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101. Fc receptors for IgE on normal rat lymphocytes.

Author

Fritsche R and Spiegelberg HL

Subjects
Alkylation, Animals, Binding, Competitive, Erythrocytes immunology, Hot Temperature, Lymphoid Tissue immunology, Oxidation-Reduction, Rats, Rosette Formation, Trypsin pharmacology, Binding Sites, Antibody, Immunoglobulin Fc Fragments, Lymphocytes immunology
Published
1978

103. IgG-, IgA-, and IgE-induced release of leukotriene C4 by monocytes isolated from patients with atopic dermatitis.

Author

Ferreri NR, Zeiger RS, and Spiegelberg HL

Subjects
Antigens, Differentiation analysis, Antigens, Differentiation, B-Lymphocyte analysis, Calcimycin pharmacology, Female, Fluorescent Antibody Technique, Humans, Immunoglobulin Fab Fragments, Leukotriene B4 metabolism, Macromolecular Substances, Male, Receptors, Fc analysis, Receptors, IgE, Receptors, IgG, Rosette Formation, Dermatitis, Atopic immunology, Immunoglobulin A immunology, Immunoglobulin E immunology, Immunoglobulin G immunology, Monocytes physiology, SRS-A metabolism
Abstract

Purified peripheral blood monocytes isolated from patients with atopic dermatitis (AD) and from nonallergic normal donors were compared for their abilities to release leukotriene C4 (LTC4), leukotriene B4 (LTB4) and beta-glucuronidase in response to challenge with aggregated immunoglobulins or anti-immunoglobulins. The relationship between mediator release and the number of monocytes that formed rosettes with immunoglobulin-coated indicator cells was examined. Patients with AD had twice as many IgA- and three times as many IgE-rosetting monocytes as normal donors (48 +/- 12% versus 27 +/- 10% and 40 +/- 15% versus 14 +/- 3%, respectively), and yet the amounts of IgA- and IgE-induced LTC4 released were similar for both groups. This apparent discrepancy did not result from a decreased capacity for arachidonate metabolism via the C5-lipoxygenase pathway, since stimulation of monocytes from patients and normal donors with the calcium ionophore A23187 induced similar amounts of LTC4 and LTB4 release (LTC4, 3.0 +/- 1.7 versus 3.0 +/- 1.0 ng/10(6) cells; LTB4, 5.3 +/- 0.7 versus 5.2 +/- 0.5 ng/10(6) cells, respectively). In addition, aggregated IgG-induced LTC4 release by monocytes of both groups was similar, concomitant with an equivalent number of IgG-rosetting cells. Determination of cytophilically bound IgG and IgE by flow cytometry demonstrated that monocytes from atopic patients had more IgG bound than monocytes from normal donors. Similar amounts of IgE were detected on most monocytes from both groups, despite the higher serum IgE levels of patients. However, approximately 3% to 8% of monocytes from atopic but not normal donors stained brightly for IgE, suggesting that relatively large amounts of cytophilic IgE were bound to a small percentage of the patients' monocytes. Challenge of monocytes with anti-IgE or anti-IgG induced release of similar amounts of LTC4 for both groups, despite the presence of more cytophilic IgG on monocytes from atopic donors. These data indicate that monocytes from patients with AD release LTC4 and LTB4 in response to challenge with aggregated IgE or anti-IgE, as well as aggregated IgG, IgA, and anti-IgG. However, under our in vitro conditions, stimulation of patients' monocytes with aggregated IgA or IgE was not associated with increased mediator release, despite higher percentages of IgA- and IgE-rosetting cells compared to normal donors.

Published
1988
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104. Concomitant immunoglobulin E and immunoglobulin G1 formation in Nippostrongylus brasiliensis-infected mice.

Author

Lebrun P and Spiegelberg HL

Subjects
Animals, Female, Immunoglobulin Isotypes analysis, Immunoglobulin M biosynthesis, Immunologic Deficiency Syndromes complications, Immunologic Deficiency Syndromes genetics, Male, Mice, Mice, Inbred Strains immunology, Mice, Nude immunology, Nematode Infections complications, Nippostrongylus, Immunoglobulin E biosynthesis, Immunoglobulin G biosynthesis, Immunologic Deficiency Syndromes immunology, Mice, Mutant Strains immunology, Nematode Infections immunology
Abstract

The immunoglobulin (Ig)E, IgG subclass, and IgM formation in vivo and in vitro were measured by radioimmunoassays in normal and immunodeficient mice infected with the parasite Nippostrongylus brasiliensis (Nbr). High IgE responder mice had higher IgE serum levels than low responder mice both before (100 to 250 vs 2 to 20 ng of IgE/ml) and after (17,000 to 27,000 vs 1,000 to 5,000 ng of IgE/ml) infection. In vitro, mesenteric lymph node cells formed 5- to 10-fold more IgE than the spleen cells. Nu/nu mice had less than 1 ng before and 5 ng of IgE/ml serum after Nbr infection; no IgE was detectable in cell supernatants. There was no difference in the in vivo and in vitro IgE formation between C57BL/6 and C57BL/6-beige mice. Both in vivo and in vitro Nbr-infected Xid+ mice (CBA/N; (CBA/N X BALB/c) F1 male) formed approximately twice the amount of IgE than Xid- mice. Concomitant with the rise of the IgE serum levels, the IgG1 serum level increased by 100 to 1,500 micrograms/ml over preinfection levels in all strains except nu/nu+ mice. The IgM serum level increased by 100 to 500 micrograms/ml. In contrast, the IgG2a and IgG2b levels decreased in most strains, and the IgG3 levels remained unchanged. Nu/nu+ mice showed an increase of all IgG subclasses after Nbr infection. The antibodies to an Nbr extract were predominantly of IgM and IgG1, except in SJL mice which also had IgG2b and nude mice which only had IgM antibodies. The concomitant increase of IgE and IgG1 formation in all but the nude strains suggests that the regulation of these two Ig isotypes may be linked via regulatory T helper cells, which corroborates recent data on the simultaneous induction of IgG1 and IgE synthesis in vitro by the B cell stimulatory factor 1.

