Your search keyword '"Panousis C"' showing total 4 results

1. rIgG1 Fc Hexamer Inhibits Antibody-Mediated Autoimmune Disease via Effects on Complement and FcγRs.

Author

Spirig R, Campbell IK, Koernig S, Chen CG, Lewis BJB, Butcher R, Muir I, Taylor S, Chia J, Leong D, Simmonds J, Scotney P, Schmidt P, Fabri L, Hofmann A, Jordi M, Spycher MO, Cattepoel S, Brasseit J, Panousis C, Rowe T, Branch DR, Baz Morelli A, Käsermann F, and Zuercher AW

Subjects

Animals, Antibody-Dependent Cell Cytotoxicity immunology, Cell Line, Complement Activation immunology, Humans, Inflammation immunology, Male, Mice, Mice, Inbred BALB C, Phagocytosis immunology, Receptors, IgG immunology, Antibodies, Monoclonal immunology, Antigen-Antibody Complex immunology, Autoimmune Diseases immunology, Complement System Proteins immunology, Immunoglobulin Fc Fragments immunology, Immunoglobulin G immunology, Receptors, Fc immunology

Abstract

Activation of Fc receptors and complement by immune complexes is a common important pathogenic trigger in many autoimmune diseases and so blockade of these innate immune pathways may be an attractive target for treatment of immune complex-mediated pathomechanisms. High-dose IVIG is used to treat autoimmune and inflammatory diseases, and several studies demonstrate that the therapeutic effects of IVIG can be recapitulated with the Fc portion. Further, recent data indicate that recombinant multimerized Fc molecules exhibit potent anti-inflammatory properties. In this study, we investigated the biochemical and biological properties of an rFc hexamer (termed Fc-μTP-L309C) generated by fusion of the IgM μ-tailpiece to the C terminus of human IgG1 Fc. Fc-μTP-L309C bound FcγRs with high avidity and inhibited FcγR-mediated effector functions (Ab-dependent cell-mediated cytotoxicity, phagocytosis, respiratory burst) in vitro. In addition, Fc-μTP-L309C prevented full activation of the classical complement pathway by blocking C2 cleavage, avoiding generation of inflammatory downstream products (C5a or sC5b-9). In vivo, Fc-μTP-L309C suppressed inflammatory arthritis in mice when given therapeutically at approximately a 10-fold lower dose than IVIG, which was associated with reduced inflammatory cytokine production and complement activation. Likewise, administration of Fc-μTP-L309C restored platelet counts in a mouse model of immune thrombocytopenia. Our data demonstrate a potent anti-inflammatory effect of Fc-μTP-L309C in vitro and in vivo, likely mediated by blockade of FcγRs and its unique inhibition of complement activation., (Copyright © 2018 by The American Association of Immunologists, Inc.)

Published

2018

2. High-Throughput IgG Reformatting and Expression.

Author

Chen CG, Sansome G, Wilson MJ, and Panousis C

Subjects

Animals, Cell Line, Humans, Recombinant Proteins biosynthesis, Recombinant Proteins genetics, Gene Expression, Gene Library, Immunoglobulin G biosynthesis, Immunoglobulin G genetics, Peptide Library, Single-Chain Antibodies biosynthesis, Single-Chain Antibodies genetics

Abstract

We have recently described a one-step zero-background IgG reformatting method that enables the rapid reformatting of phage-displayed antibody fragments into a single-mammalian cell expression vector for full IgG expression (Chen et al. Nucleic Acids Res 42:e26, 2014). The strategy utilizes our unique positive selection method, referred to as insert-tagged (InTag) positive selection, where a positive selection marker (e.g. chloramphenicol-resistance gene) is cloned together with the antibody inserts into the expression vector. The recombinant clones containing the InTag adaptor are then positively selected without cloning background, thus bypassing the need to plate out cultures and screen colonies. This IgG reformatting method is rapid and can be automated and performed in a high-throughput (HTP) format. The use of InTag positive selection with the Dyax Fab-on-phage antibody library is demonstrated. We have further optimized the protocol for IgG reformatting since the initial publication of this method (Chen et al. Nucleic Acids Res 42:e26, 2014) and also updated the transient transfection protocol using Expi293F cells, which are described herein.

Published

2018

3. One-step zero-background IgG reformatting of phage-displayed antibody fragments enabling rapid and high-throughput lead identification.

