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2. Rat class III Fc gamma receptor isoforms differ in IgG subclass-binding specificity and fail to associate productively with rat CD3 zeta

Author

D L Farber, R Giorda, M Y Nettleton, M Trucco, J P Kochan, and D W Sears

Subjects
Immunology, Immunology and Allergy
Abstract

Several new rat class III Fc gamma R isoforms are described here, extending the genetic complexity of this receptor family and further distinguishing rat CD16 from mouse CD16, represented by only one receptor isoform, and human CD16, represented by only two isoforms. RNase protection assays reveal that three rat tumor cell lines--RBL-1 basophilic leukemia cells, RM-SV1 macrophages, and CRNK-16 NK cells--all coordinately express multiple and probably identical rtFc gamma RIII-related transcripts in similar relative proportions but at significantly different levels. These results indicate that no single isoform predominates in these cell types but that the overall level of rtFc gamma RIII-related transcripts is differentially regulated. Two of the rtFc gamma RIII isoforms found to have extensive amino acid sequence differences in their second extracellular (EC2) domains are shown to bind rat and mouse IgG subclasses differently. This result suggests that the receptor isoform diversity in this species may function as a mechanism for extending the IgG-binding capacity of rat leukocytes. Cloned cDNA for the rat CD3 zeta protein was also isolated in this study and its ability to augment surface expression of class III Fc gamma R was tested by rosetting of cDNA-transfected COS cells. Like the structurally homologous mouse CD3 zeta, rat CD3 zeta fails to promote surface expression of Fc gamma RIII, sharply contrasting the efficient receptor expression produced by human CD3 zeta. Variations in the transmembrane amino acid sequences correlate with the divergent capacities of these CD3 zeta molecules to augment receptor expression. The high levels of CD3 zeta message expressed in rat NK cells may indicate that other unidentified hetero-subunits are required for assembly of rat CD3 zeta into functional CD16 receptors.

Published
1993
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3. Rat CD16 is defined by a family of class III Fc gamma receptors requiring co-expression of heteroprotein subunits

Author

D L Farber and D W Sears

Subjects
Immunology, Immunology and Allergy
Abstract

Rat CD16 is defined here by a family of highly homologous class III Fc gamma receptor isoforms. Northern blot and polymerase chain reaction analysis indicate that multiple rtFc gamma RIII alpha isoforms are expressed by rat NK and macrophages contrasting the expression of a single class III receptor isoform by human and mouse NK and macrophages. Analysis of genomic Southern blots and splice variants identified by polymerase chain reaction suggests the existence of several homologous rat Fc gamma RIII alpha genes organized similar to human and mouse class III receptor genes. All rat Fc gamma RIII alpha isoform protein sequences have conventional transmembrane insertion sequences containing the unique LFAVDTGL motif conserved in all other class III Fc gamma and Fc epsilon RI alpha receptor sequences. A model is proposed for the protein-protein interactions between this sequence and the transmembrane sequences of two heteroprotein subunits, Fc epsilon RI gamma and CD3 zeta, known to interact with human and mouse class III receptors. Rat NK, monocytes, and neutrophils were all found to express transcripts for both of these subunits, whereas rat macrophages express only Fc epsilon RI gamma subunit transcripts. Furthermore, the Fc epsilon RI gamma subunit was found to promote the cell surface expression of rtFc gamma RIII alpha isoforms in transfected COS cells.

Published
1991
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4. Rat CD16 is defined by a family of class III Fc gamma receptors requiring co-expression of heteroprotein subunits

Author

D L, Farber and D W, Sears

Subjects
Base Sequence, Transcription, Genetic, Macrophages, Molecular Sequence Data, Receptors, IgG, Rats, Inbred Strains, Receptors, Fc, Transfection, Antigens, Differentiation, Cell Line, Rats, Killer Cells, Natural, Animals, RNA
Abstract

