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Featured researches published by Galli Sj.


Journal of Histochemistry and Cytochemistry | 1993

Ultrastructural immunogold localization of tumor necrosis factor-alpha to the matrix compartment of eosinophil secondary granules in patients with idiopathic hypereosinophilic syndrome.

Waltraud Judith Beil; Peter F. Weller; Tzizik Dm; Galli Sj; Ann M. Dvorak

Peripheral blood eosinophils from two normal donors and two patients with the hypereosinophilic syndrome (HES) were analyzed with a post-embedding immunogold method to detect the substructural location of tumor necrosis factor-alpha (TNF-alpha). In eosinophils of HES patients, TNF-alpha was localized to the matrix compartment of 64% of the specific secondary granules. Other structures in the HES eosinophils were unlabeled. No TNF-alpha was detected in eosinophils of normal donors. These studies document the first ultrastructural subcellular localization of any cytokine within the major population of secretory granules in human eosinophils and support other lines of evidence indicating that the expression of TNF-alpha may be greater in the eosinophils of HES patients than in those of normal donors.


International Archives of Allergy and Immunology | 1996

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

Waltraud Judith Beil; Gary R. Login; Mikako Aoki; Laurelúcia Orive Lunardi; Ellen S. Morgan; Galli Sj; Ann M. Dvorak

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.


Journal of Histochemistry and Cytochemistry | 1992

Immunocytochemical localization of histamine in secretory granules of rat peritoneal mast cells with conventional or rapid microwave fixation and an ultrastructural post-embedding immunogold technique.

Gary R. Login; Galli Sj; Ann M. Dvorak

We used a post-embedding immunogold labeling approach to define the fine-structural localization of histamine in rat peritoneal mast cells that were fixed using either standard aldehyde fixation or a fast microwave-aldehyde fixation method. Specimens were processed routinely for electron microscopy. Thin sections were exposed first to guinea pig antihistamine antiserum and then to gold-conjugated goat IgG directed against guinea pig IgG. By transmission electron microscopy, gold particles were localized to the matrix of cytoplasmic granules. Control sections treated with non-immune sera did not show labeling of mast cells. Adsorption of antihistamine antiserum with purified histamine or histamine bound to agarose showed a significant reduction (p less than 0.005) in granule staining. We also confirmed that our isolation procedures yielded functionally competent mast cells which released histamine when stimulated with sheep anti-rat IgE antiserum or with compound 48/80. These studies define the conditions of fixation for electron microscopy that are appropriate for the localization of histamine in the granule matrix of rat peritoneal mast cells.


Science | 1983

Tumor cells secrete a vascular permeability factor that promotes accumulation of ascites fluid

Donald R. Senger; Galli Sj; Ann M. Dvorak; Carole Perruzzi; Harvey Vs; Harold F. Dvorak


Journal of Experimental Medicine | 1989

Interleukin 3-dependent and -independent mast cells stimulated with IgE and antigen express multiple cytokines.

P R Burd; Rogers Hw; Gordon; C A Martin; Sundararajan Jayaraman; S D Wilson; Ann M. Dvorak; Galli Sj; Martin E. Dorf


Journal of Immunology | 1983

Lipid bodies: cytoplasmic organelles important to arachidonate metabolism in macrophages and mast cells.

Ann M. Dvorak; Harold F. Dvorak; S P Peters; E S Shulman; Donald W. MacGlashan; Kathryn Pyne; Harvey Vs; Galli Sj; L M Lichtenstein


Journal of Cell Biology | 1982

Mast cell clones: a model for the analysis of cellular maturation.

Galli Sj; Ann M. Dvorak; J A Marcum; Teruko Ishizaka; Gary J. Nabel; H Der Simonian; Kathryn Pyne; J M Goldin; R D Rosenberg; Harvey Cantor; Harold F. Dvorak


Journal of Experimental Medicine | 1979

Rejection of first-set skin allografts in man. the microvasculature is the critical target of the immune response.

Harold F. Dvorak; Martin C. Mihm; Ann M. Dvorak; B A Barnes; Eleanor J. Manseau; Galli Sj


Blood | 1982

Ultrastructural identification of the mouse basophil.

Ann M. Dvorak; Gary J. Nabel; Kathryn Pyne; Harvey Cantor; Harold F. Dvorak; Galli Sj


Federation proceedings | 1983

Basophil and mast cell degranulation: ultrastructural analysis of mechanisms of mediator release.

Ann M. Dvorak; Galli Sj; Schulman Es; L M Lichtenstein; Harold F. Dvorak

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Ann M. Dvorak

Beth Israel Deaconess Medical Center

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Harold F. Dvorak

Beth Israel Deaconess Medical Center

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Ellen S. Morgan

Beth Israel Deaconess Medical Center

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Kathryn Pyne

Beth Israel Deaconess Medical Center

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Hajime Tsunoo

National Institutes of Health

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