Your search keyword '"Mast Cells ultrastructure"' showing total 33 results

1. Images iin Allergy and Immunology. Mouse spleen basophils.

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Author

Dvorak AM and Sciuto TE

Subjects

Animals, Eosinophils ultrastructure, Mast Cells ultrastructure, Mice, Models, Animal, Neutrophils ultrastructure, Basophils ultrastructure, Spleen cytology

Published

2004

2. Mast cell degranulation induced by lectins: effect on neutrophil recruitment.

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Author

Moreno AN, Jamur MC, Oliver C, and Roque-Barreira MC

Subjects

Animals, Immunity, Innate, Interleukin-8 metabolism, Mannose-Binding Lectins metabolism, Mast Cells ultrastructure, Rats, Rats, Wistar, Cell Degranulation drug effects, Interleukin-8 pharmacology, Lectins pharmacology, Mannose-Binding Lectins pharmacology, Mast Cells physiology, Neutrophils physiology

Abstract

The mammalian lectin macrophage-derived neutrophil chemotactic factor (MNCF) and the plant lectin KM+ were characterized for their ability to activate and degranulate mast cells. The association between mast cell activation and the induction of neutrophil migration was also investigated. Incubation of rat peritoneal mast cells with these lectins resulted in degranulation and mediator release. By confocal microscopy, both lectins were evenly distributed on the cell surface. MNCF activated RBL-2H3 mast cells only if the cells had been sensitized with IgE. KM+ was able to activate either unsensitized or IgE sensitized RBL-2H3 cells. In microplate assays MNCF, but not KM+, bound to rat IgE. In rats that were depleted of mast cells, neutrophil recruitment by MNCF and KM+ were significantly reduced indicating that mast cell activation provides an amplification loop for the neutrophil recruitment induced by these lectins. The present study supports the concept that mammalian lectins play a fundamental role in innate immunity., (Copyright 2003 S. Karger AG, Basel) more...

Published

2003

3. Involvement of arachidonic acid in nonimmunologic production of superoxide in mast cells.

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Author

Sakaguchi M, Fukuishi N, Teramoto K, Miyazaki M, Huh NH, Namba M, and Akagi M

Subjects

Animals, Histamine Agonists pharmacology, Male, Mast Cells ultrastructure, Microscopy, Electron, Scanning, Rats, Rats, Wistar, Signal Transduction drug effects, Signal Transduction immunology, Arachidonic Acid pharmacology, Mast Cells drug effects, Mast Cells metabolism, Superoxides metabolism

Abstract

Background: A number of different molecules are known to be involved in the signal pathway to release histamine from mast cells, among which arachidonic acid (AA) is one of the key mediators. On the other hand, we found that the application of compound 48/80, a typical histamine liberator, generated superoxide in mast cells. In the present study, we investigated the mechanism of superoxide production in mast cells with respect to AA signaling in conjunction with a fine structural analysis., Methods: Superoxide production was monitored by chemiluminescence in rat peritoneal mast cells and their subfractions after various treatments. For scanning electron micrography, the conditions for fixation and freeze-fracture were optimized to get natural fine images., Results: Compound 48/80 induced superoxide production in the isolated mast cells and some of their subfractions possibly through intracellular increase in Ca(2+) concentration, activation of cytosolic phospholipase A(2), and release of AA., Discussion: The present results indicate the critical role of AA in the signal pathway to generate superoxide from mast cells in response to compound 48/80., (Copyright 2003 S. Karger AG, Basel) more...

Published

2003

4. Ultrastructure of human mast cells.

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Author

Dvorak AM

Subjects

Humans, Lipids analysis, Mast Cells chemistry, Mast Cells physiology, Secretory Vesicles physiology, Secretory Vesicles ultrastructure, Mast Cells ultrastructure

Abstract

Ultrastructural studies of human mast cells define their organelles and the impact of environment, development and function on their ultrastructural morphology. The studies we review here implicate lipid bodies in eicosanoid and cytokine biology, and extend the functional repertoire of secretory-storage granules to synthesis., (Copyright 2002 S. Karger AG, Basel) more...

Published

2002

5. Roles of superoxide dismutase in rat mast cell granules.

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Author

Fukuishi N, Takahashi H, Harada N, Kanoh R, Matsui N, and Akagi M

Subjects

Animals, Calcium pharmacology, Cells, Cultured, Chemokine CCL4, Cytoplasmic Granules physiology, Hydrogen Peroxide pharmacology, Inflammation physiopathology, Macrophage Inflammatory Proteins metabolism, Male, Mast Cells ultrastructure, Rats, Rats, Wistar, Subcellular Fractions, Cytoplasmic Granules enzymology, Mast Cells enzymology, Superoxide Dismutase metabolism

Abstract

Background: It has been suggested that in the granules of rat mast cells there is some kind of superoxide dismutase (SOD), but details of this SOD in mast cells remain unclear. In the present study, we studied the mode of existence of SOD in mast cells and its releasing mechanism from the granules. In addition, we discussed the physiological role of SOD in allergic events., Methods: Purified rat mast cells were disrupted with a sonic disrupter and granules (sample I) were separated from supernatant (sample II) by centrifugation. The granules were treated with 1 mM Ca(2+), and the supernatant (sample III) was separated from the pellet (sample IV). Sample III was applied to a heparin column and the eluate was used as sample V. SOD activity was measured in these samples., Results: SOD existed in mast cell granules as a heparin-binding and an inactive form. However, when granules were released and exposed to high Ca(2+) concentration, SOD was discharged from heparin and shifted to the active form. The expression of macrophage inflammatory protein-1 alpha mRNA was enhanced when hydrogen peroxide (H(2)O(2)) or sample III with the xanthine-xanthine oxidase system were added to the culture media., Conclusions: These findings suggest that in stimulated rat mast cells, the released SOD may transform the generated superoxide anion into H(2)O(2), and the generated H(2)O(2) may enhance the expression of chemokine mRNA in the mast cells., (Copyright 2001 S. Karger AG, Basel) more...