Published
1987

105. FC epsilon receptor-positive B and T lymphocytes in atopic disease.

Author

Spiegelberg HL, Thompson LF, Mellon MH, and Zeiger RS

Subjects
Asthma immunology, Basophils metabolism, Child, Humans, Molecular Weight, Monocytes metabolism, Receptors, Fc analysis, Receptors, IgE, Rhinitis, Allergic, Seasonal immunology, Rosette Formation, T-Lymphocytes classification, B-Lymphocytes metabolism, Hypersensitivity, Immediate immunology, Receptors, Immunologic analysis, T-Lymphocytes metabolism
Published
1983

106. Increased expression of the IgE Fc receptors on rat macrophages induced by elevated serum IgE levels.

Author

Boltz-Nitulescu G, Plummer JM, and Spiegelberg HL

Subjects
Animals, Antibodies, Neoplasm biosynthesis, Antibody Specificity, Hookworm Infections immunology, Immunoglobulin E analysis, Myeloma Proteins immunology, Nippostrongylus, Plasmacytoma immunology, Rats, Rats, Inbred Strains, Receptors, IgE, Rosette Formation, Immunoglobulin E metabolism, Macrophages immunology, Receptors, Fc analysis
Abstract

Macrophages (M phi) from rats with elevated serum IgE levels induced by (i) Nippostrongylus brasiliensis (Nb) infection, (ii) IgE-secreting plasmacytoma IR 162, or (iii) i.p. injection of purified rat IgE, and M phi from normal animals cultured in the presence of 10 micrograms/ml IgE were analysed for Fc IgE receptors (Fc epsilon R) expression. To detect Fc epsilon R-bearing cells, a rosette assay employing fixed ox erythrocytes coated with rat IgE was used. With undersensitized indicator cells a significantly (P less than 0.002) greater number of M phi from animals having elevated serum IgE levels or of M phi cultured in the presence of IgE formed IgE rosettes than M phi from normal donors. The IgE rosettes were IgE class-specific, since they were inhibited by rat IgE in a dose-dependent manner, but not by any other rat Ig class, heat-denatured rat IgE or human IgE. The modulating effect of Fc epsilon R expression on M phi was IgE specific, because neither rat IgG nor heated rat IgE induced increased IgE rosette formation. Furthermore, elevated serum IgE levels did not increase the expression of Fc receptors for IgG subclasses. Studies of 125I-IgE binding showed that alveolar macrophages (AM phi) from Nb-infected rats bind IgE with similar affinity (Ka 1.1 X 10(7) M-1) as AM phi from normal animals, but they have increased numbers of IgE binding sites. Collectively, the results demonstrate that in vivo and in vitro elevated serum IgE concentrations induce increased IgE rosette formation as a result of a marked increase in the number of Fc epsilon R per macrophage.

Published
1984

107. Characterization of the IgE Fc receptors on monocytes and macrophages.

Author

Spiegelberg HL, Boltz-Nitulescu G, Plummer JM, and Melewicz FM

Subjects
Humans, Immunoglobulin E immunology, Immunoglobulin epsilon-Chains immunology, Lymphocytes immunology, Phagocytosis, Rosette Formation, Macrophages immunology, Monocytes immunology, Receptors, Fc immunology
Abstract

Subpopulations of human monocytes (15%) and alveolar macrophages (AM phi, 8%) and rat and mouse AM phi (89%) and peritoneal M phi (57%) bear Fc receptors for IgE (Fc epsilon R) as shown by IgE-specific rosette formation. Cells from M phi-like cell lines of human, rat, and mouse origins also express Fc epsilon R. Monomeric IgE binds to Fc epsilon R on M phi with an equilibrium association constant Ka congruent to 10(7) M-1. The Fc epsilon R on human monocytes and M phi are antigenically similar to Fc epsilon R on lymphocytes but differ from Fc epsilon R on basophilic granulocytes. The Fc epsilon R on human and mouse M phi promote phagocytosis and lysis of IgE-coated erythrocytes. Patients with active IgE-mediated allergic diseases have elevated percentages of Fc epsilon R(+) monocytes (56%) that show allergic increased lytic activity against IgE-coated erythrocytes as compared to monocytes from normal humans. M phi from rats infested with Nippostrongylus brasiliensis parasites express more Fc epsilon R than normal M phi. The data indicate that Fc epsilon R expressed on M phi differ from those on mast cells and basophils, increase in number during IgE immune responses, and are likely to play an important role in the host's defense against parasites and in the pathogenesis of allergic diseases.

Published
1983

108. The use of Fab fragments of anti-human immunoglobulin as analytic tools for establishing the involvement of immunoglobulin in the spontaneous cytotoxicity to cultured tumor cells by lymphocytes from patients with bladder carcinoma and from healthy donors.

Author

Troye M, Perlmann P, Pape GR, Spiegelberg HL, Näslund I, and Gidlöf A

Subjects
Aged, Animals, Antibody Specificity, Cytotoxicity Tests, Immunologic, Dose-Response Relationship, Immunologic, Female, Humans, Immunity, Cellular, Immunoglobulin Fc Fragments, Immunosuppression Therapy, Male, Middle Aged, Rabbits, Time Factors, Antibodies, Anti-Idiotypic, Carcinoma, Transitional Cell immunology, Immunoglobulin Fab Fragments, Immunoglobulin G metabolism, Lymphocytes immunology, Urinary Bladder Neoplasms immunology
Published
1977

109. Quantitation of antibodies to IgM, IgD and beta2-microglobulin in antisera to chronic lymphatic leukemia lymphocytes.

