Your search keyword '"Mark R. Alderson"' showing total 4 results

1. gld/gld mice are unable to express a functional ligand for Fas

Author

Robert E. Miller, Michael S. Seaman, Fred Ramsdell, David H. Lynch, Teresa W. Tough, and Mark R. Alderson

Subjects

Cytotoxicity, Immunologic, Programmed cell death, T cell, Immunology, Ligands, medicine.disease_cause, Autoimmune Diseases, Mice, Antigen, T-Lymphocyte Subsets, medicine, Animals, Immunology and Allergy, fas Receptor, Mice, Inbred C3H, Mutation, biology, T lymphocyte, Fas receptor, Molecular biology, Fusion protein, Lymphoproliferative Disorders, medicine.anatomical_structure, Mice, Inbred DBA, Antigens, Surface, biology.protein, Lymph Nodes, Antibody

Abstract

Mice homozygous for either the lpr or gld genes develop phenotypically identical autoimmune disorders. The gene responsible for the pathology in lpr/lpr mice encodes the Fas antigen, a protein associated with the induction of programmed cell death. To determine if the defect associated with gld represents a mutation in the ligand for Fas, we have assessed the ability of lymphoid cells from homozygous gld/gld mice to lyse target cells in a Fas-dependent manner. Using an antagonistic antibody to Fas, we demonstrate that activated T cells from normal and lpr mice are capable of inducing Fas-mediated lysis of tumor target cells. In contrast, activated T cells from gld/gld mice fail to induce lysis of tumor targets, although cells from gld mice are able to lyse specific allogeneic targets following mixed lymphocyte culture. In addition, activated T cells from gld/gld homozygous animals are not capable of binding to a Fas.Fc fusion protein at high levels, whereas activated T cells from normal and lpr/lpr animals bind Fas.Fc efficiently. These data indicate that mice homozygous for gld are unable to express a functional ligand for Fas.

Published

1994

2. Molecular and biological characterization of human 4-1BB and its ligand

Author

Raymond G. Goodwin, Elizabeth A. Baker, Craig A. Smith, Terri Davis-Smith, Wenie S. Din, Ben A. Falk, Grant R. Sutherland, Mark R. Alderson, Teresa W. Tough, Richard J. Armitage, and Eileen R. Roux

Subjects

Male, DNA, Complementary, medicine.drug_class, T cell, Immunology, Molecular Sequence Data, Clone (cell biology), Receptors, Nerve Growth Factor, Biology, Monoclonal antibody, Lymphocyte Activation, Transfection, Binding, Competitive, Receptors, Tumor Necrosis Factor, chemistry.chemical_compound, Mice, Tumor Necrosis Factor Receptor Superfamily, Member 9, Antigens, CD, Complementary DNA, medicine, Immunology and Allergy, Animals, Humans, Amino Acid Sequence, RNA, Messenger, Cells, Cultured, Genomic Library, Mice, Inbred BALB C, Membrane Glycoproteins, Base Sequence, Cell Death, T-cell receptor, Antibodies, Monoclonal, Chromosome Mapping, Flow Cytometry, Molecular biology, Fusion protein, 4-1BB ligand, medicine.anatomical_structure, chemistry, Expression cloning

Abstract

4-1BB was originally described as a cDNA expressed by activated murine T cells and subsequently demonstrated to encode a member of the tumor necrosis factor receptor family of integral membrane proteins. Recently, we identified and cloned a murine ligand for 4-1BB (mu4-1BB-L) and demonstrated it to be a member of an emerging family of ligands with structural homology to tumor necrosis factor. To characterize further the role of 4-1BB in the immune response we undertook to clone the human homologue of 4-1BB-L. However, attempts to isolate a cDNA encoding the human 4-1BB-L by cross-hybridization with the murine cDNA were unsuccessful. Therefore we first utilized cross-species hybridization to isolate a cDNA encoding human 4-1BB (hu4-1BB). A fusion protein consisting of the extracellular portion of hu4-1BB coupled to the Fc region of human immunoglobulin G1 (hu4-1BB.Fc) was then used to identify and clone a gene for human 4-1BB-L from an activated CD4+ T cell clone using a direct expression cloning strategy. Human 4-1BB-L shows 36% amino acid identity with its murine counterpart and maps to chromosome 19p13.3. Scatchard analysis demonstrated high-affinity binding of hu4-1BB.Fc to either native or recombinant human 4-1BB-L. Both monoclonal antibody to hu4-1BB and cells transfected with hu4-1BB-L induced a strong proliferative response in mitogen co-stimulated primary T cells. In contrast, ligation of 4-1BB on T cell clones enhanced activation-induced cell death when triggered by engagement of the TCR/CD3 complex.

