylation, Immunoglobulin G biosynthesis, Lymphokines chemistry, Lymphokines genetics, Mice, Molecular Sequence Data, Molecular Weight, Receptors, IgG chemistry, Receptors, IgG genetics, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins genetics, Solubility, Suppressor Factors, Immunologic biosynthesis, Suppressor Factors, Immunologic chemistry, Suppressor Factors, Immunologic genetics, Transfection, Lymphokines biosynthesis, Prostatic Secretory Proteins, Receptors, IgG biosynthesis

Abstract

The production of soluble forms of low-affinity Fc gamma R by cells expressing recombinant or natural membrane Fc gamma RII, and the structural relationships between these soluble receptors and membrane Fc gamma RII are described. We show that 37-40 kD soluble Fc gamma RII, corresponding to the two N-terminal domains of Fc gamma RII and binding to IgG, are spontaneously produced in vitro by cleavage of membrane Fc gamma RII. Moreover, we describe methods to produce and purify to homogeneity large quantities of endotoxin-free recombinant IgG-binding factor (rIgG-BF) from the culture medium of a cell line transfected with a mutated Fc gamma RII cDNA. These methods include the use of bioreactors for culturing transfected fibroblasts and the purification of rIgG-BF by ion-exchange chromatography and hydrophobic-interaction chromatography. By using such procedures, about 2.4 mg of rIgG-BF were purified from 1 liter of culture medium of transfected fibroblasts. Like natural IgG-BF, the 95-99% pure rIgG-BF suppressed, in a dose-dependent manner, secondary in vitro IgG antibody responses to sheep red blood cells.

Published

1992

257. 21.1.1, a novel activation marker of T and B cells.

Author

Malard V, Amigorena S, Bauvois B, Daeron M, Cousin MA, Lando D, Fridman WH, and Sautes C

Subjects

Animals, Antigens, Differentiation, B-Lymphocyte chemistry, Antigens, Differentiation, T-Lymphocyte chemistry, Flow Cytometry, Isoelectric Point, Mice, Molecular Weight, Spleen cytology, Thymus Gland embryology, Thymus Gland growth & development, Thymus Gland immunology, Time Factors, Antibodies, Monoclonal immunology, Antigens, Differentiation, B-Lymphocyte immunology, Antigens, Differentiation, T-Lymphocyte immunology, B-Lymphocytes immunology, Lymphocyte Activation, T-Lymphocytes immunology

Abstract

A new rat mAb designated mAb 21.1.1 was raised against a T cell hybridoma of mouse origin, T2D4. This antibody, an IgG2b, immunoprecipitates from the membrane extracts of iodinated T2D4 cells a 56-kDa glycoprotein of apparent pI 4.6 which gives a 34-kDa polypeptide after treatment with endoglycosidase F. MAb 21.1.1 reacts with an antigen expressed on murine mitogen-activated thymocytes and T cells, and on B cells stimulated by anti-IgM antibodies. Cells isolated from the spleen, lymph nodes and bone marrow are negative, as are purified resting B cells or T cells. This antigen is strongly expressed on most day-16 fetal thymocytes whereas adult thymocytes are almost negative. mAb 21.1.1 may be useful for the study of activation and differentiation of T and B cells.

Published

1991

258. Recombinant interleukin 2-activated natural killer cells regulate IgG2a production.

Author

Amigorena S, Bonnerot C, Fridman WH, and Teillaud JL

Subjects

Animals, B-Lymphocytes metabolism, Blotting, Northern, Cells, Cultured, Dose-Response Relationship, Drug, Gene Expression, In Vitro Techniques, Interferon-gamma physiology, Killer Cells, Natural metabolism, Mice, Mice, Nude, RNA analysis, Receptors, Antigen, T-Cell biosynthesis, Recombinant Proteins pharmacology, Immunoglobulin G biosynthesis, Interleukin-2 pharmacology, Killer Cells, Natural physiology, Lymphocyte Activation drug effects

Abstract

In this report we have analyzed the effect of recombinant interleukin 2 (rIL 2) and rIL 2-activated natural killer (NK) cells on the production of immunoglobulin isotypes by lipopolysaccharide (LPS)-stimulated spleen cells from nude mice. We found that rIL 2 induced a dose-dependent increase of IgG2a secretion and a concomitant inhibition of the secretion of other Ig isotypes. The analysis of the phenotype of LPS- and LPS+ rIL 2-stimulated nude spleen cells showed the appearance of a Thy-1+ asialo GM-1+slgM-CD3-CD4-CD8- cell population in the presence of rIL 2. A population with a similar phenotype was generated upon stimulation of spleen cells from nude mice with rIL 2 alone. These cells lysed YAC-1 cells, did not contain the alpha or gamma transcripts encoding the corresponding T cell receptor chains and are therefore NK cells activated by rIL 2. In co-culture experiments, these cells selectively increased the secretion of IgG2a by LPS-stimulated splenocytes from nude mice. The IgG2a induction triggered by rIL 2-activated NK cells, as well as that triggered by rIL 2, were blocked by an anti-interferon gamma monoclonal antibody. Thus, rIL 2 activated-NK cells enhance the production of IgG2a by secreting interferon-gamma.

