Your search keyword '"Sabido O"' showing total 90 results

51. Cytostatic factor proteins are present in male meiotic cells and beta-nerve growth factor increases mos levels in rat late spermatocytes.

Author

Perrard MH, Chassaing E, Montillet G, Sabido O, and Durand P

Subjects

Animals, Cyclin E metabolism, Cyclin-Dependent Kinase 2 metabolism, Cytoplasm metabolism, F-Box Proteins metabolism, Male, Rats, Rats, Sprague-Dawley, Meiosis, Nerve Growth Factor metabolism, Proto-Oncogene Proteins c-mos metabolism, Sertoli Cells metabolism, Spermatids metabolism, Spermatocytes metabolism

Abstract

Background: In co-cultures of pachytene spermatocytes with Sertoli cells, beta-NGF regulates the second meiotic division by blocking secondary spermatocytes in metaphase (metaphase II), and thereby lowers round spermatid formation. In vertebrates, mature oocytes are arrested at metaphase II until fertilization, because of the presence of cytostatic factor (CSF) in their cytoplasm. By analogy, we hypothesized the presence of CSF in male germ cells., Methodology/principal Findings: We show here, that Mos, Emi2, cyclin E and Cdk2, the four proteins of CSF, and their respective mRNAs, are present in male rat meiotic cells; this was assessed by using Western blotting, immunocytochemistry and reverse transcriptase PCR. We measured the relative cellular levels of Mos, Emi2, Cyclin E and Cdk2 in the meiotic cells by flow cytometry and found that the four proteins increased throughout the first meiotic prophase, reaching their highest levels in middle to late pachytene spermatocytes, then decreased following the meiotic divisions. In co-cultures of pachytene spermatocytes with Sertoli cells, beta-NGF increased the number of metaphases II, while enhancing Mos and Emi2 levels in middle to late pachytene spermatocytes, pachytene spermatocytes in division and secondary spermatocytes., Conclusion/significance: Our results suggest that CSF is not restricted to the oocyte. In addition, they reinforce the view that NGF, by enhancing Mos in late spermatocytes, is one of the intra-testicular factors which adjusts the number of round spermatids that can be supported by Sertoli cells.

Published

2009

52. Control of mitochondrial biogenesis, ROS level, and cytosolic Ca2+ concentration during the cell cycle and the onset of differentiation in L6E9 myoblasts.

Author

Jahnke VE, Sabido O, and Freyssenet D

Subjects

Animals, Calcium Signaling physiology, Calmodulin metabolism, Cell Cycle physiology, Cell Differentiation physiology, Cytosol metabolism, Hydrogen Peroxide metabolism, Membrane Potential, Mitochondrial physiology, NFATC Transcription Factors metabolism, Phosphorylation physiology, Rats, Calcium metabolism, Mitochondria physiology, Myoblasts, Skeletal cytology, Myoblasts, Skeletal metabolism, Reactive Oxygen Species metabolism

Abstract

Mitochondria can sense signals linked to changes in energy demand to affect nuclear gene expression. This retrograde signaling pathway is presumed to be involved in the regulation of myoblast proliferation and differentiation. We have investigated the regulation of mitochondrial biogenesis and production of putative retrograde signaling agents [hydrogen peroxide (H(2)O(2)) and Ca(2+)] during the cell cycle and the onset of differentiation in L6E9 muscle cells. The biosynthesis of cardiolipin and mitochondrial proteins was mainly achieved in S phase, whereas the expression of mitochondrial biogenesis factors [peroxisome proliferator-activated receptor (PPAR)-alpha, PPAR-delta, and neuronal nitric oxide synthase 1] was regularly increased from G(1) to G(2)M phase. In agreement with the increase in mitochondrial membrane potential, mitochondria in S and G(2)M phases have a significantly higher H(2)O(2) level when compared with G(1) phase. By contrast, the onset of differentiation was characterized by a marked reduction in mitochondrial protein expression and mitochondrial H(2)O(2) level. The capacity of mitochondria to release Ca(2+) in response to a metabolic challenge was significantly decreased at the onset of differentiation. Finally, an increase in calmodulin expression in S and G(2)M phases and a transitory increase in phosphorylated nuclear factor of activated T cells (NFAT) c3 in S phase was observed. NFATc3 phosphorylation was markedly decreased at the onset of differentiation. Our data point to functional links between the control of mitochondrial biogenesis and the regulation of the level of retrograde signaling agents during the cell cycle and the onset of differentiation in L6E9 muscle cells.

