Your search keyword '"Zohar, Mishal"' showing total 56 results

1. Thrombotic Dysfibrinogenemia: Fibrinogen “Caracas V” Relation between Very Tight Fibrin Network and Defective Clot Degradability

Author

Marchi, Rita, Mirshahi, Shah Soltan, Soria, Claudine, Mirshahi, Manouchehr, Zohar, Mishal, Collet, Jean Philippe, de Bosch, Norma B., Arocha-Piñango, Carmen Luisa, and Soria, Jeannette

Published

2000

2. Engagement of the inhibitory receptor CD158a interrupts TCR signaling, preventing dynamic membrane reorganization in CTL/tumor cell interaction

Author

Salem Chouaib, Zohar Mishal, Nadia Guerra, Asma Gati, Frédérique Michel, Oreste Acuto, Anne Caignard, Catherine Gaudin, and B. Escudier

Subjects

Cell signaling, CD3, Immunology, Receptors, Antigen, T-Cell, chemical and pharmacologic phenomena, Biology, Biochemistry, Membrane Microdomains, Receptors, KIR, Tumor Cells, Cultured, Humans, Cytotoxic T cell, Phosphorylation, Receptors, Immunologic, Carcinoma, Renal Cell, Microscopy, Confocal, Cell Membrane, T-cell receptor, hemic and immune systems, Cell Biology, Hematology, Actin cytoskeleton, Kidney Neoplasms, Cell biology, Killer Cells, Natural, CTL, Receptors, KIR2DL1, biology.protein, Calcium, Signal transduction, CD8, T-Lymphocytes, Cytotoxic

Abstract

Renal cell carcinoma (RCC) infiltrating lymphocytes (TILs) express killer cell immunoglobulinlike receptors (KIRs) that inhibit the antitumor CD8+ T-cell lysis. In the present study, to better examine the functional consequences of KIR engagement on cytotoxic T lymphocyte (CTL)/tumor interaction, we have investigated the influence of KIR CD158a on early steps of T-cell activation. We show that coengagement of T-cell receptor (TCR) and CD158a by tumor cells inhibited tyrosine phosphorylation of early signaling proteins ZAP-70 and LAT, lipid raft coalescence, and TCR/CD3 accumulation at the CTL/tumor cell interface. In addition, the guanine exchange factor Vav was not phosphorylated, and no actin cytoskeleton rearrangement was observed. Our data indicate a role of KIR CD158a in the dynamic events induced by TCR triggering, preventing CTL membrane reorganization, and subsequent completion of CTL activation program. Accordingly, the expression of CD158 by TILs may favor tumor cell escape to the immune response.

Published

2016

3. Long-term incubation with IL-4 and IL-10 oppositely modifies procoagulant activity of monocytes and modulates the surface expression of tissue factor and tissue factor pathway inhibitor

Author

Marc Vasse, Bernard Lenormand, Zohar Mishal, Philippe Nguyen, J. Paysant, Claudine Soria, Jean-Pierre Vannier, and Pascale Cornillet-Lefebvre

Subjects

Cytoplasm, Time Factors, Lipopolysaccharide, Lipoproteins, Gene Expression, Enzyme-Linked Immunosorbent Assay, Biology, Monocytes, Thromboplastin, chemistry.chemical_compound, Tissue factor, Tissue factor pathway inhibitor, medicine, Humans, RNA, Messenger, Incubation, Cells, Cultured, Interleukin 4, Microscopy, Confocal, Dose-Response Relationship, Drug, Reverse Transcriptase Polymerase Chain Reaction, Monocyte, Antibodies, Monoclonal, Interleukin, Hematology, Molecular biology, Blood Coagulation Factors, Interleukin-10, Interleukin 10, medicine.anatomical_structure, chemistry, Biochemistry, Interleukin-4

Abstract

Summary Monocytes can be induced to express both tissue factor (TF) and its inhibitor, TF pathway inhibitor-1 (TFPI-1). A short incubation (

Published

2005

4. Scrg1, a novel protein of the CNS is targeted to the large dense-core vesicles in neuronal cells

Author

Françoise Dandoy-Dron, Bernadette Griffond, Michel Dron, Michael G. Tovey, and Zohar Mishal

Subjects

Central Nervous System, Signal peptide, DNA, Complementary, Blotting, Western, Molecular Sequence Data, Immunocytochemistry, Nerve Tissue Proteins, Biology, Synaptic vesicle, Antibodies, Synaptotagmin 1, Cell Line, Mice, Synaptotagmins, symbols.namesake, Chromogranins, Animals, Amino Acid Sequence, Microscopy, Immunoelectron, Peptide sequence, Secretory pathway, Neurons, Membrane Glycoproteins, General Neuroscience, Calcium-Binding Proteins, Proteins, Colocalization, Golgi apparatus, Immunohistochemistry, Molecular biology, Recombinant Proteins, Cell biology, symbols, Synaptic Vesicles

Abstract

Scrapie responsive gene one (Scrg1) is a novel transcript discovered through identification of the genes associated with or responsible for the neurodegenerative changes observed in transmissible spongiform encephalopathies. Scrg1 mRNA is distributed principally in the central nervous system and the cDNA sequence predicts a small cysteine-rich protein 98 amino acids in length, with a N-terminal signal peptide. In this study, we have generated antibodies against the predicted protein and revealed expression of a predominant immunoreactive protein of 10 kDa in mouse brain by Western blot analysis. We have established CAD neuronal cell lines stably expressing Scrg1 to determine its subcellular localization. Several lines of evidence show that the protein is targeted to dense-core vesicles in these cells. (i) Scrg1 is detected by immunocytochemistry as very punctate signals especially in the Golgi apparatus and tips of neurites, suggesting a vesicular localization for the protein. Moreover, Scrg1 exhibits a high degree of colocalization with secretogranin II, a dense-core vesicle marker and a very limited colocalization with markers for small synaptic vesicles. (ii) Scrg1 immunoreactivity is associated with large secretory granules/dense-core vesicles, as indicated by immuno-electron microscopy. (iii) Scrg1 is enriched in fractions of sucrose density gradient where synaptotagmin V, a dense-core vesicle-associated protein, is also enriched. The characteristic punctate immunostaining of Scrg1 is observed in N2A cells transfected with Scrg1 and for the endogenous protein in cultured primary neurons, attesting to the generality of the observations. Our findings strongly suggest that Scrg1 is associated with the secretory pathway of neuronal cells.

Published

2003

5. Fenofibrate inhibits angiogenesis in vitro and in vivo

Author

J. Varet, J.-V. Pille, L. Vincent, Hong Li, P. Mirshahi, Zohar Mishal, Paule Opolon, C. Soria, Jeannette Soria, and E. Legrand

Subjects

medicine.medical_specialty, Angiogenesis, Peroxisome proliferator-activated receptor, Apoptosis, In Vitro Techniques, Protein Serine-Threonine Kinases, Biology, Cell Line, Cellular and Molecular Neuroscience, Fenofibrate, In vivo, Proto-Oncogene Proteins, Internal medicine, medicine, Humans, Endothelium, Molecular Biology, Protein kinase B, Hypolipidemic Agents, Pharmacology, chemistry.chemical_classification, Neovascularization, Pathologic, Cell Cycle, Membrane Proteins, Dermis, Cell Biology, Actin cytoskeleton, Actins, Capillaries, Isoenzymes, Endothelial stem cell, Endocrinology, chemistry, Mechanism of action, Cyclooxygenase 2, Prostaglandin-Endoperoxide Synthases, Cancer research, Molecular Medicine, medicine.symptom, Proto-Oncogene Proteins c-akt, medicine.drug

Abstract

Fenofibrate, a peroxisome proliferator-activated receptor (PPAR)-alpha activator, used as a normolipidemic agent, is thought to offer additional beneficial effects in atherosclerosis. Since angiogenesis is involved in plaque progression, hemorrhage, and instability, the main causes of ischemic events, this study was designed to evaluate the action of fenofibrate on angiogenesis. Our results show that fenofibrate (i) inhibits endothelial cell proliferation induced by angiogenic factors, followed at high concentrations by an increase in apoptosis, (ii) inhibits endothelial cell migration in a healing wound model, (iii) inhibits capillary tube formation in vitro, and (iv) inhibits angiogenesis in vivo. Concerning the mechanism of action, the inhibition of endothelial cell migration by fenofibrate can be explained by a disorganization of the actin cytoskeleton. At the molecular level, fenofibrate markedly decreased basic fibroblast growth factor-induced Akt activation and cyclooxygenase 2 gene expression. This inhibition of angiogenesis could participate in the beneficial effect of fenofibrate in atherosclerosis.

Published

2003

6. Demonstration of the mineralocorticoid hormone receptor and action in human leukemic cell lines

Author

Zohar Mishal, C. Hecquet, C. Nicolas, M. Mirshahi, MK Agarwal, S.S. Mirshahi, and Nady Golestaneh

Subjects

Cancer Research, Blotting, Western, Population, Biology, Polymerase Chain Reaction, Mineralocorticoid receptor, Sense (molecular biology), Tumor Cells, Cultured, Animals, Humans, Amino Acid Sequence, education, Receptor, DNA Primers, G alpha subunit, education.field_of_study, Leukemia, Microscopy, Confocal, Base Sequence, Cell growth, Hematology, Immunohistochemistry, Molecular biology, Rats, Receptors, Mineralocorticoid, Oncology, Biochemistry, Polyclonal antibodies, Cell culture, biology.protein, hormones, hormone substitutes, and hormone antagonists

Abstract

We studied the expression of the mineralocorticoid receptor (MCR), and of the amiloride-sensitive sodium channel (ASSC) regulated by the MCR, in human leukemic cell lines. Cell extracts from TF1 (proerythroblastic), HEL (human erythroblastic leukemia) and U937 (myeloblastic) cell line were positive for the ASSC, as a 82 kDa band in Western blots developed with the aid of a polyclonal antibody raised against the peptide QGLGKGDKREEQGL, corresponding to the region 44-58 of the alpha subunit of the epithelial sodium channel (ENaC) cloned from rat colon, linked to KLH. The polyclonal antibody against the MCR revealed a single band of about 102 kDa in extracts from HEL and TF1 cells. The immunofluorescent labelling of the MCR in all cell lines showed a nucleocytoplasmic localization of the receptor but the ASSC was exclusively membrane-bound and these results were confirmed by confocal microscopy. The expression of the MCR in the HEL cells was evident as a predicted band of 843 bp (234 amino acids) in electrophoresis of the PCR product obtained after total RNA had been reverse transcribed and then amplified using the primers 5'-AGGCTACCACAGTCTCCCTG-3' and 5'-GCAGTGTAAAATCTCCAGTC-3' (sense and antisense, respectively). The ENaC was similarly evident with the aid of the primers 5'-CTGCCmATG GATGATGGT-3' (sense) and 5'-GTTCAGCTCGAAGAAGA-3' (antisense) as a predicted band of 520 bp. In both cases, 100% identity was observed between the sequences of the PCR products compared to those from known human sources. The multiplication of the HEL cells was influenced by antagonists (RU 26752, ZK 91587) targeted for specificity to the MCR and this was selectively reversed by the natural hormone aldosterone. These steroids also provoked chromatin condensation in the HEL population. These permit new and novel possibilities to understand the pathobiology of human leukemia and to delineate sodium-water homeostasis in nonepithelial cells.

