Your search keyword '"H. F. G. Heijnen"' showing total 6 results

1. Biochemical and immunohistochemical characteristics of CD62 and CD63 monoclonal antibodies

Author

H. K. Nieuwenhuis, H. F. G. Heijnen, M. J. Metzelaar, H.-J. Schuurman, and J J Sixma

Subjects

chemistry.chemical_classification, medicine.drug_class, Biology, Monoclonal antibody, Molecular biology, Epitope, Membrane protein, chemistry, Antigen, medicine, Immunohistochemistry, Platelet activation, Glycoprotein, Integral membrane protein

Abstract

During platelet secretion granule membrane glycoproteins are translocated to the plasma membrane. We report here the biochemical and immunohistochemical characterization of a panel of platelet-secretion-specific, CD62 and CD63 monoclonal antibodies (MoAb), which we raised to thrombin-activated platelets. The CD62 MoAb identify the α-granule membrane protein GMP-140, also designated platelet activation-dependent granule external membrane protein (PADGEM). The number of epitopes on thrombin-activated platelets ranged from 15000 to 20000. The CD63 MoAb recognize a 30–60 kDalton integral membrane protein of lysosomes. Due to its distinct localization, we have designated the CD63 antigen lysosome integral membrane protein, CD63 (LIMP-CD63). The number of epitopes on thrombin-activated platelets ranged from 9000 to 11000. Expression of GMP-140, a member of the Selectin family (also referred as the LEC-CAM family) of adhesion molecules, and LIMP-CD63 was examined on human spleen, thymus and lymph node by immunohistochemistry. Both GMP-140 and LIMP-CD63 showed a wide distribution in lymphoid tissues; vascular endothelial cells and tissue compartments that were readily accessible to blood-borne components were uniformly positive for GMP-140 and LIMP-CD63. Furthermore, LIMP-CD63 was expressed in polymorphonuclear granulocytes and macrophages.

Published

1992

2. Identification of a 33-Kd protein associated with the alpha-granule membrane (GMP-33) that is expressed on the surface of activated platelets

Author

M. J. Metzelaar, H. F. G. Heijnen, H. K. Nieuwenhuis, and J. J. Sixma

Subjects

biology, Immunology, Cell Biology, Hematology, Biochemistry, Molecular biology, Blot, Thrombin, Membrane, Alpha Granule, biology.protein, medicine, Platelet, Platelet activation, Antibody, Binding site, medicine.drug

Abstract

To identify antigens on the platelet plasma membrane that are exposed after activation, we developed a monoclonal antibody (MoAb) designated RUU-SP 1.77. The RUU-SP 1.77 antigen is present on the membrane of resting platelets at a basal level and is strongly expressed on the plasma membrane after thrombin activation. Freshly fixed platelets bound 4,150 +/- 1,935 (mean +/- SD) RUU-SP 1.77 molecules per platelet; on fixed thrombin-stimulated platelets the number of binding sites was upregulated to 19,050 +/- 5,120 (kd 4.5 +/- 0.8 nmol/L). MoAb RUU-SP 1.77 recognized a major protein of 33 Kd and a minor 28-Kd protein, both under nonreduced and reduced conditions. Immunoelectron microscopic studies showed the presence of the protein associated with the membrane of alpha-granules. Due to the localization associated with the alpha-granule membrane, we have designated it GMP-33 (granule membrane protein with a molecular weight of 33 Kd). Based on structural properties, we conclude that GMP-33 is a protein associated with the alpha-granule membrane that has not been described before.

Published

1992

3. Adhesive surface determines raft composition in platelets adhered under flow

Author

Marjolijn van Lier, F. Lee, G. Gorter, J‐W. N. Akkerman, S. Verhoef, H. F. G. Heijnen, Richard W. Farndale, and Yoshiko Ohno-Iwashita

Subjects

Blood Platelets, Platelet Aggregation, Surface Properties, Platelet Membrane Glycoproteins, Platelet membrane glycoprotein, Collagen receptor, Membrane Microdomains, Platelet Adhesiveness, Von Willebrand factor, hemic and lymphatic diseases, von Willebrand Factor, Humans, Platelet, Pseudopodia, Cells, Cultured, Membrane Glycoproteins, biology, Chemistry, Membrane Proteins, Hematology, Raft, Perfusion, Cholesterol, Biochemistry, Glycoprotein Ib, Platelet Glycoprotein GPIb-IX Complex, biology.protein, Biophysics, Collagen, GPVI, Rheology, Filopodia, Signal Transduction

Abstract

Adhesion to von Willebrand factor (VWF) induces platelet spreading, whereas adhesion to collagen induces aggregation. Here we report that cholesterol-rich domains (CRDs) or rafts play a critical role in clustering of receptors that control these responses. Platelets adhered to VWF and collagen show CRDs concentrated in filopodia which contain both the VWF receptor glycoprotein (GP) Ibalpha and the collagen receptor GPVI. Biochemical analysis of CRDs shows a threefold enrichment of GPIbalpha (but not GPVI) in VWF-adhered platelets and a fourfold enrichment of GPVI (but not GPIbalpha) in collagen-adhered platelets. Depletion of cholesterol (i) leaves the initial adhesion unchanged, (ii) inhibits spreading on VWF and aggregate formation on collagen, (iii) leaves filopodia formation intact, and (iv) reduces the localization in filopodia of GPIbalpha but not of GPVI. These data show that the adhesive substrate determines the composition of CRDs, and that cholesterol is crucial for redistribution of GPIbalpha but not of GPVI.