Published

2001

6. IgG-mediated histamine release from canine mastocytoma-derived cells.

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Author

Takahashi T, Kitani S, Nagase M, Mochizuki M, Nishimura R, Morita Y, and Sasaki N

Subjects

Animals, Calcimycin pharmacology, Cell Line, Chymases, Dog Diseases pathology, Female, Intestinal Neoplasms ultrastructure, Ionophores pharmacology, Male, Mast Cells drug effects, Mast Cells ultrastructure, Mast-Cell Sarcoma ultrastructure, Microscopy, Electron, Serine Endopeptidases analysis, Skin Neoplasms ultrastructure, Substance P pharmacology, Tryptases, Tumor Cells, Cultured, Dog Diseases immunology, Dogs immunology, Histamine Release, Immunoglobulin G pharmacology, Intestinal Neoplasms veterinary, Mast Cells immunology, Mast-Cell Sarcoma veterinary, Skin Neoplasms veterinary

Abstract

Background: Recent data suggest that normal tissue mast cells can express functional receptors for IgG under certain conditions. However, little is known about IgG receptor expression and functional consequences in mast cell neoplasms., Methods: In this study, neoplastic mast cells were obtained from a dog with cutaneous mastocytoma (CM-MC) and from a dog with visceral mastocytoma (VI-MC). Both cell populations were characterized morphologically and functionally., Results: Most cells proliferated constantly in suspension without particular supplements. Doubling times of CM-MC and VI-MC were 52.2 and 27.5 h, respectively. Both cell types were sensitive to formalin fixation, did not contain heparin and were tryptase and chymase positive. Electron microscopy showed fine granules with electron-dense content in both cell populations. The total histamine content of CM-MC and VI-MC was 0.25 and 0.10 pg/cell, respectively. Calcium ionophore A23187 and substance P induced dose-dependent histamine release, whereas compound 48/80 had no effect. Most significantly, both cell types, when sensitized with monomeric dog IgG, released histamine upon stimulation by anti-dog IgG., Conclusions: Dog mastocytoma-derived cells may be useful to study the regulation of neoplastic mast cell growth and differentiation, as well as IgG receptor-mediated activation in neoplastic mast cells. Further research is required to clarify the pathophysiological significance of constitutive expression of IgG receptors in neoplastic (canine) mast cells., (Copyright 2001 S. Karger AG, Basel.) more...

Published

2001

7. Ultrastructural autoradiographic analysis of RNA in isolated human lung mast cells during secretion and recovery from secretion.

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Author

Dvorak AM, Morgan ES, Lichtenstein LM, and Schleimer R

Subjects

Autoradiography, Cell Degranulation physiology, Cytoplasmic Granules metabolism, Cytoplasmic Granules ultrastructure, Humans, Lung physiology, Mast Cells physiology, Microscopy, Electron, Subcellular Fractions metabolism, Time Factors, Tritium, Uridine metabolism, Lung metabolism, Lung ultrastructure, Mast Cells metabolism, Mast Cells ultrastructure, RNA metabolism

Abstract

Background: Previous work has implicated isolated, control human lung mast cell granules in RNA metabolism using multiple methods of high-magnification imaging based on different mechanistic principles. These methods have demonstrated ribosomes, RNA, U1snRNP and uridine in, around and attached to secretory granules., Methods: Here, we have extended these studies using ultrastructural autoradiography of radiolabeled uridine incorporation in degranulating and recovering mast cells., Results: We found that control cells incorporated uridine into granules, with values that decreased dramatically in conjunction with stimulated histamine secretion and granule extrusion, and that granule stores of tritiated uridine increased together with the reconstitution of secretory granules in recovering mast cells., Conclusion: These findings support a possible new role for secretory granules in RNA metabolism in mast cell biology., (Copyright 2000 S. Karger AG, Basel.) more...

Published

2000

8. Images in allergy and immunology. Mast cell apoptosis.

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Author

Dvorak AM

Subjects

Animals, Cell Membrane ultrastructure, Mice, Microscopy, Electron, Organelles ultrastructure, Apoptosis, Bone Marrow Cells physiology, Mast Cells physiology, Mast Cells ultrastructure

Published

1999

9. Novel autocrine and paracrine loops of the stem cell factor/chymase network.

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Author

de Paulis A, Minopoli G, Dal Piaz F, Pucci P, Russo T, and Marone G

Subjects

Autocrine Communication, Chymases, Cytoplasmic Granules immunology, Humans, Mast Cells ultrastructure, Paracrine Communication, Skin immunology, Mast Cells immunology, Serine Endopeptidases immunology, Stem Cell Factor immunology

Abstract

Background: The aim of this study was to investigate whether the secretory granules of human mast cells store stem cell factor (SCF). We also addressed the question whether mast cell chymase, a chymotrypsin-like protease, also present in the secretory granules of human mast cells cleaves SCF at the peptide bound between Phe 158 and Met159., Methods: The skin samples were obtained from patients with mastocytosis, undergoing skin biopsy for diagnostic purposes. Mast cells were isolated and purified from human lung parenchyma (human lung mast cells, HLMC) by countercurrent elutriation followed by discontinuous Percoll density gradient. SCF contents of human mast cells were assessed for immunoreactive SCF by ELISA. Western blot analysis of SCF and its cleavage products were performed with the MoAb anti-SCF 7H6. SCF and its proteolytic fragment were characterized by electrospray mass spectrometry (ES/MS)., Results: SCF is present in the secretory granules of human skin and lung mast cells. Immunoreactive SCF (iSCF) was detected in the cell lysates of HLMC, but not in basophils. iSCF was rapidly (3 min) released after challenge with anti-IgE, and iSCF in supernatants rapidly declined after 30 min. ES/MS analysis of rhSCF1-166 treated with recombinant human chymase showed a polypeptide of 17,977.1+/-0.6 Da and a minor component of 697.4+/-0.1 Da generated by specific cleavage at Phe159. SCF1-166 and SCF1-159 similarly activated HLMC and potentiated anti-IgE-induced activation of these cells. The cleavage product SCF160-166 had no effect on mast cells. Western blot analysis of supernatants of anti-IgE activated HLMC incubated for various intervals with rhSCF1-166 showed that rhSCF1-166 was converted to a faster-migrating form with a molecular weight compatible with SCF1-159 and to several SCF species., Conclusion: SCF is stored in human mast cell secretory granules and is immunologically released by mast cells. SCF1-166 is rapidly cleaved by chymase and other proteases to several SCF species. more...