Published

2000

7. Mapping the CD4 Binding Domain of gp17, a Glycoprotein Secreted from Seminal Vesicles and Breast Carcinomas

Author

Monica Autiero, Muriel Gaubin, Jean-Claude Mani, John Guardiola, Zohar Mishal, Stéphane Basmaciogullari, Claude Granier, Raphaël Culerrier, and Dominique Piatier-Tonneau

Subjects

Male, Metastatic breast, Recombinant Fusion Proteins, Molecular Sequence Data, Fluorescent Antibody Technique, Breast Neoplasms, Transfection, Biochemistry, Animals, Humans, Amino Acid Sequence, Apolipoproteins D, Glycoproteins, Cystic disease, chemistry.chemical_classification, Chemistry, Vesicle, Membrane Transport Proteins, Seminal Vesicles, Peptide Fragments, Neoplasm Proteins, Apolipoproteins, Immunoglobulin G, CD4 Antigens, COS Cells, Mutation, Cancer research, Tumor-associated glycoprotein 72, Carrier Proteins, Glycoprotein, Protein Binding, Binding domain

Abstract

gp17, a secretory CD4-binding factor isolated from the human seminal plasma, is identical to the gross cystic disease fluid protein-15, a specific marker for primary and metastatic breast tumors. We previously demonstrated that gp17 binds to CD4 with high affinity and strongly inhibits T lymphocyte apoptosis induced by sequential cross-linking of CD4 and T cell receptor (TCR). To further characterize the gp17/CD4 interaction and map the gp17 binding site, we produced a secreted form of recombinant gp17 fused to human IgG1 Fc, gp17-Ig. We showed that gp17-Ig exhibits a binding affinity for CD4 similar to that of native gp17. As no information about gp17 structure is presently available, 99 overlapping gp17 peptides were synthesized by the Spot method, which allowed the mapping of two CD4 binding regions. Alanine scanning of CD4-reactive peptides identified critical residues, selected for site-directed mutagenesis. Nine gp17-Ig mutants were generated and characterized. Three residues within the carboxy-terminal region were identified as the major binding domain to CD4. The Spot method combined with mutagenesis represents a refined approach to distinguish the contact residues from the ones contributing to the conformation of the CD4-binding domain.

Published

2000

8. Cell cycle-dependent distribution and specific inhibitory effect of vectorized antisense oligonucleotides in cell culture

Author

Zohar Mishal, Frédéric Subra, Marina Gottikh, Marc Lavignon, Claude Malvy, and Valerie Helin

Subjects

Genetic Vectors, Green Fluorescent Proteins, Cell Culture Techniques, Gene Expression, Biochemistry, Mice, Genes, Reporter, Animals, Humans, RNA, Messenger, Pharmacology, Reporter gene, Nuclease, Microscopy, Confocal, biology, Oligonucleotide, Cell Cycle, hemic and immune systems, 3T3 Cells, Oligonucleotides, Antisense, respiratory system, Cell cycle, Flow Cytometry, Molecular biology, Cell biology, Kinetics, Luminescent Proteins, Epidermoid carcinoma, Cell culture, Phosphodiester bond, biology.protein, Intracellular, HeLa Cells

Abstract

Factors limiting the use of antisense phosphodiester oligodeoxynucleotides (ODNs) as therapeutic agents are inefficient cellular uptake and intracellular transport to RNA target. To overcome these obstacles, ODN carriers have been developed, but the intracellular fate of ODNs is controversial and strongly depends on the means of vectorization. Polyamidoamine dendrimers are non-linear polycationic cascade polymers that are able to bind ODNs electrostatically. These complexes have been demonstrated to protect phosphodiester ODNs from nuclease degradation and also to increase their cellular uptake and pharmacological effectiveness. We studied the intracellular distribution of a fluorescein isothiocyanate-labeled ODN vectorized by a dendrimer vector and found that intracellular ODN distribution was dependent on the phase of the cell cycle, with a nuclear localization predominantly in the G2/M phase. In addition, in order to evaluate the relevance of ODN vectors in enhancing the inhibition of the targeted genes' expression, we developed a rapid screening system which measures the transient expression of two reporter genes, one used as target, the other as control and vice versa. This system was validated through investigating the effect of the dendrimer vector on ODN biological activity. Antisense sequence-specific inhibition of more than 70% of one reporter gene was obtained with a chimeric ODN containing four phosphorothioate groups, two at each end.

Published

1999

9. Development of a Rapid Screening System to Test Antisense ODN Modifications and Carriers

Author

Valerie Helin, Zohar Mishal, Claude Malvy, Marina Gottikh, Frédéric Subra, and Marc Lavignon

Subjects

Cholesterol derivatives, Reporter gene, Antisense oligodeoxynucleotides, Chemistry, Genetics, hemic and immune systems, Biological activity, respiratory system, Biochemistry, Molecular biology

Abstract

We developed a rapid screening system, using two reporter genes under the control of the same promoter, to identify the biological activity of modified or/and vectorized antisense oligodeoxynucleotides (ODNs). The ability of a dendrimeric structure and a monocationic cholesterol derivative to enhance ODN cellular uptake was previously investigated by fluorescence analysis. Then, the assay system was validated through investigating the effect of both vectors on antisense ODN efficiency.

Published

1999

10. Differential intracellular trafficking, secretion and endosomal localization of two IL-15 isoforms

Author

Cristina Andrei, Bruno Azzarone, Raffaella Meazza, Alessia Gaggero, Emanuela Zappia, Anna Rubartelli, Silvano Ferrini, and Zohar Mishal

Subjects

Signal peptide, Endosome, Green Fluorescent Proteins, Molecular Sequence Data, Immunology, Golgi Apparatus, CHO Cells, Endosomes, Biology, Endoplasmic Reticulum, Green fluorescent protein, symbols.namesake, chemistry.chemical_compound, Cricetinae, Animals, Humans, Immunology and Allergy, Secretion, Amino Acid Sequence, Interleukin-15, Microscopy, Confocal, Endoplasmic reticulum, Chinese hamster ovary cell, fungi, Biological Transport, Golgi apparatus, Brefeldin A, Molecular biology, Cell biology, Luminescent Proteins, chemistry, COS Cells, symbols

Abstract

To analyze the intracellular trafficking of two IL-15 isoforms bearing 48- or 21-amino acid leader peptides (L), we have generated cDNA encoding the two proteins fused at the C terminus with green fluorescent protein (GFP). Confocal microscopy analyses showed that, when transfected in CHO cells, 48L IL-15/GFP was localized in the Golgi apparatus and in early endosomes, while 21L IL-15/GFP was detectable only in the cytosol. The presence of 48L IL-15/GFP in endosomes was confirmed by enzyme-linked immunosorbent assay on endosome-enriched subcellular fractions. Exogenous IL-15 was bound and taken up in endosomes by untransfected CHO cells, indicating that endosomal localization was, at least in part, related to a receptor-mediated uptake. The 48L IL-15/GFP fusion protein was efficiently secreted by COS-7 or CHO cell transfectants, while IL-15 secretion was less efficient in transfectants expressing 21L IL-15/GFP or untagged 48L or 21L IL-15. Treatment with brefeldin A or with inhibitors of N-linked glycosylation further indicated that the 48L IL-15/GFP is secreted through the endoplasmic reticulum/Golgi pathway. Our data suggest a different trafficking of the two IL-15 isoforms and multiple mechanisms controlling IL-15 secretion.

Published

1999

11. Abnormal Fibrin Clot Architecture in Nephrotic Patients Is Related to Hypofibrinolysis: Influence of Plasma Biochemical Modifications

Author

A. Bensman, Claudine Soria, M. Mirshahi, Jeannette Soria, A. Baumelou, C. Lesty, J P Colle, Zohar Mishal, and J Peyne

Subjects

medicine.medical_specialty, biology, business.industry, medicine.medical_treatment, Albumin, Glomerulonephritis, Hematology, Fibrinogen, medicine.disease, Thrombosis, Fibrin, Endocrinology, Internal medicine, Immunology, Fibrinolysis, biology.protein, medicine, business, Nephrotic syndrome, Fibrinolytic agent, medicine.drug

Abstract

SummaryPorosity, viscoelasticity and morphological properties of plasma fibrin from 16 nephrotic patients and 16 healthy volunteers were compared. Nephrotic patients were characterized by formation of tight and rigid plasma fibrin gels which resulted in a slower rate of fibrin lysis studied either under pressure-driven permeation or diffusional transport of fibrinolytic agents. These latter findings indicated that both abnormal fibrin network conformation and abnormal fibrin fiber structure were involved in hypofibrinolysis. Albumin supplementation up to 40 mg/ml partially restored normal fibrin architecture and increased the rate of fibrinolysis in these patients. Multiparametric analysis showed that nephrotic patients were mainly characterized by a low plasma albumin level (R = -0.85), a low albumin to fibrinogen ratio (R = -0.89) and a high resistance to lysis (R = -0.82). High triglycerides level was the only plasma modification related to the slower fibrin lysis rate (R = -0.54). High fibrin rigidity (G’) was the only fibrin parameter simultaneously related to the nephrotic state (R = 0.75) and the lysis resistance (R = -0.71). After eliminating the effects of age, albumin and fibrinogen levels, low fibrin porosity (Ks) and low fiber mass-length ratio (μ) were the main features of the nephrotic state. These findings are discussed in relation to both the pathophysiology of thrombotic complications in nephrotic syndrome and their pharmacological prevention.

Published

1999

12. Mineralocorticoid hormone receptor and the epithelial sodium channel in a human leukemic cell line

Author

Nady Golestaneh, Zohar Mishal, C. Nicolas, M. Mirshahi, S.S. Mirshahi, and M. K. Agarwal

Subjects

Epithelial sodium channel, Molecular Sequence Data, Cell, Spironolactone, Sodium Channels, Endocrinology, Mineralocorticoid receptor, Tumor Cells, Cultured, medicine, Humans, Amino Acid Sequence, RNA, Messenger, Epithelial Sodium Channels, Receptor, Mineralocorticoid Receptor Antagonists, chemistry.chemical_classification, Dose-Response Relationship, Drug, Sequence Homology, Amino Acid, biology, Osmolar Concentration, General Medicine, Molecular biology, Chromatin, Amino acid, Blot, Receptors, Mineralocorticoid, medicine.anatomical_structure, chemistry, Cell culture, Polyclonal antibodies, biology.protein, Leukemia, Erythroblastic, Acute, Cell Division, hormones, hormone substitutes, and hormone antagonists

Abstract

A Cell extract from the HEL (human erythroblastic leukemia) cell line was positive for both the epithelial sodium channel (ENaC) and the mineralocorticoid receptor (MCR) as glycosylated 82-84 kDa bands, and a single 102 kDa band, respectively, in Western blots using polyclonal antibodies raised against these proteins. The immunofluorescent labeling of the MCR in all cell lines showed a nucleocytoplasmic localization of the receptor whereas the ENaC was exclusively membrane-bound. These results were confirmed by confocal microscopy. The expression of the MCR in HEL cells was evident as a predicted band of 843 bp (234 amino acids) after total RNA from HEL cells had been reverse transcribed and then amplified by PCR; the ENaC was similarly evident as a predicted band of 520 bp. In both cases, near 100% identity was observed between the deduced amino acid sequences of the PCR products and those from known human sources. The multiplication of HEL cells was influenced by antagonists (RU 26752, ZK 91587) targeted for specificity to the MCR and this was reversed by the natural hormone aldosterone. These steroids also provoked chromatin condensation in the HEL population.

