ABSTRACT
CD47, a broadly expressed cell surface protein, inhibits cell phagocytosis via interaction with phagocyte-expressed SIRPα. A variety of hematological malignancies demonstrate elevated CD47 expression, suggesting that CD47 may mediate immune escape. We discovered three unique CD47-SIRPα blocking anti-CD47 monoclonal antibodies (mAbs) with low nano-molar affinity to human and cynomolgus monkey CD47, and no hemagglutination and platelet aggregation activity. To characterize the anti-cancer activity elicited by blocking CD47, the mAbs were cloned into effector function silent and competent Fc backbones. Effector function competent mAbs demonstrated potent activity in vitro and in vivo, while effector function silent mAbs demonstrated minimal activity, indicating that blocking CD47 only leads to a therapeutic effect in the presence of Fc effector function. A non-human primate study revealed that the effector function competent mAb IgG1 C47B222-(CHO) decreased red blood cells (RBC), hematocrit and hemoglobin by >40% at 1 mg/kg, whereas the effector function silent mAb IgG2σ C47B222-(CHO) had minimal impact on RBC indices at 1 and 10 mg/kg. Taken together, our findings suggest that targeting CD47 is an attractive therapeutic anti-cancer approach. However, the anti-cancer activity observed with anti-CD47 mAbs is Fc effector dependent as are the side effects observed on RBC indices.
Subject(s)
CD47 Antigen/genetics , Leukemia/drug therapy , Amino Acid Sequence , Animals , Antibodies, Monoclonal , Female , Humans , Leukemia/genetics , Mice , Mice, Inbred NODABSTRACT
The structures of the ligand-binding domains (LBD) of the wild-type androgen receptor (AR) and the T877A mutant corresponding to that in LNCaP cells, both bound to dihydrotestosterone, have been refined at 2.0 A resolution. In contrast to the homodimer seen in the retinoid-X receptor and estrogen receptor LBD structures, the AR LBD is monomeric, possibly because of the extended C terminus of AR, which lies in a groove at the dimerization interface. Binding of the natural ligand dihydrotestosterone by the mutant LBD involves interactions with the same residues as in the wild-type receptor, with the exception of the side chain of threonine 877, which is an alanine residue in the mutant. This structural difference in the binding pocket can explain the ability of the mutant AR found in LNCaP cells (T877A) to accommodate progesterone and other ligands that the wild-type receptor cannot.
Subject(s)
Dihydrotestosterone/metabolism , Mutation/genetics , Receptors, Androgen/chemistry , Receptors, Androgen/metabolism , Amino Acid Sequence , Amino Acid Substitution/genetics , Androgens , Animals , Binding Sites , Crystallography, X-Ray , Dihydrotestosterone/chemistry , Dihydrotestosterone/pharmacology , Dimerization , Humans , Ligands , Male , Models, Molecular , Molecular Sequence Data , Progesterone/chemistry , Progesterone/metabolism , Prostatic Neoplasms/genetics , Protein Structure, Tertiary , Rats , Receptors, Androgen/genetics , Receptors, Progesterone/chemistry , Receptors, Progesterone/metabolism , Sequence Alignment , Substrate Specificity , Threonine/genetics , Threonine/metabolism , Tumor Cells, CulturedABSTRACT
The transcription factor NF-kappaB is sequestered in the cytoplasm by the inhibitor proteins of the IkappaB family. Each member of the IkappaB exhibits structural and biochemical similarities as well as differences. In an effort to address the functional redundancy of two closely related IkappaB molecules, IkappaBalpha and IkappaBbeta, we generated knock-in mice by replacing the IkappaBalpha gene with the IkappaBbeta gene. The knock-in mice do not express IkappaBalpha, but express a T7-tagged IkappaBbeta under the promoter and regulatory sequence of ikba. Unlike the IkappaBalpha-deficient mice, which display severe postnatal developmental defects and die by postnatal day 8, homozygous knock-in mice survive to adulthood, are fertile, and exhibit no apparent abnormalities. Furthermore, thymocytes and embryonic fibroblasts from the knock-in animals exhibit an inducible NF-kappaB response similar to that of wild-type animals. These results indicate that IkappaBalpha and IkappaBbeta share significant similarities in their biochemical activity, and that they acquired their different functions from divergent expression patterns during evolution.