Author

Kennel SJ, Levy RL, and Spiegelberg HL

Subjects
Antibody Specificity, Antilymphocyte Serum, Electrophoresis, Polyacrylamide Gel, Humans, Sodium Dodecyl Sulfate, Antibodies analysis, Beta-Globulins immunology, Immune Sera analysis, Immunoglobulin D immunology, Immunoglobulin M immunology, Leukemia, Lymphoid immunology, Lymphocytes immunology, beta 2-Microglobulin immunology
Abstract

Rabbit antisera were prepared to chronic lymphatic leukemia (CLL) lymphocytes and were tested for their reaction with radioiodinated, solubilized, cell surface proteins of normal and CLL lymphocytes. A pooled, hyperimmune antiserum precipitated at least 16 polypeptides from both normal and CLL lymphocytes as shown by sodium-dodecyl sulfate polyacrylamide gel electrophoresis. These polypeptides varied in molecular weight from 11,000 to 180,000. None was prominent or unique to the CLL lymphocytes, although four peptide bands in the CLL cells usually showed more radioactivity than their counterparts in normal cells. Precipitation with antisera of known specificity showed that the cell surface proteins from CLL and normal lymphocytes included HLA antigens and beta2-microglobulin. IgM and IgD were found in preparations of normal cells and in cells of 3 of 5 CLL patients. Of cells from the other 2 patients, one showed only IgD and the other no Ig. An antigen-binding capacity test was employed to quantitate the antibody content of a pooled anti-CLL lymphocyte serum. The antiserum reacted with all Ig classes; however, after absorption with light chains and F(ab')2 fragments, the serum retained activity only for IgM and IgD. The absorbed antiserum bound 45 microgram IgM, 1.5 microgram IgD and 4.5 microgram beta2-microglobulin per milliliter. These data indicate that rabbit anti-CLL lymphocyte sera fail to detect a qualitatively unique tumor-specific polypeptide on the surfaces of CLL cells. However, such antisera contain antibodies to many cell surface proteins including IgM, IgD, HLA antigens and beta2-microglobulin.

Published
1978
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110. IgE Fc receptor positive T and B lymphocytes in patients with the hyper IgE syndrome.

Author

Thompson LF, Spiegelberg HL, and Buckley RH

Subjects
Adolescent, Adult, Antigens, Surface analysis, Child, Fluorescent Antibody Technique, Humans, Immunoglobulin G immunology, Male, Rosette Formation, Syndrome, B-Lymphocytes immunology, Hypergammaglobulinemia immunology, Immunoglobulin E immunology, Receptors, Fc analysis, T-Lymphocytes immunology
Abstract

The percentages of peripheral blood lymphocytes (PBL), bearing Fc receptors for IgE (Fc epsilon R) and IgG (Fc gamma R) were determined in four patients with the hyper IgE syndrome by a rosette assay employing IgE and IgG coated fixed ox erythrocytes. The patients had 8 +/- 3% Fc epsilon R+ and 13 +/- 8% Fc gamma R+ PBL, compared to 1.2 +/- 1% Fc epsilon R+ and 17 +/- 4% Fc gamma R+ PBL for control donors. T cells were isolated by rosetting with neuraminidase treated sheep erythrocytes (EN). Indirect immunofluorescence with Lyt 3 monoclonal antibody (MoAb) to the sheep erythrocyte receptor, followed by rosetting for Fc epsilon R and Fc gamma R showed that the patients' T cells contained less than 0.1% Fc epsilon R+ and 1.4 +/- 0.2% Fc gamma R+ cells; T cells from the control subjects contained less than 0.1% Fc epsilon R+ and 11 +/- 4% Fc gamma R+ cells. The non-T (EN rosette depleted) cells of the patients included 56 +/- 18% sIgM+/sIgD+, 45 +/- 9% Fc epsilon R+ and 35 +/- 27% Fc gamma R+ cells. Indirect immunofluorescence with MoAb to IgM, IgD, and NK cells (antibody B73.1) followed by rosetting for Fc epsilon R and Fc gamma R, indicated that 92 +/- 2% of the Fc epsilon R+ cells and 9 +/- 7% of the Fc gamma R+ cells were B cells (mu+/delta+), while 3 +/- 4% of the Fc epsilon R+ and 30 +/- 23% of the Fc gamma R+ cells were NK cells (B73.1+). Thus, most of the Fc epsilon R+ non-T cells were B cells, and only a small fraction appeared to be NK cells. On the other hand, Fc gamma R+ B cells were outnumbered by Fc gamma R+ NK cells (B73.1+) by three to one. The data indicate that patients with the hyper IgE syndrome have increased numbers of Fc gamma R+ PBL, most of them being B cells, whereas their T cells contain less than 0.1% Fc epsilon R+ cells.

Published
1985

111. Immunoglobulins cytophilic for human lymphocytes, monocytes, and neutrophils.

Author

Lawrence DA, Weigle WO, and Spiegelberg HL

Subjects
Antibodies, Binding Sites, Antibody, Humans, Immune Sera, Immunity, Cellular, Immunoglobulin A analysis, Immunoglobulin D analysis, Immunoglobulin Fab Fragments analysis, Immunoglobulin Fc Fragments analysis, Immunoglobulin G analysis, Myeloma Proteins analysis, Phagocytosis, Protein Binding, Temperature, Immunoglobulins analysis, Lymphocytes immunology, Monocytes immunology, Neutrophils immunology
Abstract

The cytophilic activity of human myeloma proteins of different classes and subclasses for lymphocytes, monocytes, and neutrophils was investigated. Binding of both unaggregated immunoglobulins (Ig) and Ig aggregated with rabbit F(ab)2 anti-Fab fragment sera was determined. Lymphocytes bound unaggregated IgG1 and IgG3 proteins, but none of the proteins of the other classes. In contrast, after aggregation, IgG of all subclasses and IgE proteins bound to lymphocytes; aggregated proteins of the other classes did not bind. Monocytes bound unaggregated IgG1 and Ig3 better than Ig4 whereas the binding of proteins of other classes was insignificant. Neutrophils bound unaggregated IgG1 and IgG3 proteins and, in addition, IgA1, IgA2, secretory IgA, and IgG4 proteins. After aggregation, the neutrophils bound more Ig of all classes; however, the differences between the amounts bound remained similar to the amounts of unaggregated proteins. The native structure of the Ig molecule is necessary for the maintenance of complete activity, because Fc fragments bound less than intact Ig, and reduction and alkylation abolished cytophilia. The Fc receptors on all cell types tested showed no specificity for any of the respective cytophilic IgG subclasses; however, neutrophils appear to have separate receptors for IgG and IgA proteins.

Published
1975
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112. A serum factor in chronic hypocomplementemic hephritis distinct from immunoglobulins and activating the alternate pathway of complement.