Published

1998

13. Selective alteration of mitochondrial function by ditercalinium (NSC 335153), a DNA bisintercalating agent

Author

Evelyne Ségal-Bendirdjian, Dominique Coulaud, Zohar Mishal, Bernard P. Roques, Catherine Esnault, Stephen C. Brown, and Jean Bernard Le Pecq

Subjects

Carbonyl Cyanide m-Chlorophenyl Hydrazone, Cell Survival, Cellular respiration, Carbazoles, Antineoplastic Agents, Deoxyglucose, Mitochondrion, Biology, Biochemistry, Cell Line, Membrane Potentials, chemistry.chemical_compound, Adenosine Triphosphate, Oxygen Consumption, Cricetinae, Tumor Cells, Cultured, medicine, Animals, Leukemia L1210, Cytotoxicity, Pharmacology, Cytidine, DNA, Intracellular Membranes, Intercalating Agents, Uridine, Mitochondria, Cell biology, Microscopy, Electron, Microscopy, Fluorescence, Mechanism of action, chemistry, Toxicity, L1210 cells, medicine.symptom, Mitochondrial Swelling

Abstract

The bifunctional intercalator Ditercalinium (NSC 335153) demonstrates an anti-tumoral cytotoxicity markedly different from other intercalating agents. A delayed toxicity is observed in eucaryotic cells, both in vitro and in vivo , at drug concentrations far below those required to observe immediate toxic effects. Fluorescence microscopy demonstrates that Ditercalinium and the mit-ochondrial-staining fluorophore DiOC 2 (5) are concentrated in the same cellular organelles of L1210 cells. Electron microscopy of Ditercalinium-treated cells reveals extensive and progressive swelling of mitochondria, with no other ultrastructural changes observed. Ditercalinium uptake and toxicity are in part related to mitochondrial membrane potential. However, drug accumulation itself does not immediately alter the mitochondrial membrane potential. Cellular ATP pool levels and the rate of respiration fall progressively after drug treatment. Nucleotide pools in DC3F cells, measured between drug treatment and death, show marked drops in pyrimidine levels while purine nucleotide levels decline more slowly. Addition of uridine or cytidine partially rescues Ditercalinium-treated cells, while toxicity is increased in the presence of 2-deoxyglucose. The combined evidence indicates that the toxicity of Ditercalinium to murine leukemia cells (L1210) and Chinese Hamster lung cells (DC3F) is due to disruption of mitochondrial function.

Published

1990

14. Clot structure modification by fondaparinux and consequence on fibrinolysis: a new mechanism of antithrombotic activity

Author

Jeanne Yvonne Borg, Rémi Varin, Zohar Mishal, Gerald Kierzek, Claudine Soria, Jean-Pierre Vannier, David Sebaoun, Guy Simoneau, Pezhman Mirshahi, Jeannette Soria, and S.S. Mirshahi

Subjects

Protein Conformation, medicine.medical_treatment, Antithrombin III, Pharmacology, Fondaparinux, Fibrin, Fibrinolytic Agents, Polysaccharides, Antithrombotic, Fibrinolysis, medicine, Thrombus, Blood Coagulation, biology, Chemistry, Antithrombin, Thrombin, Hematology, Heparin, medicine.disease, Fondaparinux Sodium, Kinetics, Biochemistry, Tissue Plasminogen Activator, biology.protein, circulatory and respiratory physiology, medicine.drug

Abstract

SummaryFondaparinux is a synthetic pentasaccharide consisting of the minimal sequence of heparin which interacts with antithrombin (AT). It represents a new class of selective factor Xa inhibitors without any antithrombin activity. It has been shown to exhibit potent antithrombotic properties in clinical studies. However, the mechanism of its antithrombotic action has not yet been fully established. In the present study it was shown that fondaparinux, used at pharmacological concentration (500 ng/ml), rendered the clot more susceptible to fibrinolysis induced by t-PA: plasma fibrin clots formed in the presence of fondaparinux and perfused with t-PA were degraded at a faster rate than those formed in the absence of fondaparinux. This fibrinolytic activity of fondaparinux is mainly due to a modification of clot structure characterized by a loose fibrin conformation with less branched fibers and the presence of large pores in comparison to control clots which present a tighter conformation. The difference in fibrin structure was responsible for an increase in clot porosity leading to a better availability of t-PA to the fibrin network. It is related to the decrease in thrombin generation, in an AT-dependent pathway. It was also demonstrated that in the presence of exogenous thrombomodulin, the inhibition of TAFI activation by fondaparinux could contribute, to a lesser extent, to the increased thrombus lysis. The increase in t-PA induced thrombus lysis could contribute to the antithrombotic activity of fondaparinux.

Published

2007

15. Endostatin exhibits a direct antitumor effect in addition to its antiangiogenic activity in colon cancer cells

Author

Paule Opolon, Frank Griscelli, Fatima Dkhissi, Michel Perricaudet, He Lu, Claudine Soria, Hong Li, Patricia Khattar, Zohar Mishal, Hanfeng Liu, Hemostase, Endothelium, Angiogenese (UMR_S_553), Université Paris Diderot - Paris 7 (UPD7)-Institut National de la Santé et de la Recherche Médicale (INSERM), Micro-Environnement et Régulation Cellulaire Intégrée (MERCI), Université de Rouen Normandie (UNIROUEN), Normandie Université (NU)-Normandie Université (NU), Vectorologie et transfert de gènes (VTG / UMR8121), Université Paris-Sud - Paris 11 (UP11)-Institut Gustave Roussy (IGR)-Centre National de la Recherche Scientifique (CNRS), Fonctions cellulaires et moléculaires de l'appareil respiratoire et des vaisseaux, Institut Gustave Roussy (IGR)-Hôpital Henri Mondor-Institut National de la Santé et de la Recherche Médicale (INSERM)-Rhône-Poulenc Rorer Gencell-Centre National de la Recherche Scientifique (CNRS), Service de physiologie et d'explorations fonctionnelles [CHU Raymond-Poincaré], Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-Hôpital Raymond Poincaré [AP-HP], Centre de recherche en Myologie – U974 SU-INSERM, Institut National de la Santé et de la Recherche Médicale (INSERM)-Sorbonne Université (SU), Institut de Myologie, Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-Association française contre les myopathies (AFM-Téléthon)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), and IFR14

Subjects

Colorectal cancer, Genetic enhancement, [SDV]Life Sciences [q-bio], Genetic Vectors, Angiogenesis Inhibitors, Antineoplastic Agents, Apoptosis, Biology, law.invention, Adenoviridae, Mice, law, Genetics, medicine, Tumor Cells, Cultured, Animals, Humans, Molecular Biology, Mice, Inbred BALB C, Microscopy, Confocal, Neovascularization, Pathologic, Cell Cycle, Lewis lung carcinoma, Cancer, Integrin alphaV, medicine.disease, Flow Cytometry, Molecular biology, In vitro, Peptide Fragments, Endostatins, Endothelial stem cell, Colonic Neoplasms, Recombinant DNA, Molecular Medicine, Female, Collagen, Endothelium, Vascular, Endostatin, Cell Division, Integrin alpha5beta1

Abstract

International audience; Endostatin has been considered a highly specific inhibitor of endothelial cell proliferation and/or migration. To explore the use of endostatin in antiangiogenic gene therapy, we generated a recombinant adenovirus, AdEndo, carrying the gene for mouse endostatin. Injection of 10(9) PFU of AdEndo resulted in a low but significant suppression (25%) of preestablished tumor growth in murine models involving murine Lewis lung carcinoma (LLC) and human breast cancer MDA-MB-231 tumors. Greater anticancer activity was observed when the same dose of AdEndo was injected into two other preestablished murine models involving C51 murine colon cancer and HT29 human colon cancer (55 and 47% tumor growth reduction, respectively). In vitro, endostatin derived from AdEndo-infected MRC-5 fibroblasts inhibited the growth of C51 and HT29 cell lines (72 and 61%, respectively). The extent of this inhibition was comparable to that observed in endothelial cells: 75% for microcapillary endothelial cell line HMEC-1, 52% for human dermal microvascular endothelial cells, 46% for human umbilical vein endothelial cells, and 67% for calf pulmonary arterial endothelial cells. Both endothelial and colon cancer cells showed a clear increase in cell apoptosis (4- to 5-fold for endothelial cells and 5- to 10-fold for colon cancer cells) and an accumulation in the G(1) phase of the cell cycle. This antiproliferative activity was not observed in other tumor cell lines: LLC, MDA-MB-231, murine colon adenocarcinoma MC38, human prostate cancer cell line DU145, and human breast cancer cell line CAL51. Taken together, these results provide evidence that, in addition to its antiangiogenic activity, endostatin exerts a direct anticancer action that appears to be restricted to some tumor cell lines. Thus, endostatin could be used in some colon cancer treatments and its clinical efficacy would depend on the response of tumor cells themselves.

Published

2003

16. Processing of filamentous bacteriophage virions in antigen-presenting cells targets both HLA class I and class II peptide loading compartments

Author

Dominique Piatier-Tonneau, John Guardiola, Rossella Sartorius, Richard N. Perham, Muriel Gaubin, Piergiuseppe De Berardinis, Zohar Mishal, Cristina Fanutti, Giovanna Del Pozzo, and Antoine Durrbach

Subjects

Antigen presentation, Major histocompatibility complex, Epitope, MHC class I, Genetics, Cytotoxic T cell, Humans, Molecular Biology, Fluorescent Dyes, Antigen Presentation, B-Lymphocytes, Microscopy, Confocal, biology, Antigen processing, Histocompatibility Antigens Class I, Histocompatibility Antigens Class II, Cell Biology, General Medicine, biology.organism_classification, Filamentous bacteriophage fd, Virology, Filamentous bacteriophage, biology.protein, Fluorescein-5-isothiocyanate, Bacteriophage M13, T-Lymphocytes, Cytotoxic

Abstract

Virions of filamentous bacteriophage fd are capable of displaying multiple copies of peptide epitopes and generating powerful immune responses to them. To investigate the antigen processing mechanisms in human B cell lines used as antigen presenting cells, the major coat protein (pVIII) in intact virions was fluorescently labeled, and its localization in various intracellular compartments was followed using confocal microscopy. We show that the virions were taken up and processed to yield peptides that reach both the major histocompatibility complex (MHC) class II compartment and the endoplasmic reticulum. Moreover, when exposed to bacteriophages displaying a cytotoxic T lymphocyte (CTL) epitope from the reverse transcriptase of human immunodeficiency virus type-1 (HIV-1), B cells were lysed by specific cytotoxic lymphocytes. This confirms that filamentous bacteriophage virions are capable of being taken up and processed efficiently by MHC class I and class II pathways, even in nonprofessional antigen presenting cells. These remarkable features explain, at least in part, the unexpected ability of virions displaying foreign T-cell epitopes to prime strong T-helper-dependent CTL responses. These findings have important implications for the development of peptide-based vaccines, using filamentous bacteriophage virions as scaffolds.