Subject(s)
DNA-Binding Proteins/physiology , I-kappa B Proteins , NF-kappa B/antagonists & inhibitors , Animals , DNA-Binding Proteins/biosynthesis , DNA-Binding Proteins/genetics , Embryo, Mammalian , Female , Fibroblasts/immunology , Fibroblasts/metabolism , Genetic Vectors/chemical synthesis , Genetic Vectors/immunology , Male , Mice , Mice, Inbred ICR , Mice, Knockout , Mice, Transgenic , NF-KappaB Inhibitor alpha , NF-kappa B/genetics , NF-kappa B/physiology , Recombination, Genetic/immunology , Sequence Deletion/immunology , Signal Transduction/genetics , Signal Transduction/immunology , Thymus Gland/immunology , Thymus Gland/metabolism , Thymus Gland/pathologyABSTRACT
The transcription factor NF-kappaB is normally sequestered in the cytoplasm by members of the IkappaB family, including IkappaB alpha, IkappaB beta, and the recently cloned IkappaB epsilon. Upon cellular activation, these inhibitors are rapidly phosphorylated on two amino-terminal serines, ubiquitinated, and degraded by the 26S proteasome, releasing a functional NF-kappaB. To determine the importance of IkappaB beta in NF-kappaB regulation in T cells, we generated transgenic mice expressing a constitutively active IkappaB beta mutant (mIkappaB beta) under the control of the lck promoter. The transgene contains the two critical N-terminal serine residues mutated to alanines and therefore no longer susceptible to degradation upon cell activation. mIkappaB beta is unable to totally displace IkappaB alpha from RelA-containing complexes, thus allowing a transient activation of NF-kappaB upon T-cell stimulation. However, mIkappaB beta completely blocks NF-kappaB activity after IkappaB alpha degradation. In addition, as a consequence of this inhibition, ikba expression is down regulated, along with that of other NF-kappaB-regulated genes. These transgenic mice have a significant reduction in the peripheral T-cell population, especially CD8+ cells. The remaining T cells have impaired proliferation in response to phorbol 12-myristate 13-acetate plus phytohemagglutinin or calcium ionophore but not to anti-CD3/anti-CD28 costimulation. As a result of these alterations, transgenic animals present defects in immune responses such as delayed-type hypersensitivity and the generation of specific antibodies against T-cell-dependent antigens. These results show that in nonstimulated T cells, IkappaB beta cannot efficiently displace IkappaB alpha bound to RelA-containing complexes and that persistent NF-kappaB activity is required for proper T-cell responses in vivo.
Subject(s)
DNA-Binding Proteins/immunology , Gene Expression Regulation/immunology , I-kappa B Proteins , NF-kappa B/immunology , T-Lymphocytes/immunology , Animals , DNA-Binding Proteins/genetics , Gene Transfer Techniques , Lymphocyte Activation/genetics , Mice , Mice, Transgenic , Mutation , NF-kappa B/geneticsABSTRACT
The generation of animal models in which individual members of a gene family are genetically altered is a particularly attractive way to elucidate their function-Members of the Rel/NF-kappa B/I kappa B family constitute an important network of transcription factors and regulatory proteins that control the expression of numerous cellular and viral genes crucial for a variety of processes. A few examples are developmental pattern formation and immune response in Drosophila, viral replication, and immune, inflammatory, acute phase and stress responses in vertebrates. The findings from knockout and transgenic mice developed to study Rel/NF-kappa B/I kappa B function in vivo are reviewed here. In general, these studies point to the essential role of these factors in the development and function of the vertebrate immune system.