Published

2009

53. Could 99mTc-glucarate be used to evaluate tumour necrosis? In vitro and in vivo studies in leukaemic tumour cell line U937.

Author

Perek N, Sabido O, Le Jeune N, Prevot N, Vergnon JM, Clotagatide A, and Dubois F

Subjects

Animals, Antineoplastic Agents, Phytogenic therapeutic use, Apoptosis, Cell Survival, Etoposide therapeutic use, Humans, Lymphoma, Large B-Cell, Diffuse drug therapy, Mice, Mice, Nude, Necrosis, Neoplasm Transplantation, Radionuclide Imaging, Radiopharmaceuticals, Transplantation, Heterologous, U937 Cells, Glucaric Acid analogs & derivatives, Lymphoma, Large B-Cell, Diffuse diagnostic imaging, Lymphoma, Large B-Cell, Diffuse pathology, Organotechnetium Compounds

Abstract

Purpose: The aim of this study was to determine whether (99m)Tc-glucarate ((99m)Tc-GLA) is a powerful and discriminant tumour necrosis marker., Materials and Methods: The induction of apoptosis and secondary necrosis (by a chemotherapeutic agent) and necrosis (by intense hyperthermia) was studied on an in vitro and in vivo leukaemic cell line model (U937). The percentage of apoptosis/necrosis in vitro was determined by flow cytometry after staining cells with annexin-V-fluorescein/propidium iodide. The uptake of (99m)Tc-GLA was studied after treatments that produce an optimal of necrosis cells or apoptotic cells. Three populations of interest: viable, apoptotic and necrotic cells were sorted by flow cytometry. The uptake and the intracellular distribution of (99m)Tc-GLA on each population have been studied. We also investigated the influence of necrosis on (99m)Tc-GLA uptake in a model of U937 xenografts in nude mice., Results: The accumulation of (99m)Tc-GLA in untreated and apoptotic cells was lower than in necrotic cells. Cell sorting discriminated each cellular population and showed a 14% accumulation in necrotic cells and no more than a 3% in apoptotic cells. In apoptotic and viable cells, (99m)Tc-GLA is distributed between the cytosolic/membrane and the nucleus fractions. In necrotic cells, (99m)Tc-GLA is mainly found in the nucleus fraction. In vivo investigations showed a higher (99m)Tc-GLA uptake in necrotic tumour than in apoptotic and control ones., Conclusions: (99m)Tc-GLA may be a useful agent to specifically evaluate tumour necrosis and may be helpful for the follow-up of patients with cancer.

Published

2008

54. Meiotic progression of rat spermatocytes requires mitogen-activated protein kinases of Sertoli cells and close contacts between the germ cells and the Sertoli cells.

Author

Godet M, Sabido O, Gilleron J, and Durand P

Subjects

Aging physiology, Animals, Coculture Techniques, Enzyme Activation, Fluorescent Antibody Technique, Indirect, Fluorescent Dyes metabolism, Immunohistochemistry, Male, Rats, Rats, Sprague-Dawley, Rhodamines metabolism, Sertoli Cells physiology, Meiosis physiology, Mitogen-Activated Protein Kinases physiology, Sertoli Cells enzymology, Spermatocytes cytology, Spermatocytes enzymology

Abstract

Progression of germ cells through meiosis is regulated by phosphorylation events. We previously showed the key role of cyclin dependent kinases in meiotic divisions of rat spermatocytes co-cultured with Sertoli cells (SC). In the present study, we used the same culture system to address the role of mitogen-activated protein kinases (MAPKs) in meiotic progression. Phosphorylated ERK1/2 were detected in vivo and in freshly isolated SC and in pachytene spermatocytes (PS) as early as 3 h after seeding on SC. The yield of the two meiotic divisions and the percentage of highly MPM-2-labeled pachytene and secondary spermatocytes (SII) were decreased in co-cultures treated with U0126, an inhibitor of the ERK-activating kinases, MEK1/2. Pre-incubation of PS with U0126 resulted in a reduced number of in vitro formed round spermatids without modifying the number of SII or the MPM-2 labeling of PS or SII. Conversely, pre-treatment of SC with U0126 led to a decrease in the percentage of highly MPM-2-labeled PS associated with a decreased number of SII and round spermatids. These results show that meiotic progression of spermatocytes is dependent on SC-activated MAPKs. In addition, high MPM-2 labeling was not acquired by PS cultured alone in Sertoli cell conditioned media, indicating a specific need for cell-cell contact between germ cells and SC.