Published

2003

17. Distribution of furamidine analogues in tumor cells: targeting of the nucleus or mitochondria depending on the amidine substitution

Author

Amélie, Lansiaux, Farial, Tanious, Zohar, Mishal, Laurent, Dassonneville, Arvind, Kumar, Chad E, Stephens, Qiyue, Hu, W David, Wilson, David W, Boykin, and Christian, Bailly

Subjects

Cell Nucleus, Male, Microscopy, Confocal, Base Sequence, Molecular Sequence Data, Melanoma, Experimental, Prostatic Neoplasms, Antineoplastic Agents, DNA, Neoplasm, Adenocarcinoma, Benzamidines, Mitochondria, Mice, Structure-Activity Relationship, Microscopy, Fluorescence, Neoplasms, Tumor Cells, Cultured, Animals, Humans, HT29 Cells, Cell Division

Abstract

Diphenylfuran diamidines represent an important class of DNA minor groove binders of high therapeutic interest as antiparasitic or antitumor agents depending on the compounds structures. To exert their cytotoxic action, the compounds must first get into the cell and reach the nuclear compartment where the main target, DNA, is located. The forces that drive the drugs into cell nuclei, as well as the influence of the molecular structures on the cell distribution, are not known. To address these issues, we took advantage of the fluorescence of the molecules to analyze their intracellular distribution profiles in tumor cells of different origins (B16 melanoma, MCF7 mammary adenocarcinoma, A549 lung carcinoma, HT29 colon carcinoma, LNCaP, and PC3 prostatic carcinoma) by epifluorescence and confocal microscopy. A homogeneous series of synthetic bis-substituted alkyl or phenyl amidine and reverse amidine derivatives of furamidine was used to dissect the molecular mechanisms that control the distribution of the drugs into the cytoplasm or the nucleus of the cells. The amidine (DB75) and the various N-alkyl derivatives were found to accumulate selectively in the cell nuclei. This is also the case for a guanidine derivative but not for the phenyl-substituted compound DB569, which essentially localizes in cytoplasmic granules. Similar cytoplasmic patterns were observed with a reverse amidine analogue and a pyridine-substituted compound indicating that the presence of aromatic rings on the terminal side chain is the limiting factor that restricts the uptake of the compounds in the nuclear compartment. The use of different organelle-selective fluorescent probes, such as JC-1 and chloromethyl-X-rosamine, both specific to mitochondria and neutral red considered as a lysosome-selective probe, suggests that DB569 preferentially accumulates in mitochondria. Competition experiments with the antitumor drug daunomycin reveal that the diphenylfurans are attracted into the nuclei by the DNA. The DNA minor groove-drug interactions provide the driving force that permits massive accumulation of the fluorescent molecules in the nuclei. The DNA binding properties of the diphenylfuran derivatives were investigated by DNase I footprinting and surface plasmon resonance biosensor experiments to measure sequence selectivity and binding affinities, respectively. Furamidine and its phenyl-substituted analogue that accumulate in the cell nuclei and mitochondria, respectively, share a common selectivity for AT sites and bind equally tightly to these sites. Therefore, it is possible to modulate the intracellular distribution of the furamidine derivatives without affecting their DNA binding and sequence recognition properties. The introduction of aromatic substituents on diphenylfuran diamidines represents a novel strategy to control the intracellular compartmentalization of these DNA binding agents and directs them to mitochondria. This drug design strategy may prove useful to trigger drug-induced apoptosis.

Published

2002

18. Treatment of cancer cells with methioninase produces DNA hypomethylation and increases DNA synthesis

Author

David, Machover, Jacqueline, Zittoun, Raphaël, Saffroy, Philippe, Broët, Stéphane, Giraudier, Thierry, Magnaldo, Emma, Goldschmidt, Brigitte, Debuire, Mireille, Orrico, Yuying, Tan, Zohar, Mishal, Odile, Chevallier, Carole, Tonetti, Hélène, Jouault, Ayhan, Ulusakarya, Marie-Laure, Tanguy, Gérard, Metzger, and Robert M, Hoffman

Subjects

Antimetabolites, Antineoplastic, Carbon-Sulfur Lyases, Kinetics, Leukemia, T-Cell, Dose-Response Relationship, Drug, Tumor Cells, Cultured, Humans, DNA, Neoplasm, DNA Methylation, Recombinant Proteins

Abstract

Methionine depletion in the human cell line CCRF-CEM through the action of recombinant methioninase (rMETase), a methionine-cleaving enzyme, was previously demonstrated to produce a strong cytotoxic synergistic effect with fluorouracil (FUra) throughout a broad range of concentrations of FUra and rMETase, including subcytotoxic levels of rMETase. Potentiation was associated with a decrease in free thymidylate synthase from preexisting levels. To further investigate the action of rMETase on CCRF-CEM cells, in the present study we explored the effects of rMETase as a single agent on DNA methylation levels and DNA synthesis, which may be changed as a result of deprivation of methionine. Cells treated with rMETase under subcytotoxic conditions contained significantly lower levels of genomic methylated DNA than did control cells, as demonstrated by incorporation of the methyl radical of [methyl-(3)H]S-adenosylmethionine in DNA and by use of methylation-sensitive arbitrarily primed PCR. DNA hypomethylation produced by rMETase was of similar magnitude as that produced with the DNA methyltransferase inhibitor 5-azacytidine. Cells exposed to rMETase synthesized significantly more DNA than did untreated cells. Incorporation of [6-3H]thymidine and [6-3H]2'-deoxyuridine in these cells was augmented over that in control by mean factors of 1.78 and 2.36, respectively. Increased 3H nucleoside incorporation resulted in greater numbers of nuclear grains as demonstrated by autoradiography. The increase in DNA synthesis induced by rMETase is likely to result from enhancement of DNA repair because it was not accompanied by differences in cell cycle phase distribution or in total DNA content as determined by flow cytometry. We hypothesize that potentiation of FUra cytotoxicity by rMETase may result from increased inhibition of thymidylate synthase, together with DNA hypomethylation and enhanced DNA repair that could be involved in cell responses to drug-induced damage.

Published

2002

19. Effects of Abciximab on the architecture of platelet-rich clots in patients with acute myocardial infarction undergoing primary coronary intervention

Author

Gérard Drobinski, Gilles Montalescot, C. Soria, Daniel Thomas, C. Lesty, P. Pinton, J.P. Collet, Zohar Mishal, Paul Barragan, Rémi Choussat, and J. Soria

Subjects

Blood Platelets, Male, medicine.medical_specialty, Platelet Aggregation, medicine.medical_treatment, Abciximab, Myocardial Infarction, Immunoglobulin Fab Fragments, Double-Blind Method, Physiology (medical), Angioplasty, Internal medicine, Fibrinolysis, medicine, Humans, Platelet activation, Myocardial infarction, Blood Coagulation, Aged, business.industry, Viscosity, Percutaneous coronary intervention, Antibodies, Monoclonal, Thrombolysis, medicine.disease, Treatment Outcome, Cardiology, Female, Cardiology and Cardiovascular Medicine, business, TIMI, Platelet Aggregation Inhibitors, medicine.drug

Abstract

Background —Abciximab plus aspirin improves the TIMI 3 flow rate of the infarct-related artery in patients treated with either percutaneous coronary intervention or thrombolysis. The present study investigated whether the reperfusion efficacy of abciximab relates to modifications of clot architecture in patients admitted for acute myocardial infarction (AMI). Methods and Results —A total of 23 AMI patients in the Abciximab before Direct angioplasty and stenting in Myocardial Infarction Regarding Acute and Long term follow-up (ADMIRAL) trial received, in a double-blind fashion, either abciximab (n=13) or placebo (n=10) before primary stenting. Viscoelastic (G′ in dyne/cm 2 ) and morphological (mean platelet aggregate surface area [SAG] in μm 2 ) indexes of ex vivo platelet-rich clots (PRC) were assessed in a double-blind fashion before and after the bolus administration of abciximab or placebo. G′ and SAG reflect the mechanical and morphological impact of activated platelets on the PRC fibrin network, respectively. Abciximab administration reduced G′ by 63% ( P =0.0001) and SAG by 65% ( P =0.0007), and no effect was seen in the placebo group. These abciximab-related changes increased fibrin exposure as a consequence of the platelet-aggregate surface reduction and may have improved endogenous fibrinolysis. These effects were identified in all patients, independent of previous heparin administration. Conclusions —Abciximab dramatically reduces platelet aggregate size and increases the fibrin accessibility of ex vivo PRC in AMI patients. These modifications could participate in the better coronary artery patency observed with abciximab.

Published

2001

20. Mineralocorticoid hormone signaling regulates the 'epithelial sodium channel' in fibroblasts from human cornea

Author

C. Nicolas, Nady Golestaneh, Massoud Mirshahi, Yves Pouliquen, S.S. Mirshahi, Françoise Dagonet, Christianne Hecquet, Karim C. Lounes, Zohar Mishal, and M.K. Agarwal

Subjects

Epithelial sodium channel, medicine.medical_specialty, genetic structures, Sodium, Cell, Molecular Sequence Data, chemistry.chemical_element, Biology, Sodium Channels, Cellular and Molecular Neuroscience, chemistry.chemical_compound, Mineralocorticoid receptor, Internal medicine, Cornea, Sequence Homology, Nucleic Acid, medicine, Humans, Aldosterone, DNA Primers, Ion Transport, Microscopy, Confocal, Base Sequence, Reverse Transcriptase Polymerase Chain Reaction, Sodium channel, Epithelium, Corneal, General Medicine, Fibroblasts, eye diseases, Sensory Systems, Ophthalmology, medicine.anatomical_structure, Endocrinology, Receptors, Mineralocorticoid, chemistry, RNA, sense organs, human activities, Hormone, Signal Transduction

Abstract

We investigated the regulation of sodium absorption by steroid hormones in embryologically diverse cells from the human eye. A cell extract from human corneal fibroblasts was positive for both the epithelial sodium channel (ENaC) and the mineralocorticoid receptor (MCR) as 82- to 85-kD and 102-kD bands, respectively, by the Western blot technique. In fluorescent, confocal and electron microscopy, the MCR was revealed as a nucleocytoplasmic protein, whereas the ENaC was almost exclusively membrane bound; both appeared aligned along actin filaments of corneal keratocytes, and both were widely colocalized in various cell types of human cornea in situ. Following reverse transcription and amplification of total RNA isolated from corneal fibroblasts, the ENaC and MCR genes in the PCR product were evident as predicted bands of 520 and 843 bp, respectively, whose sequence exhibited 100% identity with those from known human sources. The multiplication of corneal fibroblasts was influenced by both the MCR-specific antagonist RU 26752 and the natural hormone aldosterone, and these steroids also stimulated protein phosphorylation. In quantitative PCR, both the basal and aldosterone-induced levels of ENaC were diminished by the MCR-specific antagonist ZK 91587. Consequently, the ocular sodium channel appears to be regulated by steroid signalling in cells of diverse embryological origins, contrary to the existing notions where (a) this process would be limited exclusively to the epithelial cells and (b) ocular sodium transport would be regulated via the Na+-K+-ATPase in the basolateral membrane.