Subject(s)
NF-kappa B/physiology , Proto-Oncogene Proteins/physiology , Transcription Factors , Animals , Mice , Mice, Knockout , Mice, Transgenic , NF-kappa B/genetics , Proto-Oncogene Proteins/genetics , Transcription Factor RelBABSTRACT
Induction of c-fos transcription by serum growth factors requires the serum response element (SRE). The SRE is a multifunctional element which responds to several positively and negatively acting signals. To identify cellular proteins that might mediate functions of the SRE, we screened a human cDNA expression library with an SRE probe. We report the isolation and characterization of SRE-ZBP, a previously unidentified SRE-binding protein. SRE-ZBP is a member of the C2H2 zinc finger family of proteins exemplified by TFIIIA and the Drosophila Krüppel protein. The seven tandemly repeated zinc finger motifs in SRE-ZBP are sufficient for high-affinity binding to the SRE. We show that SRE-ZBP is a nuclear protein and identify a candidate cellular protein encoded by the SRE-ZBP gene. Because we cannot detect any DNA-binding activity attributable to the endogenous protein, we propose that SRE-ZBP activity may be subject to posttranslational regulation. Like c-fos mRNA, SRE-ZBP mRNA is serum inducible in HeLa cells, but with slower kinetics. The role of SRE-ZBP in the regulation of c-fos transcription remains unestablished, but this protein binds to a region of the SRE where mutations lead to derepression.
Subject(s)
DNA-Binding Proteins/metabolism , Genes, fos , Nuclear Proteins/metabolism , Transcription Factors/metabolism , Zinc Fingers/genetics , Amino Acid Sequence , Animals , Base Sequence , Cloning, Molecular/methods , DNA/genetics , DNA/isolation & purification , DNA Probes , Escherichia coli/genetics , Fluorescent Antibody Technique , Gene Library , Humans , Immune Sera , Molecular Sequence Data , Oligodeoxyribonucleotides , Plasmids , Recombinant Fusion Proteins/metabolism , Sequence Homology, Nucleic Acid , Serum Response Factor , Substrate Specificity , Transfection , Zinc Fingers/physiology , beta-Galactosidase/genetics , beta-Galactosidase/metabolismSubject(s)
Cytochrome P-450 Enzyme System/genetics , Genes, Fungal , Neurospora crassa/genetics , Neurospora/genetics , Amino Acid Sequence , Base Sequence , Cycloheximide/pharmacology , Gene Expression Regulation, Fungal/drug effects , Molecular Sequence Data , Multigene Family , Sequence Homology, Nucleic AcidABSTRACT
The presence of insulin binding sites in a clonal line of cells from rat pituitary tumor (GH1 cells) is described. The binding of insulin was a reversible and specific process. Binding of 125I-insulin to GH1 cells was inhibited by unlabeled insulin and to a minor extent, by proinsulin and desalanine insulin in direct proportion to their biological activities. Trypsin abolished the insulin binding to the cells. Twelve hours incubation of cells with insulin (5 microM) reduced in a 45% of the number of binding sites for the hormone. 125I-insulin bound to GH1 cells dissociated with a t 1/2 of 8 min. At 24 C labeled insulin was degraded by GH1 cells. No degradation was detected at 6 C. Unlabeled insulin inhibited most of the degradation of 125I-insulin, suggesting that degradation resulted from a saturable process. At steady-state, radioactive degradation products as well as 125I-insulin were recovered from GH1 cells.
Subject(s)
Binding, Competitive , Pituitary Neoplasms/metabolism , Receptor, Insulin/biosynthesis , Animals , Binding Sites , Cell Count , Cells, Cultured , Chromatography, Gel , Insulin/metabolism , Iodine Radioisotopes/metabolism , RatsSubject(s)
Animals , Rats , Cells, Cultured , Binding, Competitive , Pituitary Neoplasms , Receptor, InsulinABSTRACT
The presence of insulin binding sites in a clonal line of cells from rat pituitary tumor (GH1 cells) is described. The binding of insulin was a reversible and specific process. Binding of 125I-insulin to GH1 cells was inhibited by unlabeled insulin and to a minor extent, by proinsulin and desalanine insulin in direct proportion to their biological activities. Trypsin abolished the insulin binding to the cells. Twelve hours incubation of cells with insulin (5 microM) reduced in a 45
of the number of binding sites for the hormone. 125I-insulin bound to GH1 cells dissociated with a t 1/2 of 8 min. At 24 C labeled insulin was degraded by GH1 cells. No degradation was detected at 6 C. Unlabeled insulin inhibited most of the degradation of 125I-insulin, suggesting that degradation resulted from a saturable process. At steady-state, radioactive degradation products as well as 125I-insulin were recovered from GH1 cells.