Published

1990

259. Regulatory effects of IgG-BF on hybridoma B cells. molecular characterization of variant cell lines.

Author

Brunati S, Miossec C, Mathiot C, Moncuit J, Amigorena S, Teillaud JL, and Fridman WH

Subjects

Animals, Antigens, Differentiation analysis, B-Lymphocytes cytology, Blotting, Northern, Blotting, Western, Cell Division, Cell Line, Electrophoresis, Polyacrylamide Gel, Immunoglobulin G biosynthesis, Mice, Receptors, Fc analysis, Receptors, IgG, B-Lymphocytes immunology, Hybridomas immunology, Lymphokines pharmacology, Prostatic Secretory Proteins

Abstract

Immunoglobulin G-binding factors (IgG-BF) produced by mouse T cells or hybridoma T cells (T2D4) were used to manipulate in vitro mouse hybridoma B cells. Both IgG production by, and proliferation of, these cells was inhibited by IgG-BF, or during co-cultures with IgG-BF-producing T2D4 cells. Thus, treatment of tumor B cells, besides its potential therapeutic use, represents an invaluable model for studying the regulation of Ig production by IgG-BF at a molecular level. To further analyze the molecular events induced by IgG-BF in B cell hybridomas, a set of variant clones of a hybridoma cell line (UN2) was isolated and variants were characterized for their Ig production and their Fc gamma R expression.

Published

1988

260. Software for the quantitative evaluation of in vitro monoclonal antibody production from ELISA data.

Author

Thibaut E, Amigorena S, Moncuit J, Fridman WH, and Teillaud JL

Subjects

Lymphokines biosynthesis, Antibodies, Monoclonal biosynthesis, Enzyme-Linked Immunosorbent Assay methods, Immunoglobulins analysis, Prostatic Secretory Proteins, Software

Abstract

Software has been developed which permits the quantitation of monoclonal antibodies secreted by B cell hybridomas. This program does not require the user to enter a large number of complex parameters and can be easily used without any previous computer experience. It fits all the experimental and standard curves by determining overlapping linear domains using the linear least-squares method. The program is based on logarithmic interpolations for determining Ig concentrations comparing experimental samples to Ig concentrations in standards. It provides a complete print-out of the data with editing options and is written in BASIC EDEX 4.0 Commodore computer language. It permits the accurate quantification of minute amounts of monoclonal antibodies and can be used to detect the inhibitory or enhancing effects of lymphokines or cytokines on Ig secretion by hybridoma B cells.

Published

1987

261. Fc gamma RII expression in resting and activated B lymphocytes.

Author

Amigorena S, Bonnerot C, Choquet D, Fridman WH, and Teillaud JL

Subjects

Animals, Blotting, Northern, Cell Cycle, Cell Line, Endonucleases, Interleukin-4, Interleukins pharmacology, Lipopolysaccharides pharmacology, Mice, RNA, Messenger genetics, Receptors, Antigen, B-Cell physiology, Receptors, IgG, Single-Strand Specific DNA and RNA Endonucleases, Time Factors, Antigens, Differentiation metabolism, B-Lymphocytes immunology, Lymphocyte Activation, Receptors, Fc metabolism

Abstract

In this report, we analyze the expression of the type II receptor for the Fc region of IgG (Fc gamma RII) in resting and lipopolysaccharide (LPS)-activated murine B lymphocytes. Fc gamma RII is encoded by two genes, alpha and beta. The beta gene encodes two mRNA, beta 1 and beta 2, which are generated by alternative splicing. Using an S1 nuclease protection assay, we found that resting and activated B lymphocytes express predominantly the beta 1 transcript. Very low levels of the beta 2 mRNA were detected in this assay, while no expression of the alpha transcript could be detected. Quantitative Northern blot analysis showed that the amount of Fc gamma RII beta mRNA was increased 9-fold in LPS-activated B lymphocytes. The expression of Fc gamma RII during the various phases of B cell activation was then studied by immunofluorescence using the monoclonal antibody 2.4G2. LPS stimulation induced an increase of the Fc gamma RII cellular pool as well as of its expression at the surface of B lymphocytes. The rise in Fc gamma RII surface expression occurred after the induction of class II antigens (Ia) and before transferrin receptor induction. Fc gamma RII expression was found to be enhanced during the G1 phase of the cell cycle since (a) only large cells (i.e. those that had entered the G1 phase) expressed an increased amount of Fc gamma RII and (b) blocking the entry of activated cells into the S phase (with the ion channel blocker quinine) did not affect the Fc gamma RII induction by LPS. Furthermore, only B cell activators that induced cells to enter into G1 [LPS and F(ab')2 anti-IgM antibodies, but not interleukin 4] caused an increase in the expression of Fc gamma RII. These results show that the increase in the membrane expression of Fc gamma RII occurs during the early G1 phase, establishing it as a marker for the entry of B lymphocytes into the cell cycle.