Published

2000

21. Altered natural killer cell differentiation in CD34+ progenitors from chronic myeloid leukemia patients

Author

Zohar Mishal, Nathalie Cambier, Bruno Azzarone, Julien Giron-Michel, Géraldine Carayol, Salem Chouaib, Luca Castagna, Anne Caignard, and Jean Bourhis

Subjects

Cancer Research, Cellular differentiation, Stem cell factor, Antigens, CD34, Biology, Natural killer cell differentiation, Natural killer cell, Cell Line, Leukemia, Myelogenous, Chronic, BCR-ABL Positive, Genetics, medicine, Tumor Cells, Cultured, Humans, Molecular Biology, Interleukin-15, Stem Cell Factor, Microscopy, Confocal, Receptors, Interleukin-15, Myeloid leukemia, Cell Differentiation, Receptors, Interleukin-2, eye diseases, Lymphocyte Subsets, Cell biology, Killer Cells, Natural, Haematopoiesis, medicine.anatomical_structure, Interleukin 15, Immunology, Stem cell, Cell Division

Abstract

IL-15 and SCF fail to induce NK differentiation and proliferation of CD34+ hematopoietic progenitors from chronic myeloid leukemia patients in contrast to normal stem cells although, both normal and leukemic CD34+ cells display comparable expression of c-kit or IL-15 receptor subunits. Interestingly, confocal microscopy analysis revealed that leukemic and most normal CD34+ cells produce and secrete IL-15, as shown by its trafficking through the Golgi apparatus and early endosomes. However, only leukemic progenitors express the membrane bound IL-15. Colocalization and internalization of IL-15Rbeta/gammac and IL-15Ralpha/gammac complexes indicated that IL-15 was specifically uptaken by leukemic progenitors. We also demonstrated that in both normal and leukemic progenitors, the signaling kinase Jak3 is constitutively pre-associated with the gammac chain. Anti-IL-15 neutralizing mAb treatment resulted in down-regulation of gammac chain and disruption of gammac/Jak3 interaction in normal but had no effect in leukemic progenitors. Our results suggest the existence in both normal and leukemic CD34+ cells of a constitutive production of a bioactive IL-15 that does not lead to NK differentiation and further indicate that membrane bound IL-15 and constitutive activation of gammac are hallmarks of leukemic progenitors. Oncogene (2000).

Published

2000

22. IL-15/IL-15R alpha intracellular trafficking in human cells and protection from apoptosis

Author

Bruno Azzarone, Francesco Indiveri, Zohar Mishal, Raffaele Pereno, Lorella Lanza, Silvano Ferrini, Claude Jasmin, Alessia Gaggero, Raffaella Meazza, and Marco Scudeletti

Subjects

Signal peptide, Gene isoform, medicine.medical_treatment, Apoptosis, CHO Cells, Biology, General Biochemistry, Genetics and Molecular Biology, History and Philosophy of Science, Cricetinae, medicine, Tumor Cells, Cultured, Animals, Humans, Protein Isoforms, Tissue Distribution, Interleukin-15, Microscopy, Confocal, Receptors, Interleukin-15, General Neuroscience, Proteins, Receptors, Interleukin-2, Intracellular Membranes, TNF Receptor-Associated Factor 2, Juxtacrine signalling, Molecular biology, Cell biology, Cytokine, Mechanism of action, Interleukin 15, medicine.symptom, Nuclear localization sequence, Intracellular

Abstract

IL-15 is an immunostimulatory cytokine sharing with IL-2 the IL-2R beta gamma complex. In vivo, IL-15 detection in synovial fluids has been associated with the development of rheumatoid arthritis. A debate exists as to whether IL-15 has the potential to be secreted in meaningful amounts or to act as a pericellular cytokine. Our data show (1) the presence of two IL-15 isoforms displaying signal peptides of different length and the capacity to be secreted restricted to the isoform bearing the longer one; (2) in cells expressing the two isoforms, the existence of different nuclear localization and intracellular trafficking of IL-15 and IL-15R alpha; and (3) an intercellular microcirculation of IL-15, not detectable with ELISA kits, but displaying a role as an anti-apoptotic factor able to induce the deflection of the TNFR associated factor 2 (TRAF) to IL-15R alpha. Our data point to a juxtacrine mechanism of action of IL-15 and suggest a role for IL-15/IL-15R alpha in the regulation of apoptosis.

Published

1999

23. IL-15 is produced by a subset of human melanomas, and is involved in the regulation of markers of melanoma progression through juxtacrine loops

Author

Cristina Musselli, Marco Scudeletti, Raffaele Pereno, Yassine Taoufik, Danièle Brouty-Boyé, Claude Jasmin, Francesco Indiveri, Christelle Doucet, Silvano Ferrini, Cathy Barzegar, Zohar Mishal, Jerome Ritz, Raffaella Meazza, Corinne Pottin-Clemenceau, and Bruno Azzarone

Subjects

Cancer Research, Human leukocyte antigen, Biology, Polymerase Chain Reaction, Exon, Genetics, medicine, Biomarkers, Tumor, Tumor Cells, Cultured, Humans, Secretion, Molecular Biology, Melanoma, Interleukin-15, Microscopy, Confocal, Receptors, Interleukin-15, Alternative splicing, Histocompatibility Antigens Class I, Receptors, Interleukin-2, medicine.disease, Flow Cytometry, Juxtacrine signalling, Cell biology, Culture Media, Interleukin 15, Cell culture, Immunology, Disease Progression, RNA

Abstract

IL-15 is a novel cytokine active through the IL-2R/betagamma. Since several human melanoma cell lines display functional IL-2Rs, we studied the IL-15/melanoma cells interactions. Ten out of 17 melanoma cell lines express the IL-15 transcript and four of them express levels of IL-15 mRNA similar to those detected in control activated monocytes. Nine out of ten cell lines also express two transcripts for the IL-15R alpha originated by the alternative splicing of exon'3'. Two melanoma cell lines, MELP and MELREO, derived from patients with rapidly progressive primary melanomas, co-express the two IL-15 transcripts, originated by alternative splicing of exon 'A'. Intracellular IL-15 protein was only detected in these two cells lines and it is mainly retained in the Endoplasmic Reticulum (ER). However, a small amount of IL-15 is also found in the Golgi apparatus and in the early endosomes, suggesting production and intercellular trafficking of endogenous IL-15 protein. Nevertheless, no biologically active IL-15 could be detected in the supernatant of all melanoma cells. The anti IL-15 blocking mAb M111 causes the up regulation of HLA Class I in dense MELP and MELREO cultures. These data suggest that IL-15 is probably active through juxtacrine loops negatively controlling HLA Class I molecules expression. These data offer, for the first time, a likely explanation to the controversial issue of IL-15 secretion and constitute a natural model for understanding IL-15 routing. Moreover, we identify a subset of melanoma cells producing IL-15, possibly involved in tumor escape mechanisms.

Published

1998

24. Defective cell migration in an ovarian cancer cell line is associated with impaired urokinase-induced tyrosine phosphorylation

Author

He Lu, Shah Sultan Mirshahi, A. Bernadou, Zohar Mishal, Eric Pujade-Lauraine, Claudine Soria, Jeannette Soria, Karim C Lounes, and Jean Bénard

Subjects

Glycosylphosphatidylinositols, Blotting, Western, Biophysics, Enzyme-Linked Immunosorbent Assay, Receptors, Cell Surface, Protein tyrosine phosphatase, Biochemistry, Receptor tyrosine kinase, Receptors, Urokinase Plasminogen Activator, Tyrosine phosphorylation, chemistry.chemical_compound, Ovarian cancer cell line, Structural Biology, Cell surface receptor, Cell Movement, Plasminogen Activator Inhibitor 1, Genetics, Tumor Cells, Cultured, Humans, Cell migration, Fibrinolysin, Urokinase, Phosphorylation, Phosphotyrosine, Molecular Biology, Ovarian Neoplasms, Microscopy, Confocal, biology, Cell Biology, Immunohistochemistry, Urokinase-Type Plasminogen Activator, Cell biology, Urokinase receptor, chemistry, biology.protein, Female, A431 cells, Tyrosine kinase, Platelet-derived growth factor receptor, Signal Transduction

Abstract

The urokinase receptor (u-PAR), a protein anchored to cell membrane by a glycosyl phosphatidylinositol, plays a central role in cancer cell invasion and metastasis by binding urokinase plasminogen activator (u-PA), thereby facilitating plasminogen activation. Plasmin can promote cell migration either directly or by activating metalloproteinases that degrade some of the components of the extra cellular matrix. However, the IGR-OV1-Adria cell line contains the u-PAR but does not migrate even in the presence of exogenous u-PA, although the parental IGR-OV1 cell line migrates normally in the presence of u-PA. We therefore investigated the role of cell signalling for u-PA induced cell locomotion. We show that cell migration induced by u-PA–u-PAR complex is always associated with tyrosine kinase activation for the following reasons: (1) the blockade of the u-PAR by a chimeric molecule (albumin-ATF) inhibits not only the u-PA-induced cell migration, but also the signalling in IGR-OV1 line; (2) the binding of u-PA to u-PAR on non-migrating IGR-OV1-Adria cells was not associated with tyrosine kinase activation; (3) the inhibition of tyrosine kinase also blocked cell migration of IGR-OV1. Therefore tyrosine kinase activation seems to be essential for the u-PA-induced cell locomotion possibly by the formation of a complex u-PAR–u-PA with a protein whose transmembrane domain can ensure cell signalling. Thus, IGR-OV1 and IGR-OV1-Adria cell lines represent a good model for the analysis of the mechanism of u-PA–u-PAR-induced cell locomotion.