Rat CD16 is defined here by a family of highly homologous class III Fc gamma receptor isoforms. Northern blot and polymerase chain reaction analysis indicate that multiple rtFc gamma RIII alpha isoforms are expressed by rat NK and macrophages contrasting the expression of a single class III receptor isoform by human and mouse NK and macrophages. Analysis of genomic Southern blots and splice variants identified by polymerase chain reaction suggests the existence of several homologous rat Fc gamma RIII alpha genes organized similar to human and mouse class III receptor genes. All rat Fc gamma RIII alpha isoform protein sequences have conventional transmembrane insertion sequences containing the unique LFAVDTGL motif conserved in all other class III Fc gamma and Fc epsilon RI alpha receptor sequences. A model is proposed for the protein-protein interactions between this sequence and the transmembrane sequences of two heteroprotein subunits, Fc epsilon RI gamma and CD3 zeta, known to interact with human and mouse class III receptors. Rat NK, monocytes, and neutrophils were all found to express transcripts for both of these subunits, whereas rat macrophages express only Fc epsilon RI gamma subunit transcripts. Furthermore, the Fc epsilon RI gamma subunit was found to promote the cell surface expression of rtFc gamma RIII alpha isoforms in transfected COS cells.

Published
1991

5. Molecular cloning and expression of the mouse high affinity Fc receptor for IgG

Author

D W, Sears, N, Osman, B, Tate, I F, McKenzie, and P M, Hogarth

Subjects
Base Sequence, Macrophages, Molecular Sequence Data, Receptors, IgG, DNA, Receptors, Fc, Blotting, Northern, Antigens, Differentiation, Blotting, Southern, Mice, Genes, Animals, Amino Acid Sequence, Cloning, Molecular, Oligonucleotide Probes
Abstract

Full length cDNA clones encoding the mouse Fc gamma RI were isolated by using redundant oligonucleotide probes based on previously determined amino acid sequence of protein bound to an IgG2a antibody column. Sequence analysis of cDNA clones indicates that mouse Fc gamma RI is a transmembrane glycoprotein that is composed of three disulfide bonded extracellular Ig binding domains unlike Fc gamma RII of man and mouse. These extracellular domains contain five potential sites of N-linked glycosylation; three sites in the first domain and one in each of the second and third domains. In addition a transmembrane region is present followed by a cytoplasmic tail of 84 amino acids. Analysis of the amino acid sequence of the first two extracellular domains of Fc gamma RI indicate that these are highly homologous to the extracellular domains of Fc gamma RII; the third domain is different and shows a lower level of homology to other FcR domains but is clearly related to the Ig super-family. Transfected cells expressing Fc gamma RI were shown to bind immune complexes of rabbit IgG; and monomeric IgG2a bound to transiently transfected cells with an affinity of approximately 5 x 10(7) M-1, i.e. the receptor was of high affinity and therefore was by definition Fc gamma RI. Northern analysis demonstrated that Fc gamma RI mRNA could be detected in the Fc gamma RI+ myeloid cell lines WEH1 3B and J774. Finally, Southern analysis indicated that Fc gamma RI is likely to be encoded by a single copy gene of approximately 9 kb.

Published
1990

7. Apparent sensitivity of human K lymphocytes to the spatial orientation and organization of target cell-bound antibodies as measured by the efficiency of antibody-dependent cellular cytotoxicity (ADCC)

Author

J E Christiaansen, S S Burnside, and D W Sears

Subjects
Immunology, Immunology and Allergy
Abstract

Although monoclonal antibodies (mAb) can elicit potent ADCC by human K lymphocytes, different mAb, even of the same antibody subclass or even of the same target antigen specificity, vary considerably as to their efficiency in eliciting ADCC. The extensive variability in ADCC efficiencies of murine IgG2a mAb is analyzed here. In cold-target inhibition experiments it was found that only cells coated with "ADCC-efficient" IgG2a mAb, and not "ADCC-inefficient" IgG2a mAb, inhibit K effector cell lysis of radiolabeled target cells by ADCC. This result indicates that the spatial orientation of the antibodies on the target cell membrane influences the net efficiency of ADCC reactions by affecting the efficiency of interaction between antibody and the Fc receptors (FcR) of K cells. It is proposed that a "favorable" orientation of antibodies on the target cell membrane is required for efficient ADCC reactions. This proposal is directly supported by the observation that one IgG2a mAb (20.8.4), which cross-reacts with several different H-2 alloantigens, was found to elicit efficient ADCC only when bound to certain of its possible target cell antigens. It was also observed in these studies that the organization of antibodies on a target cell membrane influences the net efficiency of ADCC reactions. It is proposed that a "favorable" antibody organization on the target cell membrane is also required for efficient ADCC reactions. This proposal is supported by the observation that certain antihuman beta 2m (anti-Hu beta 2m) IgG2a mAb, which elicit efficient ADCC lysis of human target cells, fail to elicit the lysis of murine cells having Hu beta 2m molecules coupled randomly to their external membrane surfaces. The differences in the way the Hu beta 2m was organized on the surfaces of the human cells and the murine-Hu beta 2m cell conjugates presumably caused differences in the way the bound antibodies were organized on the cell surfaces, which in turn resulted in the ADCC efficiency differences observed for the same mAb with the different target cell types. Because ADCC reactions appear to be sensitive to both the orientation and the organization of cell surface-bound antibodies, certain types of structural alterations or variations in the membrane molecules (relative to other neighboring structures on the target cell membrane) are potentially detectable by quantitative differences or variations in ADCC reactions.