Published

2005

4. Recycling compartments and the internal vesicles of multivesicular bodies harbor most of the cholesterol found in the endocytic pathway

Author

W, Möbius, E, van Donselaar, Y, Ohno-Iwashita, Y, Shimada, H F G, Heijnen, J W, Slot, and H J, Geuze

Subjects

Kinetics, Cholesterol, Humans, Serum Albumin, Bovine, Endosomes, Gold, Lysosomes, Microscopy, Immunoelectron, Endocytosis, Cell Line, Transformed

Abstract

We employed our recently developed immuno-electron microscopic method (W. Möbius, Y. Ohno-Iwashita, E. G. van Donselaar, V. M. Oorschot, Y. Shimada, T. Fujimoto, H. F. Heijnen, H. J. Geuze and J. W. Slot, J Histochem Cytochem 2002; 50: 43-55) to analyze the distribution of cholesterol in the endocytic pathway of human B lymphocytes. We could distinguish 6 categories of endocytic compartments on the basis of morphology, BSA gold uptake kinetics and organelle marker analysis. Of all cholesterol detected in the endocytic pathway, we found 20% in the recycling tubulo-vesicles and 63% present in two types of multivesicular bodies. In the multivesicular bodies, most of the cholesterol was contained in the internal membrane vesicles, the precursors of exosomes secreted by B cells. Cholesterol was almost absent from lysosomes, that contained the bulk of the lipid bis(monoacylglycero)phosphate, also termed lysobisphosphatidic acid. Thus, cholesterol displays a highly differential distribution in the various membrane domains of the endocytic pathway.

Published

2003

5. Plasminogen activator inhibitor-1 released from activated platelets plays a key role in thrombolysis resistance. Studies with thrombi generated in the Chandler loop

Author

H. A. R. Stringer, Hans Pannekoek, H. F. G. Heijnen, P. van Swieten, Jan J. Sixma, and Other departments

Subjects

Blood Platelets, Pathology, medicine.medical_specialty, medicine.medical_treatment, Drug Resistance, Tissue plasminogen activator, Models, Biological, Fibrin, chemistry.chemical_compound, Fibrinolysis, Plasminogen Activator Inhibitor 1, medicine, Humans, Thrombolytic Therapy, Platelet activation, Thrombus, biology, Thrombosis, Thrombolysis, medicine.disease, Platelet Activation, Cell biology, Microscopy, Electron, chemistry, Plasminogen activator inhibitor-1, Tissue Plasminogen Activator, biology.protein, Cardiology and Cardiovascular Medicine, Plasminogen activator, medicine.drug

Abstract

To investigate the potential role of plasminogen activator inhibitor-1 (PAI-1), which is released from the alpha-granules of activated platelets, in thrombolysis resistance, we employed a model (the "Chandler loop") that mimics the formation of arterial thrombi in vivo and that can be manipulated in terms of rheological parameters and composition of blood cells. Light and electron microscopy revealed that the distribution of blood cells in Chandler thrombi is polarized, as it is in arterial thrombi, resulting in platelet-rich "white heads" and red blood cell-rich "red tails.". Resistance toward tissue-type plasminogen activator (TPA)-mediated thrombolysis parallels the presence of platelets that are fully activated in this system. We demonstrate that the PAI-1 released by the alpha-granules is preferentially retained within the thrombus and that the concentration of PAI-1 antigen is higher in the head than in the tail of the thrombus. The relative thrombolysis resistance of the heads of Chandler thrombi can be largely abolished by inclusion of an anti-PAI-1 monoclonal antibody that blocks that inhibitory activity of PAI-1 toward TPA. We propose that PAI-1, released from activated platelets, plays a key role in thrombolysis resistance and/or reocclusion after thrombolytic therapy. This is due to binding of PAI-1 to polymerized fibrin within the thrombus, followed by inhibition of TPA-mediated fibrinolysis.

Published

1994

6. Structure-function studies on human C4b-binding protein using monoclonal antibodies

Author

T. M. Hackeng, B. N. Bouma, H. F. G. Heijnen, M. Hessing, J. J. Sixma, and D. Kanters

Subjects

medicine.drug_class, Immunoelectron microscopy, Immunology, Blotting, Western, Enzyme-Linked Immunosorbent Assay, Biology, Monoclonal antibody, Binding, Competitive, Protein S, Antigen-Antibody Reactions, Epitopes, Structure-Activity Relationship, Western blot, medicine, Complement C4b, Immunology and Allergy, Humans, Binding site, Microscopy, Immunoelectron, Glycoproteins, Complement Inactivator Proteins, medicine.diagnostic_test, C4b-binding protein, Binding protein, Ligand binding assay, Antibodies, Monoclonal, Chromosome Mapping, Molecular biology, Receptors, Complement, Hybridoma technology, Binding Sites, Antibody, Carrier Proteins

Abstract

Human C4b-binding protein (C4BP) is a multimeric regulatory complement component interacting with vitamin K-dependent protein S and complement C4b. Using hybridoma technology, a panel of monoclonal antibodies (mAb) specific for intact human C4BP and its 160-kDa chymotryptic central core fragment were prepared to study the structure-function relationships of C4BP. By Western blot analysis and competition experiments, four distinct groups of mAb were identified and mapped on the C4BP molecule. By rotary shadowing, spider-like images of C4BP-antibody complexes were obtained and immunoelectron microscopy provided some information on the stoichiometry of the antibody-C4BP interaction. Certain antibodies interacted with C4BP molecules only at a ratio of 1:1. Others formed complexes of two or more antibodies bound to homologous sites on the C4BP molecule. Using an enzyme-linked immunosorbent sandwich assay for the measurement of the complex formation between protein S and C4BP, mAb against the central core and the disulfide-linked beta chain of C4BP were identified that inhibited the binding of protein S to C4BP. In a binding assay using 125I-labeled C4BP and solid-phase C4b, the inhibitory effect of one group of anti-C4BP mAb on the binding of C4BP to C4b was demonstrated.

Published

1991