Published

1997

25. Transient adhesion mediated by ligand-receptor interaction on surfaces of variable nanotopography

Author

Laurent Limozin, Zohar Mishal, Pierre-Henri Puech, Paolo Decuzzi, Philippe Robert, Francesco Gentile, Valentina Lo Schiavo, Pierre Bongrand, Lo Schiavo, Valentina, Robert, Philippe, Mishal, Zohar, Puech, Pierre Henri, Gentile, Francesco, Decuzzi, Paolo, Bongrand, Pierre, and Limozin, Laurent

Subjects

Materials Chemistry2506 Metals and Alloy, Materials science, Ligand, Kinetics, Cell adhesion, Leucocyte adhesion, Nanotopography, Bioengineering, Nanotechnology, Condensed Matter Physic, Surface finish, Condensed Matter Physics, Intercellular adhesion molecule, Biomaterial, Biophysic, Materials Chemistry, Biophysics, Nanomedicine, Molecule, Antigen-antibody, Electrical and Electronic Engineering, Molecular environment

Abstract

Surface microtopography and nanotopography have been shown to influence cell adhesion and function, including proliferation and differentiation, leading both to fundamental questions and practical applications in the field of biomaterials and nanomedicine. However, the mechanisms of how cells sense topography remain obscure. In this study, we measured directly the effect of nanotopography on the kinetics of association and dissociation of ligand–receptor bonds, which are critically involved in the first steps of cell adhesion. We designed models of biological functionalised surfaces with controlled roughness varying from 2 to 400 nm of root mean square, and controlled ligand density. Tests of transient adhesion of receptor–coated microspheres on these surfaces were performed, using a laminar flow chamber assay. We probed Intercellular Adhesion Molecule ICAM–1–anti–ICAM–1 bond adhesion kinetics in the single molecule limit on smooth and rough substrates. Frequency of adhesion did not exhibit any noticeable dependence on roughness parameter, except at high bead velocity. Detachment rate was also independent of roughness. Finally, leucocyte transient adhesion tests were performed on similar substrates, using variable activating incubating media. Here also, no strong effect of roughness was observed in these conditions. Results are rationalised in terms of the role of local geometry on the access of ligands to receptors.

Published

2013

26. Visualization of silver-enhanced reaction products from protein-and immuno-colloidal gold probes by laser scanning confocal microscopy in reflection mode

Author

Antonio Macho, Zohar Mishal, Hans K. Lorenzo, José Uriel, and Adrian W. de Feijter

Subjects

Antigens, Differentiation, T-Lymphocyte, Silver Staining, Histology, Microscope, Materials science, Laser scanning, Confocal, Nanotechnology, Gold Colloid, Lymphoma, T-Cell, law.invention, Silver stain, law, Antigens, CD, Tumor Cells, Cultured, Humans, Muscle, Skeletal, Molecular Biology, Cells, Cultured, Microscopy, Confocal, Scanning confocal electron microscopy, Cell Biology, General Medicine, Medical Laboratory Technology, Reflection (mathematics), Colloidal gold, Biophysics, alpha-Fetoproteins, Anatomy, General Agricultural and Biological Sciences

Abstract

We have employed a laser scanning confocal microscope in reflection mode to directly and indirectly visualize sites of deposition of silver-enhanced reaction products from colloidal gold probes. A direct approach was used for the localization of alpha-fetoprotein receptors in human myoblasts by incubating primary cultures with an alpha-fetoprotein-gold conjugate. For an indirect approach, cultured CEM cells, derived from a human T-lymphoma cell line, were incubated with a mouse monoclonal antibody to mature T-cells, followed by a gold-labelled antibody to mouse immunoglobulins. Multiple optical sections of each sample were collected by reflection laser scanning confocal microscopy and combined into three-dimensional renderings. A (non-confocal) transmission image was generated of each field for comparative purposes. The increasing use of reflection laser scanning confocal microscopy combined with colloidal gold conjugates as biological markers will probably be of considerable advantage in cytochemical analysis.

Published

1995

27. Pharmacological approaches of fibrin gel architecture modulation and thrombus degradation: its implication in atherogenesis and thromboembolism disease

Author

Manouchehr Mirshahi, Marc Vasse, Jean Philippe Collet, J.P. Caen, Claudine Soria, Jeannette Soria, and Zohar Mishal

Subjects

Pathology, medicine.medical_specialty, Arteriosclerosis, Disease, Fibrinogen, Fibrin, Pathogenesis, Thromboembolism, medicine, Image Processing, Computer-Assisted, Humans, Thrombus, Microscopy, Confocal, biology, business.industry, Heparin, Fibrinogens, Abnormal, Thrombosis, Hematology, medicine.disease, Afibrinogenemia, Atheroma, biology.protein, Cancer research, business, Gels, medicine.drug

Published

1994

28. Change in Lipid Composition and in Membrane Fluidity of Human Peripheral Blood Lymphocytes Undergoing Blastic Transformation

Author

José Uriel, A. Anel, José J. Aguilar, and Zohar Mishal

Subjects

Transformation (genetics), Membrane, Antigen, Chemistry, Lipid composition, Immunology, Lymphocyte activation, Membrane fluidity, sense organs, Fatty acid composition, skin and connective tissue diseases, Peripheral blood, Cell biology

Abstract

The process of lymphocyte activation which leads to proliferation is involved in the majority of immunological events. Although the early metabolic changes in response to specific antigens or mitogenic lectins are well studied, the mechanism, however, is not yet completely understood. The increase in cell size is the first morphological change that we can observe, because the cell diameter more than doubles. This increase is followed by the enhancement of the synthesis of membrane phospholipids and by the change in their fatty acid composition implicated deacylation-reacylation reaction (Shinitzky M.).

Published

1993

29. Serum levels and receptor expression of tumor necrosis factor-alpha following human allogeneic and autologous bone marrow transplantation

Author

ERIC ROBINET, AMAD IBRAHIM, ALEMSEGED TRUNEH, MAURICE OSTRONOFF, ZOHAR MISHAL, EDMILSON ZAMBON, FRANCOISE GAY, MARCEL HAYAT, JOSE-LUIS PICO, and SALEM CHOUAIB

Subjects

Transplantation, Immunoradiometric assay, Resuscitation, Pathology, medicine.medical_specialty, medicine.diagnostic_test, business.industry, Tumor Necrosis Factor-alpha, Receptor expression, Graft vs Host Disease, Endogeny, Receptors, Cell Surface, Immunofluorescence, Peripheral blood mononuclear cell, Transplantation, Autologous, Receptors, Tumor Necrosis Factor, medicine.anatomical_structure, Leukocytes, Mononuclear, Medicine, Humans, Transplantation, Homologous, Tumor necrosis factor alpha, Bone marrow, business, Bone Marrow Transplantation

Abstract

We have investigated tumor necrosis factor-alpha levels in serum samples of patients before and after allogenic (16 patients) or autologous (8 patients) bone marrow transplantation. A sensitive immunoradiometric assay for monitoring levels of endogenous tumor necrosis factor-alpha was used. The serum levels of tumor necrosis factor-alpha were found to be relatively low (ranging from less than 15 to 77 pg/ml). Among 13 patients having graft-versus-host disease following allogeneic bone marrow transplantation 8 patients did not have detectable tumor necrosis factor-alpha (less than 15 pg/ml) while 4 out of 8 patients undergoing autologous bone marrow transplantation had detectable tumor necrosis factor-alpha levels (15 pg/ml), indicating a lack of correlation between tumor necrosis factor-alpha serum levels and the occurrence of graft-versus-host disease. Because the tumor necrosis factor-alpha levels detected in patient sera could be regulated by TNF-receptor expression, the presence of TNF-receptor on patients' peripheral blood mononuclear cells was also studied using fluorescent liposome-conjugated tumor necrosis factor-alpha and immunofluorescence analysis. Our data indicate that peripheral blood mononuclear cells of some patients receiving either autologous or allogeneic bone marrow transplantation expressed significant levels of TNF-receptors, suggesting a lack of correlation between TNF-receptor expression and graft-versus-host disease development.

Published

1992

30. Uptake and Intracellular Distribution of Oligonucleotides Vectorized by a PAMAM Dendrimer

Author

Claude Malvy, Marina Gottikh, Marc Lavignon, Valerie Helin, Zohar Mishal, and Frédéric Subra

Subjects

Microscopy, Confocal, Oligonucleotide, Chemistry, Oligonucleotides, technology, industry, and agriculture, hemic and immune systems, 3T3 Cells, macromolecular substances, respiratory system, Biochemistry, Mice, PAMAM dendrimer, Phosphodiester bond, Polyamines, Genetics, Animals, Humans, Distribution (pharmacology), Fluorescein-5-isothiocyanate, Intracellular, HeLa Cells

Abstract

We studied the uptake and intracellular distribution of an FITC labelled phosphodiester oligodeoxynucleotide (ODN) vectorized by a dendrimeric structure in cell culture.

Published

1999

31. Quantification of alpha-fetoprotein and transferrin endocytosis by lymphoid cells using flow cytometry

Author

José Uriel, J.M. Torres, Zohar Mishal, Cristina Esteban, and José J. Aguilar

Subjects

Endosome, media_common.quotation_subject, T-Lymphocytes, Immunology, Biology, Endocytosis, Lymphocyte Activation, Flow cytometry, Cell Line, symbols.namesake, medicine, Extracellular, Immunology and Allergy, Humans, Lymphocytes, Phytohemagglutinins, Internalization, media_common, Fluorescent Dyes, chemistry.chemical_classification, medicine.diagnostic_test, Transferrin, Golgi apparatus, Flow Cytometry, Fluoresceins, Molecular biology, Kinetics, chemistry, Microscopy, Fluorescence, Isotope Labeling, symbols, alpha-Fetoproteins, Intracellular, Fluorescein-5-isothiocyanate, Thiocyanates

Abstract

Alpha-fetoprotein (AFP) and transferrin (Tf) are serum proteins actively internalized by many growing cells through specific cell surface receptors. The intracellular pathways of AFP and Tf are very similar: both proteins enter the cells via coated pits and receptosomes, move to tubular elements of the transreticular portion of the Golgi and are recycled back to the cell surface and extracellular medium in native form. In the present work, the capacity of human lymphoid cells to bind AFP and Tf at 4 degrees C and to endocytose them at 37 degrees C was quantified by flow cytometry analysis on a FACS 440 using fluoresceinated derivatives of these proteins. The results obtained show that binding and internalization of AFP and Tf by lymphoid cells are saturable processes at either 4 degrees C or 37 degrees C. The method developed permits direct quantitative measurement of molecules bound to the cell surface or present within the cell.