Published
1987
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9. Acquisition of the covalent quaternary structure of an immunoglobulin G molecule. Reoxidative assembly in vitro

Author

Friedman F, Sherman Beychok, Kazin Ar, J Mohrer, and D W Sears

Subjects
Gel electrophoresis, biology, Protein Conformation, Chemistry, Stereochemistry, Alkylation, Biochemistry, Immunoglobulin G, Dithiothreitol, chemistry.chemical_compound, Covalent bond, biology.protein, Iodoacetamide, Humans, Molecule, Immunoglobulin Light Chains, Protein quaternary structure, Sulfhydryl Compounds, Immunoglobulin Heavy Chains, Oxidation-Reduction, Bence Jones Protein
Abstract

We recently reported results of an investigation of the reoxidation of a human, monoclonal immunoglobulin G, following selective reduction of its interchain disulfides by dithiothreitol (Sears, D.W., et al. (1975), Proc. Natl. Acad. Sci. U.S.A. 72, 353). In that work, we described the reoxidative behavior of the molecule under nondissociating conditions. In the present paper, results are presented of the reoxidation of heavy (H) and light (L) chains of this protein alone, or mixed in varying proportions after separation, or mixed with the L chains modified prior to recombination and reoxidation. The overall reoxidative asembly patterns in experiments with H and L separated prior to recombination are similar to those observed when the chains remain noncovalently associated throughout. With equimolar mixtures of H and L, the reoxidation rates also are similar to those of unseparated chains. However, when L chains are present in excess, the overall in vitro rates of covalent assembly are generally diminished, probably indicating transient nonproductive interactions. At the highest molar excesses of L (3:1), the assembly pathways may also be modified. In all experiments with excess L chains, covalent L2 dimers form at rates which are comparatively slow relative to the H2L2 assembly rates. Two kinds of reoxidation experiments with modified L chains are described here for the first time. In the first, the free half-cystine of L is irreversibly blocked by reaction with iodoacetamide, and the alkylated L chains are recombined with reduced H chains. This experiment isolates the reactions in which H2 disulfides are formed without the accompanying formation of HL bonds. Although the alkylated L chains do not play a direct role in the reoxidation, their presence is required to inhibit aggregation and precipitation of high-molecular-weight products which otherwise ensue; this suggests a possible biological role for excess L in vivo. In the second kind of experiment, covalent L2 dimers are mixed with reduced H chains. L2 rapidly disappears with the concurrent appearance of HL, H2L, and fully assembled H2L. H2 dimers are also reactive in this process. Special procedures were developed for analyzing the data from these experiments. A complete format is given for the quantitative determination of the concentration of each of the molecular components directly from spectroscopic scans of the gels. The computational methods solve the general analytical problem posed when staining is not proportional to mass and are applicable to a wide variety of systems utilizing gel electrophoresis to study subunit interactions. A theoretical analysis of pathway and kinetic cooperatively in this system is presented in the following paper (Sears, D.W., and Beychok, S. (1977), Biochemistry 16 (following paper in this issue)).