Published

1999

10. New aspects of mast cell biology.

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Author

Dvorak AM

Subjects

Adult, Animals, Cell Degranulation, Cytoplasmic Granules metabolism, Cytoplasmic Granules ultrastructure, Female, Histamine metabolism, Histamine Release, Humans, Lipid Metabolism, Lipoproteins, LDL metabolism, Mast Cells immunology, Mast Cells ultrastructure, Mice, Microscopy, Immunoelectron, Organelles metabolism, Organelles ultrastructure, Phagocytosis, Prostaglandin-Endoperoxide Synthases metabolism, Rats, Tumor Necrosis Factor-alpha metabolism, Mast Cells physiology

Abstract

New sources of human and mouse mast cells, which were isolated from individual organs (i.e., lung, colon, synovium, skin, uterus, heart), developed from progenitors in vitro in the presence of stem cell factor and/or interleukin (IL)-3, or enriched from fetal or adult blood, spleen or bone marrow by cell sorting, have made possible new studies of the cell biology of mast cells. Advances resulting from these new mast cell sources as well as from new methods for labeling specific products in subcellular sites and structures in resting and functional mast cells are the subject of this review. Specific advances discussed are as follows: identification of an Fc epsilonRI+ c-kit- mouse basophil population from bone marrow and spleen that is associated with IL-4 production and an Fc epsilonRI- c-kit- granulated mouse mast cell progenitor in fetal blood; identification of hyperplasia and functional activation of human skin mast cells in vivo when exposed to recombinant stem cell factor and spontaneous degranulation in X-linked immunodeficient mouse mast cells; use of an enzyme-affinity-gold method to detect histamine in mature and immature human mast cell granules, in secretion and recovery of histamine during anaphylactic degranulation of human lung mast cells ex vivo, and in secretion of histamine in vivo by piecemeal degranulation of IL-4 transgenic mouse mast cells in inflammatory eye disease and of human gut mast cells in inflammatory bowel disease; use of immunogold methods to localize cyclooxygenase and tumor necrosis factor-alpha to subcellular structures in human and rat mast cells and to localize the Charcot-Leyden crystal protein in human basophils to aid in the identification of mast cells arising in mixed cellular populations; use of a low-density lipoprotein (LDL)-gold affinity method to demonstrate a rat mast cell granule-mediated uptake of LDL by macrophages in peritoneal fluid. more...

Published

1997

11. Ultrastructural detection of histamine in human mast cells developing from cord blood cells cultured with human or murine recombinant c-kit ligands.

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Author

Dvorak AM and Morgan ES

Subjects

Animals, Cell Differentiation drug effects, Cells, Cultured, Fetal Blood cytology, Humans, Immunohistochemistry, Mast Cells cytology, Mast Cells ultrastructure, Mice, Mice, Inbred BALB C, Recombinant Proteins, Fetal Blood drug effects, Histamine analysis, Mast Cells chemistry, Microscopy, Immunoelectron, Stem Cell Factor pharmacology

Abstract

Immature human mast cells, arising from cord blood mononuclear cells cultured in the presence of the c-kit ligand of human or murine origin, contain mixtures of morphologically immature and mature secretory granules. Use of a new cytochemical technique to localize histamine in ultrastructural samples (based on the affinity of the enzyme, histaminase, for its substrate, histamine) localized this amine to mature mast cell granules of all substructural patterns present, as well as to condensation foci appearing in immature cytoplasmic granules. This cytochemical evidence of histamine bound to condensation foci during granule building in developing mast cells is analogous to evidence obtained during granule recovery of degranulated human basophils and mast cells. more...

Published

1996

12. Spontaneous degranulation of cultured bone-marrow-derived immature mast cells from X-linked immunodeficient (Xid) mice.

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Author

Dvorak AM, Miura T, Letourneau L, Ishizaka T, and Kawakami T

Subjects

Animals, Cell Size, Cells, Cultured, Interleukin-3 pharmacology, Mast Cells ultrastructure, Mice, Mice, Inbred CBA, Mice, Inbred Strains, Mice, Mutant Strains, Microscopy, Electron, Recombinant Proteins pharmacology, Bone Marrow Cells, Cell Degranulation immunology, Immunocompromised Host genetics, Mast Cells physiology

Abstract

IgE-mediated, antigen-dependent stimulation of immature mouse mast cells cultured in IL-3-containing media produces secretion by granule exocytosis. Similar cultured mast cells were derived from X-linked immunodeficient (Xid) mice and examined by electron microscopy. In these cultures, Xid mast cells were also immature. In contrast to cultures obtained from control mice, 10-20% of the immature mast cells of Xid origin were undergoing secretion by granule extrusion in the absence of any secretogogue. Spontaneous secretion may be related to discordered tyrosine kinase function and/or signal transduction pathways in the Xid mouse. more...

Published

1996

13. Purification of mast cells with an improved nonsynchronous flow-through coil planet centrifuge.

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Author

Okada T, Metcalfe DD, and Ito Y

Subjects

Animals, Cell Degranulation, Female, Histamine Release, Male, Mast Cells physiology, Mast Cells ultrastructure, Mice, Mice, Inbred BALB C, Peritoneal Cavity cytology, Rats, Rats, Sprague-Dawley, Cell Separation instrumentation, Centrifugation, Density Gradient instrumentation, Mast Cells cytology

Abstract

A method for cell purification was designed without using high-density media which may impair membrane receptors. Rat and mouse mast cells were separated with an improved nonsynchronous flow-through coil planet centrifuge. Peritoneal cells were suspended at a concentration of 2-3x10(7) cells/ml in conditioned RPMI 1640, supplemented with 50% heat-inactivated FCS and 0.32% sodium citrate. In each separation 3 ml of cell suspension were loaded into the coiled column and elutriated at 4 degrees C. Several conditions, including the centrifugal force, revolution/rotation ratio, density of separation media, flow speed, and designs of both coiled column and flow tubes, were examined and optimized for mast cell purification. Rat mast cells were separated at the purity of 99.2%, with an average yield of 40% under sterile conditions. Nearly 90% pure mouse mast cells were harvested, despite a very low population of mast cells available in murine peritoneal cells. Purified cells were morphologically intact and discharged granules by exocytosis as indicated by electron-microscopic observations. The average histamine release with antigenic specificity was 34 and 61%, in passive sensitization in vitro and in vivo, respectively. Mast cells sensitized with mouse monoclonal IgE antibody released histamine, similar to cells sensitized with homologous antibody. This newly devised method of cell separation will be useful to purify biologically intact mast cells. more...