Published

1990

32. Defective uptake of alpha-fetoprotein (AFP) and transferrin (Tf) by PHA-activated peripheral blood lymphocytes from patients with AIDS and related syndromes

Author

José Uriel, Juan María Torres, Claude Jasmin, Vassilis Georgoulias, Zohar Mishal, Javier Naval, Robert Lowi, Y Lunardi-Iskandar, and Jorge Laborda

Subjects

chemistry.chemical_classification, Acquired Immunodeficiency Syndrome, medicine.diagnostic_test, T-Lymphocytes, Immunology, Transferrin, T lymphocyte, Biology, Cell sorting, Lymphocyte Activation, Peripheral blood mononuclear cell, Flow cytometry, Infectious Diseases, chemistry, AIDS-Related Complex, Virology, Immunopathology, medicine, Humans, alpha-Fetoproteins, Phytohemagglutinins, Alpha-fetoprotein, Receptor

Abstract

Serum alpha-fetoprotein (AFP) and transferrin (Tf) are actively endocytosed by many growing cells during ontogenic and neoplastic growth, but also by peripheral T lymphocytes upon mitogen activation. AFP and Tf uptake occurs through receptor-mediated endocytosis. The purpose of the present work was to assess whether the expression and functional activity of AFP and Tf receptors are impaired in mitogen-activated T cells from several groups of HIV-1 seropositive (HIV+) individuals. Forty HIV+ cases were studied, including 12 patients with AIDS, 12 with lymphoadenopathy syndrome (LAS), as well as 16 asymptomatic homosexuals (As). Quantification of AFP and Tf uptake was carried out by fluorescence-activated cell sorting (FACS) using fluoresceinated derivatives of these proteins. Compared with healthy blood donors, the three HIV-1 seropositive groups exhibited clear impairment in the ability of their peripheral blood mononuclear cells (PBMC) to internalize AFP and Tf. The decrease in mean values of AFP uptake correlates roughly with the severity of the clinical status. Although these observations need to be confirmed after a much wider study groups, the AFP-Tf-endocytosis assay presented here clearly reveals early defective functions of mitogen-responsive T cells in disease-free subjects and may provide the basis for a prognostic test. The pathophysiological implications of these facts are discussed in relation to the structural and/or metabolic activities of fatty acids and iron, the ligands carried by AFP and Tf, respectively.

Published

1990

33. Thrombotic Dysfibrinogenemia

Author

Marchi, Rita, primary, Mirshahi, Shah Soltan, additional, Soria, Claudine, additional, Mirshahi, Manouchehr, additional, Zohar, Mishal, additional, Collet, Jean Philippe, additional, de Bosch, Norma B., additional, Arocha-Piñango, Carmen Luisa, additional, and Soria, Jeannette, additional

Published

2000

34. 94. Pharmacological remodeling of platelet-rich clots architecture by ABCIXIMAB (C-7E3) may explain the mechanism of its curative antithrombotic effect

Author

C. Lesty, D. Thomas, Claudine Soria, J.P. Collet, Zohar Mishal, J. Soria, McMirshahi, and Gilles Montalescot

Subjects

medicine.medical_specialty, business.industry, Mechanism (biology), Antithrombotic, medicine, Abciximab, Platelet, Hematology, General Medicine, Pharmacology, business, Surgery, medicine.drug

Published

1998

35. 63. Fibrin assembly of the homozygous dysfibrinogenemia ???Fibrinogen Metz??? (A?? 16 Arg ??? Cys) depends solely on B-?? interaction

Author

J. Soria, Michael W. Mosesson, Claudine Soria, M. Mirshahi, J.P. Collet, Zohar Mishal, and S. S. Mirshahi

Subjects

medicine.medical_specialty, biology, Chemistry, Hematology, General Medicine, medicine.disease, Fibrin, Endocrinology, Biochemistry, Internal medicine, Fibrinogen Metz, medicine, biology.protein, Dysfibrinogenemia

Published

1998

36. 72. Dysfibrinogenemia Guarenas I associated with bleeding tendency despite a defective thrombus lysis related to a decreased network porosity

Author

Rita Marchi, S. Soltan Mirshahi, M. Mirshahi, J. Soria, J.P. Collet, Zohar Mishal, Claudine Soria, C. L. Arocha-Pifiango, and U. Lundberg

Subjects

Pathology, medicine.medical_specialty, Lysis, business.industry, medicine, Hematology, General Medicine, Thrombus, Dysfibrinogenemia, medicine.disease, business, Surgery

Published

1998

37. 73. Platelet interaction with fibrin depends upon fibrin physical properties. Consequences on fibrin rigidity

Author

M. Mirshahi, J.P. Collet, John W. Weisel, Zohar Mishal, Claudine Soria, S. S. Mirshahi, J. P. Caen, and J. Soria

Subjects

Rigidity (electromagnetism), biology, Chemistry, Biophysics, biology.protein, Platelet, Hematology, General Medicine, Fibrin

Published

1998

38. 87. Ex vivo fibrin architecture modulation

Author

Zohar Mishal, J. P. Caen, Claudine Soria, Jean-Philippe Collet, and Jeannette Soria

Subjects

Venous thrombosis, Pathology, medicine.medical_specialty, biology, business.industry, biology.protein, medicine, Hematology, General Medicine, medicine.disease, business, Ex vivo, Fibrin

Published

1998

39. The decrease in cell migration of a derived ovarian carcinoma cell line with defective urokinase production and normal urokinase receptor expression is not corrected by addition of urokinase: A possible explanation

Author

H. Lu, Claudine Soria, S.S. Mirshahi, J. Benard, A. Bernadou, E. Pujade-Lauraine, J. Soria, Zohar Mishal, and P. Burtin

Subjects

Urokinase receptor, Urokinase, medicine.medical_specialty, Endocrinology, Chemistry, Cell culture, Ovarian carcinoma, Internal medicine, medicine, Cancer research, Hematology, medicine.drug

Published

1994

40. Endostatin Exhibits a Direct Antitumor Effect in Addition to Its Antiangiogenic Activity in Colon Cancer Cells.

Author

Fatima Dkhissi, He Lu, Claudine Soria, Paule Opolon, Frank Griscelli, Hanfeng Liu, Patricia Khattar, Zohar Mishal, Michel Perricaudet, and Hong Li

Published

2003

41. QUANTIFICATION BY CYTOFLUOROMETRY OF GLUCOCORTICOID-INDUCED APOPTOSIS: STRUCTURE-ACTIVITY RELATIONSHIP

Author

Marc Pallardy, Zohar Mishal, Mallory Perrin-Wolff, and Claude Bohuon

Subjects

Apoptosis, medicine, Structure–activity relationship, Cell Biology, General Medicine, Biology, Glucocorticoid, medicine.drug, Cell biology

Published

1993

42. Effect of 7,12- dimethylbenz (A) anthracene (DMBA) on signal transduction following activation of human peripheral blood lymphocytes

Author

H. Lebree, Claude Bohuon, Zohar Mishal, and Marc Pallardy

Subjects

chemistry.chemical_compound, chemistry, 7,12-Dimethylbenz[a]anthracene, Immunology, Cancer research, DMBA, Cell Biology, General Medicine, Signal transduction, Biology, Peripheral blood

Published

1992

43. LETHAL GRAFT-VERSUS-HOST REACTION AGAINST NON-H-2 ANTIGENS.

Author

Bruley-Rosset, Martine, Pritchard, Linda L., Zohar, Mishal, and Halle-Pannenko, Olga

Published

1989

44. Determination of ultrastructural peroxidases and immunologic membrane markers in the diagnosis of acute leukemias

Author

Jacqueline Zittoun, Robert Zittoun, Jean Yves Perrot, C. Rosenfeld, Michèle Kayibanda, Zohar Mishal, Marie Claire Martyre, Jean Pierre Marie, and Claude Boucheix

Subjects

Adult, Male, Pathology, medicine.medical_specialty, Myeloid, Immunology, Biochemistry, Myelogenous, chemistry.chemical_compound, Antigen, DNA Nucleotidylexotransferase, hemic and lymphatic diseases, medicine, Humans, Aged, Acute leukemia, Leukemia, biology, business.industry, Cell Membrane, Cell Biology, Hematology, Middle Aged, medicine.disease, Leukemia, Lymphoid, Leukemia, Myeloid, Acute, Microscopy, Electron, medicine.anatomical_structure, chemistry, Terminal deoxynucleotidyl transferase, Peroxidases, Myeloperoxidase, Acute Disease, biology.protein, Female, Sudan Black B, business

Abstract

Detection of membrane markers and ultrastructural peroxidase activity was carried out on the blasts of 16 apparently nonmyeloid adult acute leukemias. These patients were selected from 73 adult leukemic patients by the negativity of their routine cytochemical myeloid markers: i.e., myeloperoxidase, chloresterase activity, and Sudan Black B staining. B and T acute lymphoid leukemias (ALL) were excluded from the study. After concurrent testing from human T lymphocyte antigen (HuTLA), common ALL antigen (cALL), la-like antigens, and peroxidase activity at the electron microscopic level (POEM), only two patients remained undifferentiated (cALL-, POEM-). The other cases were classified as following : 6 common ALL (cALL+, POEM-), 1 pre-T-ALL (cALL+, HuTLA+, POEM-), 5 very poorly differentiated acute myelogenous leukemia (AML) (cALL-, POEM+), and 2 mixed leukemias (cALL+, POEM+). Terminal deoxynucleotidyl transferase activity (TdT) was measured in 7 cases and was found to be present at high levels in 4 cases of cALL and in the 2 cases of acute undifferentiated leukemias (AUL): it was absent in two cases of AML. Cytogenetic analysis had showed that 2 of the cALLs, 3 of the AMLs, and the 2 mixed leukemias were PH1+. We conclude that POEM detection is useful in apparently nonmyeloid leukemias with negative immunologic lymphoid markers, and that the existence of a Ph1 chromosome should be investigated, particularly in the unusual case of mixed (lymphoid-myeloid) acute leukemia.

Published

1982

45. Expression of alpha-fetoprotein receptors by human T-lymphocytes during blastic transformation

Author

Javier Naval, Zohar Mishal, Miguel Calvo, José Uriel, Jorge Laborda, Juan María Torres, and Darracq N

Subjects

medicine.medical_specialty, Receptors, Peptide, T-Lymphocytes, media_common.quotation_subject, Immunology, Cell, Receptors, Cell Surface, Stimulation, Biology, Lymphocyte Activation, Peripheral blood mononuclear cell, Flow cytometry, Internal medicine, medicine, Humans, Phytohemagglutinins, Receptor, Internalization, Molecular Biology, Cells, Cultured, media_common, chemistry.chemical_classification, medicine.diagnostic_test, Transferrin, Flow Cytometry, Molecular biology, Kinetics, Endocrinology, medicine.anatomical_structure, Microscopy, Fluorescence, chemistry, alpha-Fetoproteins, Alpha-fetoprotein

Abstract

Alpha-fetoprotein (AFP) and transferrin (Tf) are actively internalized by many growing cells during ontogenic and neoplastic development, including human malignant T- and B-lymphoblastoid cells. Their internalization is, on the contrary, greatly diminished or absent in mature, non-proliferating elements. In the present work, peripheral blood mononuclear cells (PBMCs) and T-lymphocytes, harvested from normal human donors, were induced to blastic transformation with phytohemagglutinin (PHA) and their ability to uptake AFP and Tf was measured and compared with Tf uptake in the same conditions. The capacity of the cells to internalize both proteins was quantified by fluorescence activated cell sorter (FACS) using fluoresceinated derivatives of these proteins. The results obtained show a significant uptake of AFP by T-lymphocytes upon PHA stimulation. The values of AFP incorporation were similar for all the cells studied (PBMCs, T-cells and T4, T8 cell subsets). The time course of AFP uptake paralleled, under the same conditions, the uptake of Tf and the expression of IL2 receptors. AFP uptake increased rapidly from the zero time (resting T-cells) and reached a maximum around 72 hr after PHA activation. Scatchard analysis of kinetic data at 4°C revealed for Hu-AFP one single group of specific binding sites in PHA activated T-lymphocytes with a dissociation constant of 3.03 × 10−7M and around 88,000 sites/cell. There results strongly suggest the transitory expression of AFP receptors in T-lymphocytes during blastic transformation.