Published
1977
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11. Polymorphism of murine major histocompatibility Class I antigen: assignment of putative allodeterminants to distinct positions of the amino acid sequence within the first external domain of the antigen

Author

K Ozato, H Takahashi, E Appella, D W Sears, C Murre, J G Seidman, S Kimura, and N Tada

Subjects
Immunology, Immunology and Allergy
Abstract

Forty-five new monoclonal antibodies reacting with the mouse H-2Dd antigen have been established. The specificities of 34 of these antibodies were mapped into the first external domain (N) of the Dd antigen by testing reactivities with the products of mosaic H-2 genes in which the coding sequences of the first and/or the second external domains of the H-2Dd genes were recombined in vitro with the remaining portion of the H-2Ld gene. These antibodies reacted with at least 13 distinct allodeterminants located in the N domain, composed of 91 amino acids, as judged from panel tests carried out on various H-2 haplotypes. To assign possible positions of antigenic determinants of these and other anti-H-2Dd antibodies, we compared primary sequences of seven H-2 antigens and searched for correspondence between the pattern of amino acid substitutions in the N domain, allowing 15 positions to be assigned for the antigenic sites. These putative antigenic determinants were assessed for possible relationships with several parameters of protein secondary structure postulated according to predictive methods. Many of these sites appear to be associated with greatest local hydrophilicity, known to correlate with sites of antibody binding in various proteins. We therefore propose that some of the correspondences found in this work represent structural correlates of allodeterminants.

Published
1985
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12. Relative susceptibilities of the interchain disulfides of an immunoglobulin G molecule to reduction by dithiothreitol

Author

D W Sears, Sherman Beychok, and J Mohrer

Subjects
biology, Protein Conformation, Chemistry, Cooperativity, Biochemistry, Immunoglobulin kappa-Chains, Medicinal chemistry, Immunoglobulin G, Dithiothreitol, chemistry.chemical_compound, Protein structure, biology.protein, Humans, Organic chemistry, Molecule, Immunoglobulin Light Chains, Reactivity (chemistry), Disulfides, Immunoglobulin Heavy Chains, Oxidation-Reduction, Anaerobic exercise
Abstract

The reduction by dithiothreitol (DTT) of the four interchain disulfides of a human IgGlkappa immunoglobulin has been studied by two methods: variation of the concentration of DTT relative to the protein concentration (incremental reduction); and variation of the time of reduction at fixed levels of DTT and protein (kinetic reduction). In both cases, the results depend on whether the reduction is carried out aerobically or anaerobically. Under aerobic conditions, the relative levels of intermediates (HL, H2, and H2L) which are generated as native molecules (H2L2) are converted to reduced heavy (H) and light (L) chains depend on the concentrations of protein and DTT as well as on the exposure time to DTT; no stable equilibrium is reached between reduced and oxidized states and conditions gradually revert from those favoring reduction to those favoring reoxidation. By contrast, anaerobic reduction is independent of protein concentration or time of exposure to DTT, beyond about 30 min, indicating that an equilibrium between partially reduced and oxidized states is achieved. The distribution of intermediates observed under anaerobic conditions has been analyzed according to theoretical models (Sears, D.W., and Beychok, S. (1977), Biochemistry 16 (second in a series of three articles in this issue)). Within experimental error, both kinds of anaerobic experiments resemble a random reduction process wherein the four disulfides are equivalent and independent of each other with respect to rate and extent of reduction by D. It is concluded that there are no readily detected pathways in the process, as would occur if the intrinsic reactivities of the bonds were distinct, and no marked cooperatively between the four reaction sites, as would be observed if reduction of one bond materially facilitated or hampered reactivity at another site. Both of these characteristics of the reduction are in direct contrast to those of the reoxidative process, which is marked by the initial preference for formation of a bond between heavy and light chains, and by kinetic cooperativity in bond formation during the course of the reaction (Sears, D.W., et al. (1977), Biochemistry 16 (first in a series of three articles in this issue); Sears, D.W., and Beychok, S. (1977), Biochemistry 16 (second in this series)).