Published

1996

14. Tumor necrosis factor alpha immunoreactivity of rat peritoneal mast cell granules decreases during early secretion induced by compound 48/80: an ultrastructural immunogold morphometric analysis.

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Author

Beil WJ, Login GR, Aoki M, Lunardi LO, Morgan ES, Galli SJ, and Dvorak AM

Subjects

Animals, Cell Degranulation drug effects, Cytoplasmic Granules drug effects, Cytoplasmic Granules metabolism, Cytoplasmic Granules ultrastructure, Immunohistochemistry, In Vitro Techniques, Male, Mast Cells drug effects, Mast Cells ultrastructure, Microscopy, Immunoelectron, Peritoneal Cavity cytology, Rats, Rats, Sprague-Dawley, p-Methoxy-N-methylphenethylamine pharmacology, Mast Cells physiology, Tumor Necrosis Factor-alpha metabolism

Abstract

We used fast (seconds) and ultrafast (milliseconds) microwave energy-assisted chemical fixation protocols, postembedding immunogold staining, and a morphometric analysis to investigate the early morphological changes and the TNF-alpha immunoreactivity in the cytoplasmic granules of rat peritoneal mast cells that had been stimulated to secrete by exposure to compound 48/80. Exposure to compound 48/80 induced the development of increased numbers of cytoplasmic granules that exhibited decreased electron density; these granules often also appeared swollen. These granule alterations were accompanied by a significantly decreased proportion of granules that were positive for TNF-alpha immunoreactivity. We also calculated the density of TNF-alpha labeling/mu 2 in both dense (unaltered) and altered granules in specimens. TNF-alpha immunoreactivity was present in dense granules (regardless of whether or not the specimens had been stimulated with compound 48/80) and in cells that were fixed with either fast or ultrafast microwave energy. However, altered granules exhibited a decreased density of TNF-alpha label. These findings show that changes in the immunolocalization and/or density of TNF-alpha immunoreactivity occur very rapidly upon stimulation of rat peritoneal mast cells with compound 48/80. more...

Published

1996

15. Analysis of mast cell activation using diamine oxidase-gold enzyme-affinity ultrastructural cytochemistry.

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Author

Dvorak AM, Morgan ES, Monahan-Earley RA, Estrella P, Schleimer RP, Weller PF, Tepper RI, Lichtenstein LM, and Galli SJ

Subjects

Animals, Blepharitis pathology, Cytoplasmic Granules chemistry, Cytoplasmic Granules ultrastructure, Humans, Interleukin-4 genetics, Interleukin-4 physiology, Lung cytology, Mast Cells chemistry, Mast Cells ultrastructure, Mice, Mice, Transgenic, Microscopy, Electron, Tissue Fixation, Affinity Labels, Amine Oxidase (Copper-Containing), Exocytosis physiology, Gold, Histamine analysis, Histamine Release physiology, Mast Cells physiology

Abstract

We review a new technique--diamine oxidase (DAO)-gold ultrastructural enzyme-affinity labeling--which we developed to localize histamine in subcellular sites of mast cells. The DAO-gold method showed that isolated human lung mast cells contained abundant histamine in their cytoplasmic granules, a conclusion which was verified by a large number of specificity controls. We also studied mast-cell-rich eyelid lesions which developed in interleukin-4 transgenic mice. The DAO-gold method demonstrated histamine in the electron-dense granules of mast cells in these lesions, but little or no histamine was detected in the swollen, empty granules of mast cells undergoing piecemeal degranulation. This new enzyme-affinity-gold method has permitted the first ultrastructural localization of histamine in subcellular sites of routinely prepared electron microscopy samples. The method has also permitted the first morphological studies of histamine secretion in vivo and has demonstrated that such secretion can be associated with the ultrastructural changes of piecemeal degranulation. more...

Published

1995

16. Immunolocalization of stromelysin-related protein in murine mast cell granules.

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Author

Brownell E, Fiorentino L, Jolly G, Wolfe K, Kincaid S, Seperack P, and Visco D

Subjects

Animals, Antibodies, Monoclonal immunology, Bone Marrow Cells, Cells, Cultured, Extracellular Matrix metabolism, Humans, Immunoenzyme Techniques, Immunohistochemistry, Interleukin-3 pharmacology, Mast Cells drug effects, Mast Cells ultrastructure, Matrix Metalloproteinase 3, Mice, Microscopy, Immunoelectron, Species Specificity, Cytoplasmic Granules chemistry, Mast Cells chemistry, Metalloendopeptidases analysis, Metalloendopeptidases immunology

Published

1995

17. Influence of genetic and environmental factors on surface expression and occupancy of IgE receptors and on histamine releasability of mast cells.

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Author

Chen XJ and Enerbäck L

Subjects

Animals, Immunoglobulin E genetics, Male, Mast Cells ultrastructure, Rats, Rats, Inbred Strains, Rats, Inbred WKY, Rats, Sprague-Dawley, Receptors, IgE genetics, Species Specificity, Specific Pathogen-Free Organisms immunology, Histamine Release genetics, Immunoglobulin E immunology, Mast Cells immunology, Receptors, IgE biosynthesis

Abstract

The relationship between the IgE load on mast cells and their secretory capacity when challenged with anti-IgE was studied in peritoneal cells obtained from rats of three different strains, Hooded Lister (HL), Wistar Kyoto (WKY) and Sprague-Dawley (SD). IgE was determined cytofluorometrically after labelling with FITC-conjugated anti-IgE before and after the saturation of the IgE receptors to provide a measure of the surface expression of IgE receptors (number of receptors available for bindings) as well as the IgE occupancy of the receptors (native IgE content). The secretory capacity of the mast cells was examined in vitro in terms of histamine release as a function of anti-IgE concentration. Mast cells obtained from HL and WKY rats were found to carry significantly higher levels of IgE receptors and IgE than the mast cells of SD rats bred and raised under the same conventional laboratory conditions. The mast cells of SD rats kept under barrier-maintained conditions carried significantly less IgE than the mast cells obtained from SD rats kept under conventional conditions, but their IgE receptor levels were similar. The IgE-mediated histamine-releasing capacity of the mast cells, evaluated in terms of maximum release or of the slopes of regression lines (histamine release versus anti-IgE concentration), was positively correlated to the levels of native IgE and IgE receptors in the three strains of rat combined. The mast cells obtained from WKY rats showed the highest secretory capacity in the three strains of rat examined, significantly higher than the mast cells of HL rats, even though the latter displayed similar levels of IgE and IgE receptors.(ABSTRACT TRUNCATED AT 250 WORDS) more...