Published

2008

55. Glial cell-line-derived neurotropic factor and its receptors are expressed by germinal and somatic cells of the rat testis.

Author

Fouchécourt S, Godet M, Sabido O, and Durand P

Subjects

Animals, Blotting, Western methods, DNA Replication drug effects, Flow Cytometry, Glial Cell Line-Derived Neurotrophic Factor analysis, Glial Cell Line-Derived Neurotrophic Factor pharmacology, Glial Cell Line-Derived Neurotrophic Factor Receptors analysis, Glial Cell Line-Derived Neurotrophic Factor Receptors genetics, Immunohistochemistry methods, Male, Microscopy, Confocal, Neuroglia metabolism, RNA, Messenger analysis, Rats, Rats, Sprague-Dawley, Reverse Transcriptase Polymerase Chain Reaction, Sertoli Cells chemistry, Sertoli Cells metabolism, Spermatozoa chemistry, Spermatozoa drug effects, Spermatozoa metabolism, Glial Cell Line-Derived Neurotrophic Factor metabolism, Glial Cell Line-Derived Neurotrophic Factor Receptors metabolism, Testis metabolism

Abstract

Glial cell-line-derived neurotropic factor (GDNF) and its receptors glial cell-line-derived neurotropic factor alpha (GFR1alpha) and rearranged during transformation (RET) have been localized in the rat testis during postnatal development. The three mRNAs, and GDNF and GFR1alpha proteins were detected in testis extracts from 1- to 90-day-old rats by reverse transcriptase PCR and Western blotting respectively. The three mRNAs were present in Sertoli cells from 20- and 55-day-old rats, pachytene spermatocytes (PS), and round spermatids (RS). The GDNF and GFR1alpha proteins were detected in PS, RS, and Sertoli cells. GDNF and GFR1alpha were also detected using flow cytometry in spermatogonia and preleptotene spermatocytes, and in secondary spermatocytes. The localization of GDNF and GFR1alpha in germ and Sertoli cells was confirmed by immunocytochemistry. The hypothesis that GDNF may control DNA synthesis of Sertoli cells and/or spermatogonia in the immature rat was addressed using cultures of seminiferous tubules from 7- to 8-day-old rats. Addition of GDNF for 48 h resulted in a twofold decrease in the percentage of spermatogonia able to duplicate DNA, whereas Sertoli cells were not affected. These results are consistent with a role of GDNF in inhibiting the S-phase entrance of a large subset of differentiated type A spermatogonia, together with an enhancing effect of the factor on a small population of undifferentiated (stem cells) spermatogonia. Moreover, the wide temporal and spatial expression of GDNF and its receptors in the rat testis suggest that it might act at several stages of spermatogenesis.

Published

2006

56. Phosphatidylserine externalization in human sperm induced by calcium ionophore A23187: relationship with apoptosis, membrane scrambling and the acrosome reaction.

Author

Martin G, Sabido O, Durand P, and Levy R

Subjects

Acrosome metabolism, Amino Acid Chloromethyl Ketones pharmacology, Biomarkers, Calcium metabolism, Caspase Inhibitors, DNA Fragmentation, Enzyme Inhibitors pharmacology, Flow Cytometry, Fluorescein-5-isothiocyanate pharmacology, Humans, In Situ Nick-End Labeling, Male, Membrane Cofactor Protein biosynthesis, Microscopy, Fluorescence, Propidium pharmacology, Pyrimidinones pharmacology, Sperm Capacitation drug effects, Spermatozoa metabolism, Spermatozoa pathology, Acrosome Reaction drug effects, Apoptosis, Calcimycin pharmacology, Cell Membrane metabolism, Ionophores pharmacology, Phosphatidylserines pharmacology, Spermatozoa drug effects