Published
1977
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13. Oil and Gas Developments in Alaska in 1981

Author

B. C. Jones and D. W. Sears

Subjects
Hydrology, business.industry, Fossil fuel, Energy Engineering and Power Technology, Drilling, Geology, Mineral resource classification, Well drilling, chemistry.chemical_compound, Fuel Technology, Lease, chemistry, Geochemistry and Petrology, Natural gas, Earth and Planetary Sciences (miscellaneous), Petroleum, business, Bay
Abstract

Twenty-three exploratory wells were drilled in Alaska in 1981. Ten oil or gas discovery wells were drilled on the North Slope. 154 development and service wells were drilled and completed in the Prudhoe Bay and Kuparuk River fields on the North Slope. Geologic and geophysical field activity increased significantly in 1981, mainly because of increased North Slope activity and for OCS sale preparation in the Bering Sea. Two OCS lease sales were held and the first NPR-A lease sale was held. The State of Alaska continued a series of scheduled state lease sales.

Published
1982
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16. Apparent sensitivity of human K lymphocytes to the spatial orientation and organization of target cell-bound antibodies as measured by the efficiency of antibody-dependent cellular cytotoxicity (ADCC)

Author

J E, Christiaansen, S S, Burnside, and D W, Sears

Subjects
Killer Cells, Natural, Structure-Activity Relationship, Immunoglobulin G, Cell Membrane, Antibody-Dependent Cell Cytotoxicity, Dose-Response Relationship, Immunologic, H-2 Antigens, Antibodies, Monoclonal, Humans, Receptors, Fc, beta 2-Microglobulin, Cells, Cultured
Abstract

Although monoclonal antibodies (mAb) can elicit potent ADCC by human K lymphocytes, different mAb, even of the same antibody subclass or even of the same target antigen specificity, vary considerably as to their efficiency in eliciting ADCC. The extensive variability in ADCC efficiencies of murine IgG2a mAb is analyzed here. In cold-target inhibition experiments it was found that only cells coated with "ADCC-efficient" IgG2a mAb, and not "ADCC-inefficient" IgG2a mAb, inhibit K effector cell lysis of radiolabeled target cells by ADCC. This result indicates that the spatial orientation of the antibodies on the target cell membrane influences the net efficiency of ADCC reactions by affecting the efficiency of interaction between antibody and the Fc receptors (FcR) of K cells. It is proposed that a "favorable" orientation of antibodies on the target cell membrane is required for efficient ADCC reactions. This proposal is directly supported by the observation that one IgG2a mAb (20.8.4), which cross-reacts with several different H-2 alloantigens, was found to elicit efficient ADCC only when bound to certain of its possible target cell antigens. It was also observed in these studies that the organization of antibodies on a target cell membrane influences the net efficiency of ADCC reactions. It is proposed that a "favorable" antibody organization on the target cell membrane is also required for efficient ADCC reactions. This proposal is supported by the observation that certain antihuman beta 2m (anti-Hu beta 2m) IgG2a mAb, which elicit efficient ADCC lysis of human target cells, fail to elicit the lysis of murine cells having Hu beta 2m molecules coupled randomly to their external membrane surfaces. The differences in the way the Hu beta 2m was organized on the surfaces of the human cells and the murine-Hu beta 2m cell conjugates presumably caused differences in the way the bound antibodies were organized on the cell surfaces, which in turn resulted in the ADCC efficiency differences observed for the same mAb with the different target cell types. Because ADCC reactions appear to be sensitive to both the orientation and the organization of cell surface-bound antibodies, certain types of structural alterations or variations in the membrane molecules (relative to other neighboring structures on the target cell membrane) are potentially detectable by quantitative differences or variations in ADCC reactions.

Published
1987

18. Feasibility of simulation of health maintenance organizations

Author

A T, Moustafa and D W, Sears

Subjects
Insurance, Health, Legislation, Medical, Longevity, Ownership, Politics, Health Maintenance Organizations, Models, Theoretical, United States, Economics, Medical, Health Planning, Life Expectancy, Socioeconomic Factors, Organization and Administration, Group Practice, Humans, Health Expenditures, Mortality, Delivery of Health Care, Minority Groups
Published
1974

19. Unusually efficient tumor cell lysis by human effectors of antibody-dependent cellular cytotoxicity mediated by monoclonal antibodies

Author

J E, Christiaansen and D W, Sears

Subjects
Adult, Killer Cells, Natural, Mice, Inbred C57BL, Kinetics, Mice, Lymphoma, Immune Sera, Immunoglobulin G, Antibody-Dependent Cell Cytotoxicity, Leukocytes, Animals, Antibodies, Monoclonal, Humans
Abstract