Published

1995

18. Fibroblasts determine the fate of Fc epsilon RI+ cell populations in vitro by selectively supporting the viability of mast cells while internalizing and degrading basophils.

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Author

Kirshenbaum AS, Goff JP, Albert JP, Kessler SW, and Metcalfe DD

Subjects

Basophils ultrastructure, Cell Count, Cells, Cultured, Chymases, Fibroblasts chemistry, Fibroblasts ultrastructure, Humans, Mast Cells ultrastructure, Phagocytosis, Serine Endopeptidases analysis, Tryptases, Basophils physiology, Fibroblasts physiology, Mast Cells physiology, Receptors, IgE physiology

Abstract

To determine the fate of Fc epsilon RI+ cells on fibroblasts in vitro, human bone marrow derived CD34+ cells were cultured in the presence of recombinant human interleukin 3 and recombinant human hematopoietic stem cell factor for 3 weeks, and Fc epsilon RI+ cells were purified by immunomagnetic selection. This enriched Fc epsilon RI+ cell population consisted of 92-94% basophils and 3-5% mast cells as determined by morphologic, immunohistochemical, and ultrastructural criteria. The Fc epsilon RI+ cells were then cocultured with 3T3 fibroblasts. Basophils decreased markedly by 1 week and were absent from cocultures by 2-3 weeks, while the mast cell numbers on the fibroblast monolayers remained constant. Ultrastructural examination of cocultures at 2 days demonstrated phagocytosis of basophils by fibroblasts. By 1 week, phagocytosed basophil membranes and granules gave fibroblasts the superficial appearance of mast cells by toluidine blue staining. Mast cells surviving in cocultures could be distinguished from granule-containing fibroblasts by IgE surface labeling and by ultrastructural demonstration of tryptase-positive granules. Thus, while mast cells remain viable in coculture with 3T3 fibroblasts, basophils do not survive and are internalized and degraded by the fibroblast monolayer. more...

Published

1994

19. In vitro culture of cardiac mast cells from mice experimentally infected with Trypanosoma cruzi.

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Author

Postan M, Correa R, Ferrans VJ, and Tarleton RL

Subjects

Animals, Cells, Cultured, Male, Mast Cells ultrastructure, Mice, Mice, Inbred C3H, Microscopy, Microscopy, Electron, Microscopy, Phase-Contrast, Myocardium ultrastructure, Chagas Disease pathology, Mast Cells pathology, Myocardium pathology

Abstract

In this study we describe a mast cell population obtained by in vitro culture of hearts of Trypanosoma-cruzi-infected mice. Heart tissue was placed in culture and observed daily for the efflux of cells. Mast cells appeared in the medium during the 1st week of culture in the area immediately surrounding the tissues and increased in numbers over time. The cells were identified as mast cells by electron microscopy and by positive staining of granules with Giemsa, toluidine blue, and berberine sulfate techniques. Histopathological analysis of the cultured heart fragments from infected mice showed numerous mast cells, located mostly in areas where the histologic structure was abnormal and surrounded by fibrous connective tissue. This is the first report on in situ proliferation and migration of mast cells form inflamed heart tissues. In situ grown mast cells might be useful in developing in vitro models to study the role of these cells in T. cruzi-induced and other myocardiopathies. more...

Published

1994

20. Histochemical and cytological characterizations of mucosal and connective tissue mast cells of Mongolian gerbils (Meriones unguiculatus).

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Author

Nawa Y, Horii Y, Okada M, and Arizono N

Subjects

Animals, Cell Degranulation drug effects, Chymases, Connective Tissue Cells, Gerbillinae, Glycosaminoglycans metabolism, Histocytochemistry, Intestinal Mucosa cytology, Jejunum cytology, Jejunum metabolism, Male, Mast Cells ultrastructure, Phenotype, Serine Endopeptidases metabolism, Skin cytology, Skin metabolism, Tongue cytology, Tongue metabolism, Tryptases, p-Methoxy-N-methylphenethylamine pharmacology, Connective Tissue metabolism, Intestinal Mucosa metabolism, Mast Cells cytology, Mast Cells metabolism

Abstract

Mast cells in jejunum, skin, and tongue of Mongolian gerbils (Meriones unguiculatus) were examined in terms of their histochemical, enzyme-histochemical, and ultrastructural properties. When glycosaminoglycans of mast cells in jejunum and tongue were characterized by measuring the critical electrolyte concentration, the salt concentration at which 50% of mast cells could be stained was > 1.0 M for those in the jejunum and also in the tongue, indicating that mast cells in both sites contained heparin. Enzyme-histochemical study revealed that mast cells in the jejunum of Mongolian gerbils were strongly positive for chymase and tryptase, whereas those in tongue and skin were essentially negative for both proteases. By electron microscopy, granular morphology and distribution of surface microfolds of mast cells in the jejunum were different from those in the ear skin. After in vivo stimulation with compound 48/80, however, mast cells in both sites showed remarkable degranulation. From these results, although Mongolian gerbils also have distinct mast cell subsets, their phenotypic properties are different from those of the previously known mast cell subsets of other animals. more...