Author

Vallota EH, Götze O, Spiegelberg HL, Forristal J, West CD, and Müller-Eberhard HJ

Subjects
Adsorption, Antibodies, Antibodies, Anti-Idiotypic, Centrifugation, Density Gradient, Chromatography, Gel, Chromatography, Ion Exchange, Glomerulonephritis complications, Humans, Immunodiffusion, Immunoelectrophoresis, Immunoglobulin G, Immunologic Deficiency Syndromes complications, Properdin, Complement System Proteins, Glomerulonephritis immunology, Immunologic Deficiency Syndromes immunology
Abstract

Nephritic factor (C3NeF) has been isolated from plasma of patients with hypocomplementemic chronic glomerulonephritis (HCG) by ion exchange and molecular sieve chromatography. This material was further treated with solidified anti-Ig antiserum. The purified material failed to react with antiserum to human IgG, IgG3, Fab, Fc, and kappa and lambda chains, but retained full C3NeF activity. The nonidentity of C3NeF with IgG was further demonstrated by Ouchterlony analysis using anti-IgG and anti-C3NeF. Isolated C3NeF was found to be a protein with a sedimentation coefficient of 7S and a mol wt of 150,000 daltons, which on microzone electrophoresis and gel electrophoresis at pH 8.6 behaved as a gamma-globulin. C3NeF is not a C1q precipitin and does not activate the classical complement pathway. Unlike cobra venom factor, it failed to enter into a complex with C3 proactivator (C3PA) when incubated with normal human serum (NHS) and then subjected to sucrose density gradient ultracentrifugation. The action of isolated C3NeF on C3 requires C3PA, C3PA convertase (C3PAse), and properdin (P). Similarly, C3PA conversion by C3NeF requires P, C3PAse, and C3. Total hemolytic activity was lost by incubation of 64 microg of C3NeF/1 ml NHS at 37 degrees C for 30 min. Both C3a and C5a anaphylatoxin could be generated by C3NeF in serum previously depleted of anaphylatoxin inactivator. Anti-C3NeF was found to detect an antigen in all NHS tested. Treatment of NHS with solidified anti-C3NeF caused impairment of the alternate complement pathway. It failed to sustain lysis of glutathione-treated human erythrocytes initiated by inulin. It is conceivable that the normal serum constituent which is removed by anti-C3NeF constitutes the inactive precursor of C3NeF, and a heretofore unrecognized component of the alternate pathway.

Published
1974
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113. Biological role of different antibody classes.

Author

Spiegelberg HL

Subjects
Animals, Complement Activation, Humans, Immunoglobulin Isotypes analysis, Lymphokines physiology, Receptors, Fc physiology, Immunoglobulin Isotypes physiology
Abstract

Antibodies are divided into different classes and subclasses (isotypes) according to structural differences in the constant region of the heavy polypeptide chains. The different isotypes mediate specific biologic functions that are important for the response to pathogens and in the pathogenesis of immunological diseases such as allergies. The numbers of different isotypes vary in different species, humans have 9 different Ig classes and subclasses. Of these 9, only IgM, IgG1, IgG2 and IgG3 activate the classical pathway of complement. All four IgG and both IgA subclasses, but not IgM, IgE and IgD, bind to Fc receptors on neutrophils, and induce the release of granule enzymes. All four IgG subclasses but no other Ig isotype induce serotonin release from platelets. In man, only IgE binds to the high-affinity Fc receptors (Fc epsilon RI) on mast cells and basophils and induces histamine and leukotriene release. IgE also binds to low-affinity Fc receptors (Fc epsilon RII) on lymphocytes, monocytes and eosinophils; however, the functions of Fc epsilon RII on these cells are not fully established. Monocytes from patients with atopic dermatitis that express more Fc epsilon RII than monocytes from normals do not release more LTC4 than monocytes from nonallergic healthy humans after activation with aggregated IgE. IgG and IgA are more efficient than IgE in inducing the release of mediators of inflammation from monocytes. The antibody response to certain antigens such as carbohydrates and allergens are often restricted to IgG2 and IgG1, IgG4 and IgE, respectively.(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1989
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114. Tryptic degradation of the CH1 and VL regions of IgD and IgE.

Author

Kocher HP and Spiegelberg HL

Subjects
Amino Acid Sequence, Chromatography, Gel, Cyanogen Bromide pharmacology, Electrophoresis, Polyacrylamide Gel, Humans, Immunoglobulin Fab Fragments, Peptides isolation & purification, Time Factors, Binding Sites, Antibody, Immunoglobulin Constant Regions, Immunoglobulin D, Immunoglobulin E, Immunoglobulin Variable Region, Immunoglobulins, Trypsin pharmacology
Published
1979

115. IgA rheumatoid factor in the sera and saliva of patients with rheumatoid arthritis and Sjögren's syndrome.

Author

Dunne JV, Carson DA, Spiegelberg HL, Alspaugh MA, and Vaughan JH

Subjects
Cross Reactions, Humans, Immunoglobulin M analysis, Lupus Erythematosus, Systemic immunology, Radioimmunoassay, Arthritis, Rheumatoid immunology, Immunoglobulin A analysis, Rheumatoid Factor analysis, Saliva immunology, Sjogren's Syndrome immunology
Abstract

With a sensitive radioimmunoassay we have found elevated IgA rheumatoid factor (IgA-RF) levels in the sera of patients with rheumatoid arthritis, Sjögren's syndrome, and systemic lupus erythematosus. The IgA--RF showed a pattern of reaction with human IgG subclasses and animal gammaglobulins similar to that of IgM-RF from the same patients. Rheumatoid factors of both classes were shown to be present in saliva of patients with rheumatoid arthritis and Sjögren's syndrome.

Published
1979
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116. Receptors specific for IgE on rat alveolar and peritoneal macrophages.

Author

Boltz-Nitulescu G and Spiegelberg HL

Subjects
Animals, Ascitic Fluid cytology, Cattle, Erythrocytes immunology, Immunoglobulin G, Lung cytology, Male, Rats, Rats, Inbred BN, Rats, Inbred BUF, Rats, Inbred Lew, Rosette Formation, Trypsin pharmacology, Immunoglobulin E immunology, Macrophages immunology, Receptors, Fc
Published
1981
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117. Cervical lymph node metastasis as the first manifestation of localized extramedullary plasmacytoma.