Published

1989

262. Control of B cell function by Fc gamma receptor-positive T cells and immunoglobulin-binding factors.

Author

Teillaud JL, Brunati S, Amigorena S, Mathiot C, Sautes C, and Fridman WH

Subjects

Animals, Antigens, Surface, B-Lymphocytes immunology, Cell Line, Humans, Immunoglobulin G biosynthesis, Receptors, IgG, Antigens, Differentiation metabolism, B-Lymphocytes metabolism, Lymphokines metabolism, Prostatic Secretory Proteins, Receptors, Fc metabolism, T-Lymphocytes metabolism

Published

1989

263. Bases for an isotypic network.

Author

Fridman WH, Daëron M, Amigorena S, Rabourdin-Combe C, and Neauport-Sautes C

Subjects

Immunoglobulin Idiotypes immunology, Receptors, Fc analysis, Receptors, Fc immunology, Immunoglobulin Isotypes immunology

Published

1986

264. Molecular heterogeneity of murine IgG-BF.

Author

Neauport-Sautes C, Blank U, Daëron M, Galinha A, Teillaud JL, Moncuit J, Amigorena S, and Fridman WH

Subjects

Animals, Chemical Phenomena, Chemistry, Chromatography, Affinity, Chromatography, Gel, Electrophoresis, Polyacrylamide Gel, Epitopes analysis, Immune Tolerance, Mice, Molecular Weight, Receptors, Fc immunology, Receptors, IgG, T-Lymphocytes immunology, Lymphokines immunology, Prostatic Secretory Proteins

Published

1986

265. The isotypic circuit: immunoglobulins, Fc receptors and immunoglobulin binding factors.

Author

Fridman WH, Teillaud JL, Amigorena S, Daëron M, Blank U, and Néauport-Sautès C

Subjects

Animals, B-Lymphocytes immunology, Mice, Models, Biological, T-Lymphocytes immunology, Immunoglobulin Isotypes biosynthesis, Lymphokines immunology, Prostatic Secretory Proteins, Receptors, Fc biosynthesis

Published

1987

266. Regulation of hybridoma B-cell proliferation by immunoglobulin-binding factor.

Author

Teillaud JL, Mathiot C, Amigorena S, Brunati S, Moncuit J, and Fridman WH

Subjects

Animals, B-Lymphocytes cytology, B-Lymphocytes immunology, Cell Division drug effects, Culture Media, Immunoglobulin G immunology, Isoelectric Point, Mice, Multiple Myeloma immunology, Necrosis, B-Lymphocytes drug effects, Hybridomas immunology, Lymphokines pharmacology, Prostatic Secretory Proteins

Abstract

Immunoglobulin-binding factors (IBF), which are cytokines able to suppress the immunoglobulin production by normal and transformed B cells, have been tested for their ability to interfere with hybridoma B-cell growth. Coculture experiments performed in soft agar between hybridoma B cells and hybridoma T cells secreting IgG-BF indicated that IgG-BF act as a growth regulatory molecule able to inhibit strongly the development of hybridoma B-cell colonies; this cytostatic effect, which appeared not to be a direct cytotoxic effect, was confirmed when using semi-purified IgG-BF in both soft agar and liquid medium cultures of hybridoma B cells. Thus, IBF appear to act as both immunoregulatory and growth regulatory factors. Some of the molecular consequences of this dual effect and its possible role in certain B-cell lymphoproliferative diseases such as multiple myeloma are discussed.

Published

1988

267. A sensitive method for testing the effect of immunoglobulin binding factor on Ig secretion by hybridoma B cells.

Author

Amigorena S, Moncuit J, Fridman WH, and Teillaud JL

Subjects

Animals, B-Lymphocytes drug effects, Cell Line, Enzyme-Linked Immunosorbent Assay, Hemolytic Plaque Technique, Hybridomas drug effects, Mice, T-Lymphocytes immunology, B-Lymphocytes immunology, Hybridomas immunology, Immunoglobulins immunology, Lymphokines pharmacology, Prostatic Secretory Proteins, Suppressor Factors, Immunologic pharmacology

Abstract

A microtiter plate assay to detect the effect of immunoglobulin binding factor (IBF) on Ig secretion by hybridoma B cells is described. This technique permits the analysis of Ig secretion by only 200-400 hybridoma B cells using a PFC assay and an ELISA, and therefore increases the IBF/cell number ratio. This increase allows the detection of a strong IBF-mediated inhibitory effect on Ig secretion by hybridoma B cells, which is otherwise difficult to obtain reproducibly. The technique is simple, does not require any transferring step and is convenient, since it permits large numbers of samples to be tested. It can be extended to test IBF for all isotypes or other lymphokines that affect Ig secretion.

Published

1987