Published

1994

21. Mast cells alter granular properties and spatial relation to nerve fibres in spondylitis of adjuvant-treated rats.

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Author

Imai S, Hukuda S, and Maeda T

Subjects

Animals, Cell Count, Cytoplasmic Granules ultrastructure, Disease Models, Animal, Freund's Adjuvant, Male, Rats, Rats, Wistar, Sacrococcygeal Region, Spondylitis etiology, Mast Cells ultrastructure, Nerve Fibers ultrastructure, Peripheral Nerves ultrastructure, Spondylitis pathology

Abstract

It has been long implicated that mast cells (MCs) have a close spatial relationship to the peripheral nerve fibres. In the present study, which used spondylitis of adjuvant-treated rats, we investigated the behaviour of MCs in relation to peripheral nerve fibres and other inflammatory cells. Rat MCs with staining properties like connective tissue MCs decreased in number as inflammation progressed. With additional electron microscopic studies it was possible to observe the sequence of changes in their granular ultrastructure during active inflammation. Thus, the decrement of MCs with staining properties like connective tissue MCs was attributable to the changes in their granular conformation. In contrast, enzyme histochemistry of nerve fibres indicated that the percentages of MCs which were distant from nerve fibres increased significantly during the early stage of inflammation (p < 0.01). We speculate that while other inflammatory cells infiltrate, MCs deviate actively form nerve fibres and release their granular content. more...

Published

1994

22. Treatment of secretory otitis media with local instillation of hydroxyzine.

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Author

Theoharides TC, Manolidis SS, Vliagoftis H, and Manolidis LS

Subjects

Child, Child, Preschool, Female, Histamine analysis, Humans, Hydroxyzine therapeutic use, Injections, Male, Mast Cells ultrastructure, Otitis Media with Effusion metabolism, Prednisolone administration & dosage, Single-Blind Method, Tympanic Membrane surgery, Hydroxyzine administration & dosage, Otitis Media with Effusion drug therapy

Abstract

The study is a preliminary single-blind, placebo- and prednisolone-controlled investigation of the treatment of 156 children with otitis media with effusion (secretory otitis media, SOM), ranging from 2 to 12 years. The protocol involved tympanotomy and placement of a ventilation tube (grommet), through which control or drug solutions were introduced. Other parameters and coexisting symptoms which could contribute to SOM were also examined. Patients were divided into 3 groups as follows: group A: control (normal saline, 2 ml); group B: prednisolone (25 mg in 2 ml); group C: hydroxyzine pamoate (10(-5) M in 2 ml). The results indicate that in those children treated with hydroxyzine, the rate of relapse was significantly reduced and so was the amount of histamine present in middle ear effusions. The effectiveness of hydroxyzine is discussed in the context of the pathophysiology of SOM, especially with respect to mast cells and their activation by allergic and nonallergic means. more...

Published

1994

23. Human and murine recombinant c-kit ligands support the development of human mast cells from umbilical cord blood cells: ultrastructural identification.

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Author

Dvorak AM, Mitsui H, and Ishizaka T

Subjects

3T3 Cells metabolism, Animals, Cell Division drug effects, Cells, Cultured, Fetal Blood cytology, Hematopoietic Cell Growth Factors metabolism, Humans, Mast Cells ultrastructure, Mice, Recombinant Proteins metabolism, Recombinant Proteins pharmacology, Stem Cell Factor, Hematopoietic Cell Growth Factors pharmacology, Mast Cells cytology

Abstract

The recently identified ligand for c-kit, a protooncogene encoded by the W locus in mice, is a member of the tyrosine kinase receptor family with growth factor activity for mouse mast cells. Mature human mast cells regularly develop from agranular precursors in cord blood in long-term cocultures of cord blood and murine fibroblasts. Since the c-kit ligand is a product of murine fibroblasts, we examined the growth effect of recombinant human c-kit ligand (stem cell factor), of recombinant murine c-kit ligand (mast cell growth factor), and of a partially purified fraction derived from mouse fibroblast culture supernatant on the mast cell lineage of humans by electron microscopy in 8-week cultures of cord blood cells. We found that immature mast cells which developed in cultures containing the recombinant ligand for c-kit of human or murine origin as well as the naturally occurring c-kit ligand in 3T3 fibroblast supernatants were identical. Thus, each of these sources of the c-kit ligand exerted identical effects on the ontogeny of human mast cells as they develop from their agranular precursors in cord blood. Full maturity of factor-supported mast cells did not occur. more...

Published

1993

24. Dermatitis characterized by mastocytosis at immunization sites in mast-cell-deficient W/Wv mice.

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Author

Theoharides TC, el-Mansoury M, Letourneau R, Boucher W, and Rozniecki JJ

Subjects

Animals, Cell Count, Dermatitis pathology, Disease, Encephalomyelitis, Autoimmune, Experimental immunology, Female, Histamine Release immunology, Mast Cells immunology, Mast Cells ultrastructure, Mastocytosis pathology, Mice, Mice, Inbred C57BL, Mice, Mutant Strains, Serotonin biosynthesis, Skin immunology, Skin ultrastructure, Dermatitis immunology, Immunization, Mast Cells drug effects, Mastocytosis immunology

Abstract

W/Wv mice have been extensively used as an important model to study the maturation/differentiation and pathophysiology of mast cells. These albino mice have been shown to have less than 1% of the mast cells found in the skin of their +/+ controls or other normal mice. Moreover, no mast cells are detected in other organs even though they apparently have an adequate number of mast cell precursors. Presumably, these precursors do not respond appropriately to microenvironmental growth factors, while 'normal' precursors from the +/+ controls of S1/S1d-deficient mice mature appropriately in the tissue microenvironment of the W/Wv mice. Female W/Wv mice and +/+ controls were immunized with allogeneic spinal cord homogenate in complete Freund's adjuvant and Mycobacterium tuberculosis in order to induce experimental allergic encephalomyelitis. All W/Wv mice developed extensive dermatitis with mastocytosis at the injection sites about 4 months after inoculation. Mast cells were identified by light microscopy following staining with toluidine blue and berberine sulfate as well as electron microscopy. They were also found to be functional since they secreted serotonin and histamine in response to either compound 48/80 or carbachol. The majority of these mast cells were, therefore, considered to be mature, connective tissue like, but many of them were in different stages of granule maturation as seen with electron microscopy. These findings imply that W/Wv mice may not always be appropriate as models of mast cell deficiency. Moreover, these results suggest that the 'defect' in W/Wv mast cell precursors can be overcome by factors produced during immunization and/or development of dermatitis. These findings may, therefore, help elucidate what regulates mast cell maturation/differentiation as well as their pathophysiology. more...

Published

1993

25. Supernormal histamine release and normal cytotoxic activity of beige (Chédiak-Higashi syndrome) rat mast cells with giant granules.