Author

Fishkin BG and Spiegelberg HL

Subjects
Aged, Diagnosis, Differential, Epiglottis, Female, Humans, Laryngeal Neoplasms blood, Lymphatic Metastasis pathology, Male, Middle Aged, Multiple Myeloma pathology, Myeloma Proteins blood, Nasopharyngeal Neoplasms blood, Neck, Plasmacytoma blood, Laryngeal Neoplasms pathology, Nasopharyngeal Neoplasms pathology, Plasmacytoma pathology
Abstract

Two patients who had cervical lymph node metastases as the first symptom of a localized soft tissue extramedullary plasmacytoma of the epiglottis and nasopharynx, respectively, are described. Classical multiple myeloma was excluded by bone marrow biopsies and x-ray studies of the skeleton. In both patients, the primary tumor was diagnosed 2 years after excision of the cervical lymph node. One patient had a IgD, lambda myeloma protein in the serum and excreted lambda Bence-Jones protein into the urine. No M-component was found in the other patient. Both are living with a long survival of 8 and 4 years respectively. The presence of a cervical lymph node plasmacytoma should suggest an upper respiratory tract or oropharynx plasmacytoma rather than a primary lymph node plasmacytoma.

Published
1976
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118. Release of leukotrienes, prostaglandins, and histamine into nasal secretions of aspirin-sensitive asthmatics during reaction to aspirin.

Author

Ferreri NR, Howland WC, Stevenson DD, and Spiegelberg HL

Subjects
Adult, Dinoprostone, Drug Hypersensitivity complications, Drug Hypersensitivity physiopathology, Female, Forced Expiratory Volume, Histamine Release, Humans, Leukotriene B4 metabolism, Male, Middle Aged, Prostaglandins E metabolism, Reference Values, SRS-A metabolism, Aspirin pharmacology, Asthma etiology, Drug Hypersensitivity metabolism, Nasal Mucosa metabolism
Abstract

The levels of leukotriene C4 (LTC4), leukotriene B4 (LTB4), prostaglandin E2 (PGE2), and histamine were measured in nasal lavage fluids obtained from aspirin-sensitive, desensitized aspirin-sensitive, and aspirin-insensitive asthmatics and normal volunteers before and after ingestion of aspirin. Increased levels of LTC4 and histamine were associated with significant decreases in the FEV1 for 3 of 4 aspirin-sensitive asthmatics who had both naso-ocular and bronchospastic reactions to aspirin. In contrast, no increase in LTC4 or histamine release was detected in aspirin-sensitive asthmatics who had only bronchospastic reactions to aspirin. No significant decreases in PGE2 levels or increases in LTB4 levels were detected during these reactions to relatively low doses of aspirin regardless of the clinical symptoms, nor was any increase in mediator release apparent in lavage fluids from normal donors, aspirin-insensitive asthmatics, and desensitized aspirin-sensitive subjects before or after various doses of aspirin. Levels of PGE2 decreased in nasal secretions from normal volunteers, aspirin-insensitive asthmatics, and desensitized aspirin-sensitive subjects after ingestion of 650 mg of aspirin. These decreases were not associated with increased LTC4 or LTB4 or with histamine release, decreased FEV1, or naso-ocular symptoms. In addition, reductions of PGE2 release were similar for normal and desensitized aspirin-sensitive volunteers (63 +/- 11 versus 61 +/- 10%, respectively). The data demonstrate that LTC4 and histamine are released into nasal secretions of aspirin-sensitive asthmatics with naso-ocular and bronchospastic reactions after ingestion of low doses of aspirin without a decrease in the levels of PGE2 and suggest that LTC4 and histamine contribute to the naso-ocular and bronchospastic symptoms characteristic of reactions to aspirin.

Published
1988
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119. Human myeloma IgG half-molecules. Structural and antigenic analyses,.

Author

Spiegelberg HL, Heath VC, and Lang JE

Subjects
Amino Acid Sequence, Amino Acids analysis, Animals, Binding Sites, Electrophoresis, Polyacrylamide Gel, Electrophoresis, Starch Gel, Epitopes, Guanidines, Humans, Immunodiffusion, Immunoglobulin Fc Fragments, Immunoglobulin Fragments, Immunoglobulin Heavy Chains, Macromolecular Substances, Molecular Weight, Peptide Fragments analysis, Protein Binding, Rabbits immunology, Ultracentrifugation, Immunoglobulin G, Myeloma Proteins
Abstract

The structure and antigenic characteristics of a human k, IgG myeloma protein that formed half-molecules were analyzed. Most of the myeloma protein found in the patient's serum and urine consisted to two chain 4.3S half-molecules. A small amount of four chain 7S myeloma protein was, however, found in the serum and was apparently formed by the same clone of tumor cells. Polyacrylamide gel electrophoresis in 8 M urea and 1% sodium dodecyl sulfate and analytical ultracentrifugation in 6 M guanidine of the fully reduced and alkylated half-molecule indicated that this myeloma protein had a heavy chain of a smaller molecular weight (approximately 45,000) than that of normal gamma chains, Except for this apparent deletion, the heavy chain resembled gamma1 chains. The amino acid composition of the peptides containing the half-cysteine residues forming the interchain disulfide bonds, the glycopeptide of the Fc fragment and the COOH-terminal structure were similar if not identical with the analogous structures of gamma1 chains. No Fc fragment could be prepared because the Fc portion of the heavy chain of the myeloma protein was extremely susceptible to degradation with papain. After mild reduction and alkylation, the 7S myeloma protein dissociated into half-molecules, indicating a lack of noncovalent interactions in the Fc fragment that are present in all classes of human immunoglogulins and are responsible for the formation ofFc dimers. The half-molecule was antigenically deficient in the Fc fragment. It failed to precipitate with anti-Fc fragment antisera in double gel diffusion tests and inhibited a Fc-anti-Fc fragment binding reaction weakly and incompletely. The half-molecule and the 7S protein had the same genetic markers on the first and second homology region of the gamma chain. The half-molecule lacked, however, the corresponding markers on the third homology region, These findings suggest that this myeloma protein had a deletion in the gamma chain which was probably located in third homology region and was likely the structural abnormality responsible for the lack of noncovalent interaction in the Fc fragment and absence of most of the antigenic determinants characteristic of gamma chains.

Published
1975
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121. Relationship between molecular size and intra- and extravascular diribution of protein antigens.