Published

1989

46. Comparison of inhibitory effect of galactose analogs on the binding and cytotoxicity of an anti-globotriaosylceramide monoclonal antibody coupled or not coupled to pokeweed antiviral protein

Author

Simone Junqua, Jean-Bernard Le Pecq, Pierre Wils, and Zohar Mishal

Subjects

Cytotoxicity, Immunologic, Immunology, Globotriaosylceramide, Ricin, Biology, Binding, Competitive, Glycosphingolipids, Epitope, Epitopes, Structure-Activity Relationship, chemistry.chemical_compound, Antigen, Antigens, Neoplasm, Immunotoxin, Animals, Humans, Immunology and Allergy, Cytotoxic T cell, Leukemia L1210, Cytotoxicity, N-Glycosyl Hydrolases, Plant Proteins, Globosides, Immunotoxins, Trihexosylceramides, Antibody-Dependent Cell Cytotoxicity, Antibodies, Monoclonal, Galactose, Complement System Proteins, Burkitt Lymphoma, Immunoglobulin M, chemistry, Biochemistry, Ribosome Inactivating Proteins, Type 1, biology.protein, Antibody, Hapten

Abstract

The results described here provided an example of a human IgM monoclonal antibody against a tumor-associated glycolipid and of the unusual properties of its corresponding immunotoxin (IT). The monoclonal antibody referred to as 38-13 has been previously described and reacted with the globotriaosylceramide [Gb3:Gal(alpha 1----4)-Gal(beta 1----4)-Glc(beta 1----1)ceramide] specifically expressed on surface membrane of Burkitt's lymphoma (BL) cells. An immunotoxin (38-13 IT) combined with the pokeweed antiviral protein (PAP) toxin via S-S bridges showed paradoxically a lower cytotoxic effect in BL Ramos cells than in non-BL cells such as leukemic mouse L1210 cells, while these cells appeared not to be involved by flow cytometric analysis and complement-dependent cytotoxicity. Consequently, the inhibitory effect of selective galactose analogs on the binding and the cytotoxicity of 38-13 antibody conjugated or not to PAP toxin was compared on BL and non-BL cells. Only the galactose blocked in alpha configuration provided a fine inhibition of 38-13 binding on BL Ramos cells and both alpha and beta-galactose allowed us to establish a clear distinction between the pathway entry of 38-13 IT in BL and non-BL cells; in close correlation with the 38-13 binding specificity the 38-13 IT cytotoxic effect in Ramos BL cells could also be prevented by alpha-Gal only, suggesting that this toxic action is probably mediated through the IT binding to Gb3 antigenic sites. In contrast, on apparently irrelevant L1210 cells, 38-13 IT showed a cytotoxic effect which was inhibited preferentially by lactose (Gal in beta configuration). It was discussed that IT binding alone to either antigenic sites which are inhibited by the hapten alpha-Gal, or nonspecific sites which can compete with the hapten beta-Gal is unable to induce efficient killing of cells. But cooperation of both bindings might give an attractive explanation of IT cytotoxic effect. It was concluded that the unexpected activity of 38-13 IT in non-BL cells probably could be mediated through an active macromolecular transport process which could implicate a beta-galactoside-binding protein (lectin).

Published

1987

47. Use of a monoclonal antibody (GA3) to demonstrate lineage restricted O- glycosylation on leukosialin during terminal erythroid differentiation

Author

MT Mitjavila, T Tursz, Françoise Farace, Zohar Mishal, Marie-Christine Dokhélar, William Vainchenker, Ali Bettaieb, N Kieffer, and J. Breton Gorius

Subjects

Glycosylation, Antibodies, Neoplasm, medicine.drug_class, Sialoglycoproteins, CD3, Immunology, Population, Neuraminidase, Monoclonal antibody, Biochemistry, Epitope, Epitopes, Mice, Antigen, Antigens, CD, Antigens, Neoplasm, hemic and lymphatic diseases, Tumor Cells, Cultured, medicine, Animals, Humans, Glycophorin, Erythropoiesis, education, education.field_of_study, Leukosialin, biology, Tunicamycin, Antibodies, Monoclonal, Cell Differentiation, Cell Biology, Hematology, Hematopoietic Stem Cells, Molecular biology, Cell culture, biology.protein, Leukemia, Erythroblastic, Acute

Abstract

A murine monoclonal antibody (GA3) obtained by immunizing mice with cells of the human erythroleukemic cell line K562 is shown to define a 105 kilodalton (kd) membrane antigen on K562 cells that is restricted within the hematopoietic system to the erythroid lineage and to a minor population of CD3, CD4 positive T lymphocytes. Cocapping studies and immunoprecipitation experiments performed with GA3 and L10, an anti- sialophorin monoclonal antibody reacting with leukosialin (Gp 105) on K562 cells, demonstrate that the antigen detected by GA3 on K562 cells is identical to leukosialin. Neuraminidase treatment but not tunicamycin treatment of K562 cells abolishes the expression of the GA3- epitope without affecting the L10-epitope thus providing evidence that terminal sialic acid present on O-linked oligosaccharide chains on Gp 105 is essential for the expression of the GA3-epitope. Further analysis by flow cytometry and immune panning experiments performed on bone marrow cells with GA3 or L10 demonstrate that, in contrast to L10, which reacts with all types of hematopoietic progenitors, the epitope recognized by GA3 is restricted to the erythroid lineage, and appears during erythroid differentiation before glycophorin A on the earliest morphologically recognizable erythroid precursor, the proerythroblast. Our results therefore suggest that O-linked oligosaccharides on leukosialin express lineage restricted and even maturation restricted antigenic structures that might serve as cell lineage specific markers.

Published

1988

48. Parallel induction of fibrinolysis and receptors for plasminogen and urokinase by interferon gamma on U937 cells

Author

C. Picot, Hong Li, A. Bernadou, M. Mirshahi, Zohar Mishal, E. Pujade, He Lu, Olivier F. Bertrand, J. Soria, Jean-Yves Perrot, Claudine Soria, Patricia Krief, and J.P. Caen

Subjects

medicine.medical_specialty, Cellular differentiation, medicine.medical_treatment, Biophysics, Receptors, Cell Surface, Biology, Biochemistry, Monocytes, Cell Line, Interferon-gamma, Plasminogen Activators, Interferon, Internal medicine, Fibrinolysis, medicine, Humans, Interferon gamma, Fibrinolysin, Molecular Biology, Urokinase, U937 cell, Plasminogen, hemic and immune systems, Cell Biology, Flow Cytometry, Urokinase-Type Plasminogen Activator, Kinetics, Endocrinology, Cell culture, Cancer research, Plasminogen activator, medicine.drug

Abstract

A new cell sorter technique was employed to study the role of interferon gamma (INF gamma) in fibrinolysis induced by U937 monocytic cells. INF-gamma induced the differentiation of U937 cells as evidenced by the appearance of CD 14 antigen on the cell surface. Scatchard analysis and dose response curves showed a parallel increase in the number of receptors on U937 cells capable of accepting exogenous plasminogen and urokinase (UPA) synthetized by differentiating U937 monocytic cells. This would favour an activation of plasminogen by UPA. This adds a new parameter in the regulation of cell-mediated fibrinolysis and may be important in a number of biological processes.

Published

1988

49. Expression of platelet glycoprotein Ib alpha in HEL cells

Author

Zohar Mishal, Nelly Kieffer, Najet Debili, William Vainchenker, A N Wicki, A Henri, J Breton-Gorius, Kenneth J. Clemetson, and Monique Titeux

Subjects

Peanut agglutinin, chemistry.chemical_classification, medicine.drug_class, Cell Biology, Tunicamycin, Biology, Platelet membrane glycoprotein, Monoclonal antibody, Biochemistry, Molecular biology, chemistry.chemical_compound, chemistry, Polyclonal antibodies, biology.protein, medicine, Antibody, Glycoprotein, Molecular Biology, G alpha subunit

Abstract

We have previously shown that platelet glycoprotein Ib is expressed in a minority of cells of the human leukemic cell line HEL (Tabilio, A., Rosa, J. P., Testa, U., Kieffer, N., Nurden, A. T., Del Canizo, M. C., Breton-Gorius, J., and Vainchenker, W. (1984) EMBO J. 3, 453-459). In this report, we have selected a stable HEL subclone with increased expression of glycoprotein (GP) Ib as assessed by 6 different monoclonal antibodies in order to investigate the biochemical characteristics of this glycoprotein. A single polypeptide chain of apparent Mr = 60,000 was precipitated under reducing and nonreducing conditions by a specific polyclonal anti-platelet glycocalicin antibody and two anti-GPIb alpha monoclonal antibodies (AN51 and AP1), both from surface-labeled and metabolically labeled HEL cells. We were unable to demonstrate the presence of a polypeptide corresponding to the beta subunit of GPIb or GPIX which is closely associated with GPIb. Competitive immunoprecipitation performed in the presence of an excess amount of cold platelet glycocalicin completely displaced the Mr = 60,000 polypeptide. Synthesis of N-linked oligosaccharide chains on this Mr = 60,000 polypeptide was inhibited by the antibiotic tunicamycin, and a shift of the apparent Mr from 60,000 to 48,000 was observed. O-Linked oligosaccharide chains identical to platelet GPIb hexasaccharides were deficient or incomplete since no peanut agglutinin binding to the Mr = 60,000 polypeptide was observed after neuraminidase treatment of HEL cells. Thus, our results provide evidence that the Mr = 60,000 polypeptide expressed on the surface membrane of HEL cells is closely related to platelet GPIb and corresponds to an incompletely or abnormally O-glycosylated GPIb alpha subunit.

Published

1986

50. LETHAL GRAFTVERSUS-HOST REACTION AGAINST NONH-2 ANTIGENS

Author

BRULEY-ROSSET, MARTINE, PRITCHARD, LINDA L., ZOHAR, MISHAL, and HALLE-PANNENKO, OLGA

Published

1989