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Author

Jippo-Kanemoto T, Kasugai T, Yamatodani A, Ushio H, Mochizuki T, Tohya K, Kimura M, Nishimura M, and Kitamura Y

Subjects

Animals, Cell Degranulation, Immunity, Cellular, Mast Cells ultrastructure, Peritoneal Cavity cytology, Rats, Rats, Mutant Strains, Chediak-Higashi Syndrome physiopathology, Cytotoxicity, Immunologic, Histamine Release, Mast Cells physiology

Abstract

The beige rat is an animal model of the Chédiak-Higashi syndrome. Since mast cells can be easily purified from the peritoneal cavity of rats, we investigated the function of beige rat mast cells with giant granules by using quantitative methods. Beige and normal rat mast cells were sensitized with anti-dinitrophenol (DNP) IgE antibodies and stimulated by DNP conjugated with human serum albumin. The proportion of histamine released to total histamine was significantly greater in beige rat mast cells than in normal rat mast cells. Since the supernormal histamine release of beige rat mast cells was observed after treatment with 12-O-tetradecanoylphorbol 13-acetate, calcium ionophore A23187, substance P or compound 48/80, it appeared to be attributable to the enlargement in granules in beige rat mast cells. Spontaneous cytotoxic activity of mast cells was assayed by incubating purified mast cells with 51Cr-labelled WEHI-164 cells. Both beige and normal rat mast cells showed significant cytotoxic activity, but no significant difference was detectable between beige and normal rat mast cells. Even after IgE-mediated stimulation, no significant difference in cytotoxic activity was detectable between beige and normal rat mast cells either. Giant granules of beige rat mast cells did not appear to influence the cytotoxic activity of mast cells. more...

Published

1993

26. Steroid-induced depletion of mucosal mast cells and eosinophils in intestine of athymic nude rats.

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Author

Soda K, Kawabori S, Kanai N, Bienenstock J, and Perdue MH

Subjects

Animals, Cell Count drug effects, Eosinophils parasitology, Eosinophils ultrastructure, Intestinal Mucosa parasitology, Intestinal Mucosa ultrastructure, Male, Mast Cells parasitology, Mast Cells ultrastructure, Nippostrongylus immunology, Rats, Rats, Nude, Serine Endopeptidases analysis, Strongylida Infections enzymology, Strongylida Infections immunology, Strongylida Infections pathology, Dexamethasone pharmacology, Eosinophils drug effects, Intestinal Mucosa drug effects, Mast Cells drug effects

Abstract

In conventional rats, we have previously demonstrated that corticosteroid treatment caused macrophage engulfment and destruction of intestinal mucosal mast cells and eosinophils by 24 h without evidence of local tissue destruction, inflammation or secretion of rat mast cell protease II. As the growth and survival of these cells appear to be dependent on factors derived from T lymphocytes, we examined the response in congenitally athymic rnu/rnu rats and euthymic rnu/+ rats 35 days after parasitic infection. Rats were injected intraperitoneally with 1 mg dexamethasone and sections of jejunum were examined at 0, 7, 13 and 24 h. The numbers of mucosal mast cells significantly decreased in both groups and became less than 30% of the original values at 24 h. Tissue mast cell protease decreased similarly. However, protease in serum did not increase and there were no inflammatory changes at any time. The numbers of eosinophils also rapidly decreased and became less than 20% at 24 h in both rnu/rnu and rnu/+ rats. By electron microscopy, we saw granular changes (fusion) in mast cells and nuclear changes (apoptosis) in eosinophils by 7 h after corticosteroid in athymic rats. Macrophage engulfment of these cells was observed at 7 and 13 h. Our results suggest that inflammatory cell depletion by macrophages is not dependent on suppression of typical thymus-derived T lymphocytes, and may be due either to direct effects of steroids on the cells themselves, or indirectly upon cells other than T cells which normally supply maintenance and growth factors for them. more...

Published

1993

27. Mast cell abnormalities in the Chédiak-Higashi syndrome.

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Author

Galli SJ, Dvorak AM, and Hammel I

Subjects

Animals, Cytoplasmic Granules physiology, Histamine Release, Humans, Mast Cells ultrastructure, Membrane Fusion, Mice, Chediak-Higashi Syndrome physiopathology, Mast Cells physiology

Published

1993

28. Ultrastructural similarity between bat and human mast cell secretory granules.

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Author

Oliani SM, Vugman I, and Jamur MC

Subjects

Animals, Female, Humans, Male, Tongue cytology, Chiroptera anatomy & histology, Cytoplasmic Granules ultrastructure, Mast Cells ultrastructure

Abstract

Mast cells in the tongue of the bat (Artibeus lituratus) show a well-developed Golgi area and abundant mitochondria in the granule-free perinuclear cytoplasm. Rough endoplasmic reticulum profiles, free ribosomes, mitochondria, bundles of filaments and a great number of secretory granules are found throughout the remaining cytoplasm. The granules, of various shapes and sizes, are simple containing an electron-dense, homogeneous matrix, coarse particles or cylindrical scrolls, or combinations (cylindrical scrolls with either electron-dense, homogeneous matrix or coarse particle contents). Up to now, scroll-containing granules have been considered to be a unique feature of human mast cells. more...

Published

1993

29. Studies on the allergenicity of the amino-terminal epitope (Bet v I 23-38) from birch pollen allergen.

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Author

Vik H, Steinvåg SK, and Elsayed S

Subjects

Allergens isolation & purification, Amino Acid Sequence, Antigens, Plant, Cell Degranulation, Epitopes analysis, Humans, Lymphokines analysis, Mast Cells chemistry, Mast Cells ultrastructure, Molecular Sequence Data, Nasal Provocation Tests, Peptide Fragments chemical synthesis, Peptide Fragments chemistry, Plant Proteins isolation & purification, Pollen chemistry, Radioallergosorbent Test, Skin Tests, Allergens immunology, Epitopes immunology, Peptide Fragments immunology, Plant Proteins immunology, Pollen immunology, Prostatic Secretory Proteins

Abstract

An N-terminal peptide of the major allergen of birch (Bet v I 23-38) was selected for studying the activity of this segment on the basis of optimal hydrophilicity as it was tentatively suggested to be a surface exposed epitope. In addition two control peptides in the region 1-38 were similarly used for comparative assignment of the allergenicity. Peptide analogues from the amino acid terminal region, amino acid residues No. 23-38 of Bet v I, were synthesized by semiautomatic solid-phase peptide synthesis. In vitro and in vivo biological activity studies were performed on these analogous peptides. The IgE-binding capacity of the synthetic peptide 23-38 was examined using the following tests: specific IgE inhibition, skin prick test, nasal provocation and Prausnitz-Küstner inhibition. The results of these investigations suggested that the region 23-38 from the birch and hazel major allergen encompassed a single haptenic epitope. more...