Author

Chen CG, Fabri LJ, Wilson MJ, and Panousis C

Subjects

Immunoglobulin Fragments genetics, Immunoglobulin G biosynthesis, Transfection, Cell Surface Display Techniques, Immunoglobulin G genetics

Abstract

We describe a novel cloning method, referred to as insert-tagged (InTag) positive selection, for the rapid one-step reformatting of phage-displayed antibody fragments to full-length immunoglobulin Gs (IgGs). InTag positive selection enables recombinant clones of interest to be directly selected without cloning background, bypassing the laborious process of plating out cultures and colony screening and enabling the cloning procedure to be automated and performed in a high-throughput format. This removes a significant bottleneck in the functional screening of phage-derived antibody candidates and enables a large number of clones to be directly reformatted into IgG without the intermediate step of Escherichia coli expression and testing of soluble antibody fragments. The use of InTag positive selection with the Dyax Fab-on-phage antibody library is demonstrated, and optimized methods for the small-scale transient expression of IgGs at high levels are described. InTag positive selection cloning has the potential for wide application in high-throughput DNA cloning involving multiple inserts, markedly improving the speed and quality of selections from protein libraries.

Published

2014

4. Targeted bioactivity of membrane-anchored TNF by an antibody-derived TNF fusion protein.

Author

Bauer S, Adrian N, Williamson B, Panousis C, Fadle N, Smerd J, Fettah I, Scott AM, Pfreundschuh M, and Renner C

Subjects

Animals, Antigens, Neoplasm metabolism, Biomarkers, Tumor metabolism, Cell Line, Cell Line, Tumor, Cytotoxicity, Immunologic genetics, Dimerization, Endopeptidases, Endothelium, Vascular cytology, Endothelium, Vascular metabolism, Gelatinases, Humans, Hydrogen Peroxide metabolism, Immunoglobulin G administration & dosage, Immunoglobulin G toxicity, Membrane Proteins genetics, Mice, Mice, Inbred BALB C, Neoplasm Transplantation, Neutrophils metabolism, Oxidation-Reduction, Protein Structure, Tertiary genetics, Recombinant Fusion Proteins administration & dosage, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins toxicity, Sequence Deletion, Serine Endopeptidases metabolism, Solubility, Thromboplastin biosynthesis, Tumor Necrosis Factor-alpha administration & dosage, Tumor Necrosis Factor-alpha toxicity, Xenograft Model Antitumor Assays, Antigens, Neoplasm immunology, Binding Sites, Antibody genetics, Biomarkers, Tumor immunology, Immunoglobulin G genetics, Immunoglobulin G metabolism, Membrane Proteins metabolism, Recombinant Fusion Proteins metabolism, Serine Endopeptidases immunology, Tumor Necrosis Factor-alpha genetics, Tumor Necrosis Factor-alpha metabolism

Abstract

We describe the generation and characterization of a fusion protein consisting of a humanized anti-fibroblast-activating protein (anti-FAP) Ab and human TNF replacing the IgG1 CH2/CH3 Fc domain. The construct was generated by recombinant DNA technology and preserved its IgG1-derived dimeric structure with the TNF molecule linked as a dimer. Expression in CHO cells was optimized in serum-free medium under GMP conditions to achieve production levels up to 15 mg/liter. Recognition of the FAP Ag by the construct was as good as that by the parental anti-FAP Ab. TNF signaling was induce able via both TNF receptor types. When acting in solution, the Ab-linked TNF dimer exhibited a 10- to 20-fold lower activity compared with recombinant trimeric TNF. However, after binding to FAP-expressing cells, immobilized anti-FAP-TNF dimer was equivalent to membrane-anchored TNF with regard to bioactivity. Amplification of TNF-related pathways by mimicking the membrane-integrated TNF signaling was detectable in various systems, such as apoptosis induction or tissue factor production. The difference in TNF receptor type 1 and 2 signaling by the anti-FAP-TNF construct correlated well with its Ag-bound or -soluble status. Translating the approach into a xenograft animal model (BALB/c nu/nu mice), we demonstrated low toxicity with measurable antitumor efficacy for the TNF fusion protein after i.v. application. Immunohistochemical analysis of tumor sections showed restricted TNF-mediated macrophage recruitment to the targeted tissue in a time- and dose-dependent manner. These data warrant transfer of the anti-FAP-TNF immunocytokine into clinical trials for the treatment of FAP-positive tumors.

Published

2004