Author

Nakamura RM, Spiegelberg HL, Lee S, and Weigle WO

Subjects
Animals, Extracellular Space, Fibrinogen metabolism, Iodine Isotopes, Lymph analysis, Macroglobulins metabolism, Plasma analysis, Rabbits, Serum Albumin metabolism, Serum Albumin, Bovine metabolism, Serum Globulins metabolism, Thoracic Duct, Antigens, Blood Proteins metabolism, Molecular Weight
Published
1968

123. The interaction of Hageman factor and immune complexes.

Author

Cochrane CG, Wuepper KD, Aiken BS, Revak SD, and Spiegelberg HL

Subjects
Animals, Azo Compounds, Blood Coagulation, Cattle, Centrifugation, Density Gradient, Chromatography, Gel, Chromatography, Ion Exchange, Hot Temperature, Humans, Immunoglobulin G, Iodine Isotopes, Kallikreins, Kaolin, Macromolecular Substances, Myeloma Proteins, Precipitin Tests, Rabbits immunology, Serum Albumin, Bovine, Spectrophotometry, Ultraviolet Rays, Antigen-Antibody Complex, Factor XII isolation & purification
Abstract

The possible interaction of Hageman factor from human or rabbit plasma with a variety of immunologic reactants was studied. Evidence of an interaction was not obtained and neither binding of radiolabeled Hageman factor to immune aggregates nor depletion of the Hageman factor from the supernate was observed. Cleavage of the labeled Hageman factor molecule into its 30,000 molecular weight-active fragments was not detectable after incubation with immune complexes. Isolated Hageman factor was far more sensitive to activation than Hageman factor in plasma or serum. There was no consistent activation of isolated Hageman factor by immunologic reactants as determined by conversion of prekallikrein to its enzymatic form or by shortening of the clotting time of factor XII-deficient plasma. A variety of immunologic stimuli were tested: (a) antigen-antibody complexes in soluble or precipitated form; (b) particulate antigen-antibody complexes, i.e., zymosan-anti-zymosan in which a surface was presented for activation; (c) human IgM-IgG and IgG-IgG (rheumatoid factor) complexes; (d) immune aggregates consisting of heat or bis-diazotized benzidine-aggregated myeloma proteins of all human immunoglobulin classes and subclasses: IgG(1,2,3,4), IgA, IgD, IgM, and IgE. Absorption with immune aggregates did not reduce the quantity of Hageman factor in solution, nor was the Hageman factor bound to the precipitates. The presence of plasma or serum with immune aggregates did not generate activity of the Hageman factor. The only preparations of immunoglobulins capable of activating Hageman factor were found to be contaminated with bacteria. These bacteria, upon isolation, activated Hageman factor.

Published
1972
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124. Catabolism of human gammaG-immunoglobulins of different heavy chain subclasses. I. Catabolism of gammaG-myeloma proteins in man.

Author

Spiegelberg HL, Fishkin BG, and Grey HM

Subjects
Animals, Blood Protein Electrophoresis, Chemical Phenomena, Chemistry, Chromatography, Female, Hexoses analysis, Humans, Immune Sera, Iodine Isotopes, Male, Molecular Weight, Multiple Myeloma blood, Neoplasm Proteins blood, Ultracentrifugation, Multiple Myeloma immunology, gamma-Globulins metabolism
Abstract

The rates of catabolism of human gammaG-immunoglobulins of subclasses gammaG(1), gammaG(2), gammaG(3), and gammaG(4) were studied by determining the rates of elimination from the circulation of pairs of (131)I-and (125)I-labeled gammaG-myeloma proteins in 57 patients suffering from cancer other than multiple myeloma. On the average, gammaG(1)-, gammaG(2)-, and gammaG(4)-myeloma proteins were catabolized at a rate similar to that of normal gammaG-immunoglobulin, whereas gammaG(3)-myeloma proteins were catabolized more rapidly than normal gammaG-immunoglobulin. The average half-lives for the myeloma proteins were 12.3 days for normal gammaG, 11.6 days for gammaG(1), 12.4 days for gammaG(2), 8.2 days for gammaG(3), and 11.3 days for gammaG(4). However, significant differences in catabolic rates were observed when individual myeloma proteins of a single subclass were compared. These individual variations were present within all four heavy chain subclasses. The extent of differences ranged from 10 to 47%. The catabolic rate of normal gammaG was in an intermediate range when compared with myeloma proteins of relatively long and short half-lives. The rate of catabolism of an individual myeloma protein did not correlate with its light chain type, Gm factor, carbohydrate content, or electrophoretic mobility. These findings indicate that the structure(s) related to the catabolism of gammaG-immunoglobulins are complex and differ from one immunoglobulin molecule to another.

Published
1968
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125. The in vivo formation and fate of antigen-antibody complexes formed by fragments and polypeptide chains of rabbit gamma-G-antibodies.

Author

Spiegelberg HL and Weigle WO

Subjects
Animals, Rabbits, Antibodies, Antigen-Antibody Reactions, Peptides, gamma-Globulins
Abstract

The in vivo formation and subsequent fate of complexes formed between specific rabbit gammaG-antibody subunits and circulating protein antigens was studied in rabbits and guinea pigs. Subunits obtained from purified antibodies were injected immediately after an injection of antigen, and the elimination from the circulation of either I*-labeled gammaG-subunits or labeled antigen determined. In the absence of antigen, all gammaG-subunits which lack the Fc fragment were rapidly eliminated. In the presence of excess antigen, F (ab')(2), Fab and Fd fragments reacted with antigen and remained in the circulation as complexes which were eliminated at the same rate as the antigen. Fab hybrids containing a specific Fd fragment and a nonspecific L chain similarly reacted with antigen and remained in the circulation complexed to antigen. In contrast, L chains and Fab hybrids containing a specific L chain and a nonspecific Fd fragment did not react with antigen in vivo and were rapidly eliminated in both presence and absence of antigen. H chains remained in the circulation of rabbits in the absence of antigen, however, in the presence of antigen, more H chains which formed complexes with antigen remained in the intravascular space and were rapidly eliminated when the immune elimination of the antigen by the host occurred. Nonspecific H chains were rapidly eliminated from the circulaion of guinea pigs, whereas specific H chains remained in the circulation with the antigen. F (ab')(2) fragments formed complexes with antigen near antibody equivalence and in antibody excess which were rapidly eliminated, however, less effectively than complexes formed near antibody equivalence with intact gammaG. Complexes formed in antibody excess between Fab fragments and H chains remained in the circulation at all concentrations studied and were eliminated at the rate of antigen. The role of the Fc fragment in the immune elimination of antigen-antibody complexes is discussed.