Published

1994

3. CD40 ligand is a T cell growth factor

Author

William C. Fanslow, Mark R. Alderson, Fred Ramsdell, Melanie K. Spriggs, Teresa W. Tough, Richard J. Armitage, and Brian M. Macduff

Subjects

CD3 Complex, T cell, T-Lymphocytes, Immunology, CD40 Ligand, chemical and pharmacologic phenomena, Biology, Ligands, Lymphocyte Activation, Interleukin 21, Antigens, CD, medicine, Immunology and Allergy, Cytotoxic T cell, Humans, IL-2 receptor, CD40 Antigens, Antigen-presenting cell, Cells, Cultured, Interleukin 3, Membrane Glycoproteins, Antibodies, Monoclonal, hemic and immune systems, Natural killer T cell, Cell biology, Antigens, Differentiation, B-Lymphocyte, medicine.anatomical_structure, Interleukin 12, Interleukin-2

Abstract

CD40 ligand (CD40L) is a 33-kDa type II membrane glycoprotein induced on T cells upon activation. CD40L has previously been shown to induce proliferation of resting B cells, immunoglobulin (Ig) secretion from B cells cultured with cytokines and cytokine secretion and tumoricidal activity from monocytes. In this report CD40L is shown to be stimulatory for human T cells, inducing CD25 (p55 IL-2R) and CD40L expression on resting peripheral blood T cells, enhanced expression of these molecules and CD69 on CD3-activated cells and secretion of interferon-gamma, tumor necrosis factor-alpha and interleukin (IL)-2 from T cells cultured in the presence of a sub-mitogenic concentration of phytohemagglutinin A (PHA). Furthermore, stimulation with CD40L induces proliferation of CD3- or PHA-activated T cells of blood, tonsillar or thymic origin. A similar proliferative response is observed with CD4+ and CD8+ T cells and this effect is largely IL-2 independent. A soluble construct of the extracellular domain of the CD40L has similar activity to that of membrane-expressed ligand in the induction of T cell surface antigens and proliferation. The results presented here taken together with the various activities ascribed for CD40L on B cells and monocytes demonstrate that CD40L has pleiotropic biological activity for cells of the hemopoietic lineage.

Published

1993

4. Molecular characterization of the early activation antigen CD69: a type II membrane glycoprotein related to a family of natural killer cell activation antigens

Author

Ethan M. Shevach, Mark R. Alderson, Kathryn B. Hennen, Kenneth H. Grabstein, Richard J. Armitage, Fred Ramsdell, Steven F. Ziegler, Terry Farrah, Kathryn A. Hjerrild, and William C. Fanslow

Subjects

Antigens, Differentiation, T-Lymphocyte, CD4-Positive T-Lymphocytes, Immunology, Molecular Sequence Data, Early Activation Antigen CD69, CD1, chemical and pharmacologic phenomena, Biology, Lymphocyte Activation, Natural killer cell, Interleukin 21, Mice, Antigens, CD, medicine, Immunology and Allergy, Animals, Humans, Lectins, C-Type, Amino Acid Sequence, Cloning, Molecular, Membrane Glycoproteins, Base Sequence, ZAP70, DNA, Natural killer T cell, Molecular biology, Killer Cells, Natural, medicine.anatomical_structure, Interleukin 12, Natural killer cell activation, Sequence Alignment

Abstract

CD69 is a disulfide-linked homo-dimer expressed on the surface of activated T cells, B cells, natural killer cells, neutrophils and platelets. Antibody crosslinking of CD69 in the presence of phorbol ester results in cellular activation events including proliferation and the induction of specific genes. Using an expression cloning strategy we have isolated cDNA encoding human CD69 from a CD4+ T cell clone. Transfection of the cDNA clone in CV-1/EBNA cells results in the expression of a covalently linked homodimer. The cDNA insert hybridizes to a 1.7-kb mRNA in phorbol 12-myristate 13-acetate- or phytohemoagglutinin-stimulated human T cells. Using the human clone we have isolated cDNA encoding mouse CD69, which, when expressed in human T cells allowed those cells to respond to anti-mouse CD69 antibodies by secreting interleukin-2 and interferon-gamma. Sequence analysis showed that both mouse and human CD69 are type II membrane glycoproteins related to the NKR-P1 and Ly-49 families of natural killer cell activation molecules.

Published

1993