Published

1993

30. Human gut mucosal mast cells: ultrastructural observations and anatomic variation in mast cell-nerve associations in vivo.

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Author

Dvorak AM, McLeod RS, Onderdonk AB, Monahan-Earley RA, Cullen JB, Antonioli DA, Morgan E, Blair JE, Estrella P, and Cisneros RL

Subjects

Adenocarcinoma ultrastructure, Colitis, Ulcerative pathology, Crohn Disease pathology, Humans, Intestinal Mucosa innervation, Intestinal Neoplasms ultrastructure, Microscopy, Electron, Precancerous Conditions ultrastructure, Intestinal Mucosa ultrastructure, Mast Cells ultrastructure

Abstract

One hundred and seventeen coded intestinal biopsy specimens were examined by electron microscopy. All surgical biopsies were obtained from uninvolved sites of patients with two inflammatory bowel diseases (ulcerative colitis or Crohn's disease) and from patients with preneoplastic and neoplastic diseases (adenocarcinoma, rectal polyp, familial polyposis). Biopsy sites included normal ileum, colon, and rectum as well as conventional ileostomies and continent pouches constructed from the ileum. The data reported here describe the ultrastructural anatomy of human gastrointestinal tract mucosal mast cells in vivo and their anatomic associations with enteric nerves. more...

Published

1992

31. Long-term cultured mouse mast cells: ultrastructure, histamine and leukotriene levels.

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Author

Haisa S, Chang HS, Bewtra AK, Hiratani M, Tamura N, Bewtra C, and Townley RG

Subjects

Animals, Bone Marrow Cells, Calcimycin pharmacology, Cell Degranulation, Cells, Cultured, Female, In Vitro Techniques, Mice, Mice, Inbred BALB C, Spleen cytology, Thymus Gland cytology, Time Factors, Histamine metabolism, Leukotrienes metabolism, Mast Cells metabolism, Mast Cells ultrastructure

Abstract

Interleukin 3 (IL3), dependent cells were obtained from bone marrow (9/10 experiments) and spleen cells (4/5 experiments), but not from the thymus. These cells were similar to mucosal mast cell toluidine blue staining and electron microscopy. They had heterogenous metachromatic granules, and some had large scroll-like structures. They also contained histamine (200-800 ng/10(6) cells) for the first 2-5 weeks, whose level diminished to less than 30 ng/10(6) cells by 10 weeks of culture. They also generated leukotriene (LT) C4/D4 (10-40 ng/10(6) cells) and LTB4 (2-5 ng/10(6) cells) for over 100 days of culture. In one experiment, bone marrow-derived mast cells after 150 days of culture began to produce an IL3-like substance and proliferated exponentially without exogenous IL3. more...

Published

1992

32. Ultrastructural evidence for piecemeal and anaphylactic degranulation of human gut mucosal mast cells in vivo.

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Author

Dvorak AM, McLeod RS, Onderdonk A, Monahan-Earley RA, Cullen JB, Antonioli DA, Morgan E, Blair JE, Estrella P, and Cisneros RL

Subjects

Basophils physiology, Basophils ultrastructure, Biopsy, Humans, Intestinal Mucosa innervation, Cell Degranulation, Gastrointestinal Diseases pathology, Intestinal Mucosa ultrastructure, Mast Cells physiology, Mast Cells ultrastructure

Abstract

One hundred and seventeen coded intestinal biopsies were examined by electron microscopy and evaluated for morphological evidence of mast cell and basophil secretion in situ. Sixty percent of the biopsies had evidence of secretion. Mast cell secretion was evident in control biopsies, many of which were obtained from uninvolved tissues of patients with inflammatory bowel disease. Biopsies of inflamed continent pouches from ulcerative colitis (UC) patients showed more mast cell secretion than noninflamed UC pouch biopsies. This evidence of mast cell secretion supports recent work that documents high constitutive levels of histamine in jejunal fluids of Crohn's disease patients and suggests a proinflammatory role for mast cells in inflammation associated with pouchitis. more...

Published

1992

33. Effect of inhaled platelet-activating factor on bronchial inflammation in atopic non-asthmatic subjects.

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Author

Lai CK, Djukanović R, Wilson JW, Wilson SJ, Britten KM, Howarth PH, and Holgate ST

Subjects

Administration, Inhalation, Adult, Asthma physiopathology, Bronchial Hyperreactivity physiopathology, Bronchial Provocation Tests, Bronchitis physiopathology, Cell Degranulation, Double-Blind Method, Eosinophils immunology, Eosinophils ultrastructure, Female, Humans, Male, Mast Cells immunology, Mast Cells ultrastructure, Methacholine Chloride administration & dosage, Placebos, Bronchial Hyperreactivity immunology, Bronchitis immunology, Platelet Activating Factor administration & dosage

Abstract

We have investigated the effect of inhaled platelet-activating factor (PAF) on bronchial mucosal inflammation in 6 atopic non-asthmatic subjects in a double-blind, placebo-controlled, randomised and crossover study. On 2 study periods at least 4 weeks apart, fiberoptic bronchoscopy was performed 24 h after inhalation of either 200 micrograms PAF or methacholine (control) to obtain endobronchial biopsies. Immunocytochemistry using antibodies for trypase (AA1) and eosinophil cationic protein (EG2) was performed to enumerate mast cells and eosinophils, respectively, in the bronchial submucosa. Median values of AA1+ cells and EG2+ cells did not differ significantly after inhalation of PAF or control (23.8 vs. 39 and 6 vs. 8/mm2, respectively, PAF vs. control, non-significant). Our findings suggest that within 24 h of inhaling a bronchoconstrictor dose of PAF, this agonist does not induce bronchial hyperresponsiveness or mucosal inflammation in atopic non-asthmatic subjects. However, because of the small number of subjects studied, these preliminary data should be interpreted with caution. more...

Published

1992