Published
1966
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126. The release of granule enzymes from human neutrophils stimulated by aggregated immunoglobulins of different classes and subclasses.

Author

Henson PM, Johnson HB, and Spiegelberg HL

Subjects
Chromatography, DEAE-Cellulose, Cytoplasm enzymology, Cytoplasmic Granules enzymology, Humans, Immunodiffusion, Immunoglobulin A analysis, Immunoglobulin G analysis, Iodine Isotopes, L-Lactate Dehydrogenase metabolism, Macroglobulins pharmacology, Micropore Filters, Microscopy, Electron, Muramidase metabolism, Myeloma Proteins analysis, Myeloma Proteins classification, Peroxidases metabolism, Phagocytosis, Protein Denaturation, Tetanus Antitoxin, Tetanus Toxoid, Glucuronidase blood, Immunoglobulins analysis, Myeloma Proteins pharmacology, Neutrophils enzymology
Published
1972

127. Studies on the catabolism of gamma- G subunits and chains.

Author

Spiegelberg HL and Weigle WO

Subjects
Blood Protein Electrophoresis, Humans, Immunochemistry, In Vitro Techniques, Iodine Isotopes, Neuraminidase, Papain, Urine, Bence Jones Protein, Heavy Chain Disease, Multiple Myeloma, Peptides, gamma-Globulins
Published
1965

128. THE CATABOLISM OF HOMOLOGOUS AND HETEROLOGOUS 7S GAMMA GLOBULIN FRAGMENTS.

Author

SPIEGELBERG HL and WEIGLE WO

Subjects
Animals, Guinea Pigs, Mice, Rabbits, Antibodies, Cysteine, Immunoglobulin G, Papain, Pepsin A, Proteins metabolism, Research, Thyroid Function Tests, Urine, gamma-Globulins
Abstract

The catabolism of homologous and heterologous 7S gamma globulin fragments obtained by pepsin and papain digestion was studied in rabbits, guinea pigs, and mice. The elimination from the circulation of I* labeled gamma globulin fragments was followed and the urinary excretion of the total and protein-bound I* activity determined. Evidence is presented that the molecular structure responsible for the catabolism of 7S gamma globulin is located in papain fragment III. The elimination of papain fragment III was slow and closely related to the intact gamma globulin, whereas the pepsin fragment and papain fragments I and II were rapidly eliminated and catabolized in all species examined. Prolonged incubation with cysteine altered papain fragment III as shown by a rapid catabolism of a large portion of incubated fragment III within 24 hours after injection. Small amounts of intact RGG and RGG papain fragment III were excreted as protein-bound I* activity in the urine. On the other hand, large amounts of the pepsin fragment and papain fragments I and II of RGG were excreted as protein-bound I* activity in the urine. The possibility of a molecular structure present in papain fragment III, which may be responsible for tubular reabsorption in the kidney, is discussed. The rate of urinary excretion of fragments obtained from RGG was different from that of fragments obtained from gamma globulin of several other species. In general, small amounts of the pepsin fragment and papain fragment III obtained from gamma globulin other than RGG were excreted as protein-bound I* activity. The amounts of fragment I* excreted as protein-bound I* activity depended on the species in which it was injected, as well as the source of the gamma globulin. The rapid catabolism of the pepsin fragment and papain fragments I or II which bear antibody-combining sites suggest that their use for the prophylactic treatment of tetanus and diphtheria in man is limited.

Published
1965
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129. Localization of the carbohydrate within the variable region of light and heavy chains of human gamma g myeloma proteins.

Author

Spiegelberg HL, Abel CA, Fishkin BG, and Grey HM

Subjects
Amino Acid Sequence, Amino Acids analysis, Blood Protein Electrophoresis, Fucose analysis, Glucosamine analysis, Hexoses analysis, Humans, Immunoglobulins analysis, Models, Chemical, Multiple Myeloma blood, Neuraminic Acids analysis, Peptides analysis, Bence Jones Protein analysis, Carbohydrates analysis, Immunoglobulin G analysis
Published
1970
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130. IgE multiple myeloma: a report of the third case.

Author

Fishkin BG, Orloff N, Scaduto LE, Borucki DT, and Spiegelberg HL

Subjects
Aged, Allopurinol therapeutic use, Animals, Blood Transfusion, Bone Marrow Examination, Cyclophosphamide therapeutic use, Electrophoresis, Female, Goats, Humans, Immune Sera, Immunochemistry, Immunodiffusion, Immunoglobulin E analysis, Melphalan therapeutic use, Multiple Myeloma complications, Multiple Myeloma therapy, Osteosclerosis etiology, Pelvis diagnostic imaging, Rabbits, Radiography, Multiple Myeloma immunology, Myeloma Proteins analysis
Published
1972

131. Structural studies of human gamma D myeloma protein.

Author

Spiegelberg HL, Prahl JW, and Grey HM

Subjects
Amino Acids analysis, Autoanalysis, Carbohydrates analysis, Chemical Phenomena, Chemistry, Cyanides, Electrophoresis, Fibrinolysin, Glucosamine analysis, Glycoproteins analysis, Hexosamines analysis, Humans, Immunoglobulins, Iodine, Iodine Isotopes, Methods, Models, Structural, Molecular Weight, Multiple Myeloma blood, Neuraminidase, Oxidation-Reduction, Papain, Trypsin, Ultracentrifugation, Immunoglobulin G analysis, Multiple Myeloma immunology, Peptides analysis, Peptides isolation & purification
Published
1970
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132. IgD multiple myeloma: a report of five cases.

Author

Fishkin BG, Glassy FJ, Hattersley PG, Hirose FM, and Spiegelberg HL

Subjects
Adult, Aged, Bence Jones Protein analysis, Blood Protein Electrophoresis, Cyclophosphamide therapeutic use, Humans, Male, Middle Aged, Multiple Myeloma drug therapy, Immunoglobulin G analysis, Multiple Myeloma immunology
Published
1970
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133. Structural studies of human J chain.