Concentrations ranging between 0.01 and 10 pg per cell of certain monoclonal antibodies (MAbs) are shown to constitute 4-hr 50% lethal doses for tumor cells mixed with human effectors of antibody-dependent cellular cytotoxicity (ADCC). This efficient and rapid tumor cell lysis is achieved at low effector cell levels (effector:target ratios, less than or equal to 25:1) at which the effectors are nonadherent peripheral blood leukocytes (PBL) enriched by density centrifugation. Comparable MAb-mediated ADCC efficiency has not been reported previously, probably because most MAbs (e.g., 10 of 13 tested in this study) are typically inefficient or completely inactive in mediating ADCC, even at 100-fold greater concentrations. By analyzing the ADCC efficiencies of several MAbs specific for murine cell surface alloantigens, it is shown that murine IgG2a and IgG3 MAbs and a rat IgG2b MAb are very efficient mediators of ADCC. However, ADCC efficiency was found not to correlate strictly with subclass, since 4 of 6 murine IgG2a MAbs tested were completely inactive, even though they all bound the target cells readily. It is shown that the relative differences in ADCC efficiencies are not accounted for directly by antibody affinity for antigen; one MAb was very efficient in ADCC but had demonstrably low antigen affinity, while a second MAb showed no ADCC activity in spite of its high affinity for the same target antigen. These results point to other experimentally testable properties of MAbs and of MAb-antigen complexes which may be critical for efficient ADCC reactions. This study underscores an important immunotherapeutic value which certain MAbs potentially have for mediating tumor cell lysis: in low concentrations (and without toxic drug modification), some MAbs efficiently mediate the lysis of tumors by ADCC, which itself is as effective as other immune lytic processes but which requires no prior immunological education of effector cells.

Published
1984

20. Alaska

Author

null B. C. Jones (1), D. W. Sears (1)

Subjects
Fuel Technology, Geochemistry and Petrology, Earth and Planetary Sciences (miscellaneous), Energy Engineering and Power Technology, Geology
Published
1981
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21. STUDIES ON THE CHEMICAL BASIS OF VARIABILITY AND THE COMPLEX CELLULAR EXPRESSION OF THE H-2K and H-2D PRODUCTS

Author

Bruce M. Ewenstein, J. H. Freed, T.V. Rajan, Matthew D. Scharff, Stanley G. Nathenson, D. W. Sears, L.E. Mole, and J.K. Brown

Subjects
chemistry.chemical_classification, biology, Mutant, Peptide, Major histocompatibility complex, Molecular biology, Papain, chemistry.chemical_compound, Protein structure, chemistry, Biochemistry, Gene expression, biology.protein, Glycoprotein, Gene
Abstract

The H-2K and H-2D alloantigens are primary products of genes of the K and D regions which map at opposite ends of the mouse H-2 MHC (major histocompatibility complex). These membrane-located glycoproteins are approximately 45,000 daltons in molecular weight and in the membrane are associated with a 12,000 molecular weight polypeptide, the murine β 2 -microglobulin. The H-2 products were analyzed by comparative tryptic peptide techniques. Comparison of products of the D and K genes, or of alleles within the D or K gene series showed that only from about 30 to 60% of the peptides were identical. This degree of variability is consistent with the high degree polymorphism shown by serological analysis of the H–2 products. Studies of mutants both at the H-2K and H-2D region showed small differences in peptide profiles, thus suggesting that minor alterations in primary protein structure may have remarkable biological effects. Preliminary N-terminal amino acid sequence analysis of the H-2 glycoproteins has supported the findings of their peptide variability. Comparison of the H-2 fragment released by papain digestion of the native glycoprotein also suggests that a region near the C-terminus is the site at which papain cleaves the native H-2 glycoprotein. Another approach to understanding the complexity of H-2 gene expression came from analysis of a regulatory variant selected for the lack of expression of H-2K d . This variant clone also did not express the linked but separate H-2D d product thus suggesting coordinate control of K and D gene expression. Altered homing properties of the variant suggested H-2 glycoproteins may play a role in cell sorting or recognition.

Published
1976
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