Author

Meinke GC and Spiegelberg HL

Subjects
Alkylation, Amino Acid Sequence, Asparagine analysis, Autoanalysis, Carbon Isotopes, Humans, Immunoglobulin A analysis, Immunoglobulin M analysis, Iodoacetates metabolism, Macroglobulins analysis, Multiple Myeloma immunology, Myeloma Proteins analysis, Oxidation-Reduction, Peptide Chain Termination, Translational, Polymers, Waldenstrom Macroglobulinemia immunology, Immunoglobulin Fragments analysis
Published
1972

134. THE EFFECT OF 6-MERCAPTOPURINE AND AMINOPTERIN ON EXPERIMENTAL IMMUNE THYROIDITIS IN GUINEA PIGS.

Author

SPIEGELBERG HL and MIESCHER PA

Subjects
Animals, Guinea Pigs, Aminopterin, Antibody Formation, Antigen-Antibody Reactions, Hypersensitivity, Delayed, Immunization, Mercaptopurine, Pharmacology, Research, Thyroglobulin, Thyroiditis
Abstract

The influence of 6-mercaptopurine and aminopterin was studied on immune response and immune thyroiditis in guinea pigs immunized with thyroid extract. 1. Both compounds depressed delayed hypersensitivity to thyroglobulin and immune thyroiditis. 2. Antibody formation to thyroglobulin was strongly depressed by aminopterin but not significantly influenced by 6-mercaptopurine. 3. Immune response and thyroiditis were suppressed as long as the compounds were administered; after discontinuation of treatment, immune response and thyroiditis appeared in the same time intervals as observed in control animals after initiation of immunization. 4. Treatment with 6-mercaptopurine and aminopterin 10 days after immunization lead to suppression of delayed hypersensitivity and thyroiditis. 5. Treatment with 6-mercaptopurine of animals after onset of thyroiditis lead to suppression of delayed hypersensitivity and disappearance or diminution of round cell infiltration in the thyroid. 6. The results are discussed in terms of the pathogenesis of experimental immune thyroiditis, the mode of action of these antimetabolites on this experimental immune disease, and in view of the potential value of these compounds in human diseases.

Published
1963
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139. Release of serotonin from human platelets induced by aggregated immunoglobulins of different classes and subclasses.

Author

Henson PM and Spiegelberg HL

Subjects
Antigen-Antibody Complex, Biphenyl Compounds pharmacology, Blood Platelets drug effects, Blood Platelets enzymology, Complement System Proteins, Hot Temperature, Humans, Immunoglobulin Fab Fragments, Immunoglobulin Fc Fragments, Immunoglobulin G, L-Lactate Dehydrogenase metabolism, Macroglobulins, Myeloma Proteins, Platelet Adhesiveness, Tritium, Blood Platelets metabolism, Immunoglobulins, Serotonin metabolism
Abstract

The ability of human myeloma proteins of different classes and subclasses and of macroglobulins (all aggregated with bis-diazotized benzidine or heat) to aggregate washed human platelets and release [(3)H]-serotonin from the platelets was investigated and compared with the activity of normal IgG and tetanus-antitetanus IgG antigen-antibody complexes. Aggregated IgG1, IgG2, IgG3, IgG4, and normal IgG complexes all aggregated platelets and caused release of serotonin to similar extents. In contrast, IgA1, IgA2, IgD, and IgE myeloma proteins as well as IgM macroglobulins were completely inactive in this respect. Approximately 50% of the actvity remained in aggregated, mildly reduced and alkylated IgG myeloma proteins and their Fc fragments, whereas aggregated F(ab')(2) fragments were completely inactive. Addition of fresh serum inhibited the release of serotonin caused by aggregated IgG1 and IgG3 proteins and normal IgG antigen-antibody complexes by about 50% but had no effect upon the release of serotonin obtained with IgG2 and IgG4 proteins. This inhibition appeared to be mediated by complement. The release of serotonin was not accompanied by liberation of the cytoplasmic enzyme lactic dehydrogenase, indicating that no significant lysis of the platelets occurred. Addition of neutrophils did not enhance the serotonin release.

Published
1973
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140. Autoimmunity and termination of immunological unresponsiveness.

Author

Weigle WO, Nakamura RM, Spiegelberg HL, Golub ES, and High GJ

Subjects
Animals, Hemagglutination, Injections, Iodine Isotopes, Proteins, Rabbits, Serum Albumin, Bovine, Thyroglobulin pharmacology, gamma-Globulins, Antibody Formation, Autoantibodies, Autoimmune Diseases, Immune Tolerance, Thyroiditis immunology
Published
1967

143. Immunoglobulin G subclass of human antinuclear antibodies.

Author

Tojo T, Friou GJ, and Spiegelberg HL

Subjects
Antibodies, Antinuclear isolation & purification, Complement Fixation Tests, DNA, Immunodiffusion, Lupus Erythematosus, Systemic immunology, Nephritis immunology, Procainamide adverse effects, Antibodies, Antinuclear analysis, Immunoglobulin G analysis
Published
1970

144. 2,4-Dinitrophenyl receptors on mouse thymus and spleen cells.

Author

Lawrence DA, Spiegelberg HL, and Weigle WO

Subjects
Animals, Autoradiography, Binding Sites, Cortisone pharmacology, Immune Sera, Mice, Mice, Inbred CBA, Ovalbumin, Serum Albumin, Bovine, gamma-Globulins, Antigens, Dinitrophenols, Spleen immunology, T-Lymphocytes immunology
Abstract

A higher percentage of specific antigen-binding cells can be detected not only in normal CBA/J mouse spleen cell preparations (0.99%), but also in the normal thymus cell preparations (0.15%) with the use of [(125)I]2,4-dinitrophenyl-human IgG (DNP-HGG) as compared with most other antigens employed under similar conditions. The receptors on these cells are mainly specific for the DNP group as shown by the inhibition studies with DNP-lysine and the other DNP conjugates. In addition, it was shown by the inhibition studies with DNP-lysine that the thymus cells seem to have a lower avidity for DNP than the spleen cells. Preincubation of cell suspensions with antisera to immunoglobulins showed that the DNP-HGG antigen-binding cells in the thymus are inhibited predominantly with anti-micro-chain serum and the spleen cells with both anti-micro-chain and anti-gamma-chain sera; both cell populations were also significantly inhibited with the antisera to kappa-chains and Fab fragments. These data indicate that the nature of the receptor on the T cell differs from that on the majority of spleen cells.

Published
1973
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