Abstract

Background: Translocation of phosphatidylserine (PS) from the inner to the outer leaflet of the plasma membrane is a modification of the lipid architecture occurring in sperm. This is one of the earliest signs of apoptosis that can be monitored by the calcium-dependent binding of annexin V., Methods and Results: Flow cytometric analysis of annexin V binding was performed. Calcium ionophore A23187 led to a significant increase in the proportion of living sperm with PS exposure: 7.3 3.2% of cells in the untreated ejaculate versus 47.5 5.6% of cells after 1 h of incubation with A23187. Conversely, diminution of mitochondrial membrane potential [DiOC6(3)/propidium iodide (PI) assay], caspase activation [fluorescein isothiocyanate (FITC)-Val-Ala-Asp-fluoromethylketone (VAD-FMK)/PI assay], increased plasma membrane permeability (Yo-Pro-1/PI assay) and increased DNA fragmentation [TdT (terminal deoxynucleotidyl transferase)-mediated dUDP nick-end labelling assay], which are among the main signs of apoptosis, were not observed in sperm, even after 4 h of incubation with A23187. However, A23187 significantly increased the proportion of sperm with plasma membrane scrambling and with a reacted acrosome, as detected with the merocyanine 540 probe (M540) and the monoclonal anti-human CD46-PE antibody respectively., Conclusions: Our results suggest that PS exposure in human sperm, as induced by A23187, is mainly related to the acrosome reaction rather than to apoptosis.

Published

2005

57. Transforming growth factor beta-1 decreases the yield of the second meiotic division of rat pachytene spermatocytes in vitro.

Author

Damestoy A, Perrard MH, Vigier M, Sabido O, and Durand P

Subjects

Animals, Bromodeoxyuridine analysis, Cell Count, Cell Differentiation physiology, Cells, Cultured, Coculture Techniques, Cyclin-Dependent Kinase Inhibitor p21 metabolism, Male, Ploidies, Rats, Sertoli Cells cytology, Spermatocytes metabolism, Transforming Growth Factor beta1, Pachytene Stage physiology, Spermatocytes cytology, Transforming Growth Factor beta physiology

Abstract

Background: TGF beta and its receptors are present in both germ cells and somatic cells of the male gonad. However, knock-out strategies for studying spermatogenesis regulation by TGF beta have been disappointing since TGF beta-or TGF beta receptor-null mice do not survive longer than a few weeks., Methods: In the present study, we addressed the role of TGF beta-1 on the completion of meiosis by rat pachytene spermatocytes (PS) cocultured with Sertoli cells. Identification and counting of meiotic cells were performed by cytology and cytometry., Results: Under our culture conditions, some PS differentiated into round spermatids (RS). When TGF beta-1 was added to the culture medium, neither the number of PS or of secondary spermatocytes nor the half-life of RS was modified by the factor. By contrast, the number of RS and the amount of TP1 mRNA were lower in TGF beta-1-treated cultures than in control cultures. Very few metaphase I cells were ever observed both in control and TGF beta-1-treated wells. Higher numbers of metaphase II were present and their number was enhanced by TGF beta-1 treatment. A TGF beta-like bioactivity was detected in control culture media, the concentration of which increased with the time of culture., Conclusion: These results indicate that TGF beta-1 did not change greatly, if any, the yield of the first meiotic division but likely enhanced a bottleneck at the level of metaphase II. Taken together, our results suggest strongly that TGF beta participates in an auto/paracrine pathway of regulation of the meiotic differentiation of rat spermatocytes.

Published

2005

58. Different DNA ploidy patterns for the differentiation of common subtypes of renal tumors.

Author

Li G, Cottier M, Sabido O, Gentil-Perret A, Lambert C, Genin C, and Tostain J

Subjects

Adenocarcinoma, Clear Cell genetics, Adenoma, Chromophobe genetics, Adenoma, Oxyphilic genetics, Biopsy, Carcinoma, Papillary genetics, Cell Differentiation, Chromosome Aberrations, DNA metabolism, DNA, Neoplasm analysis, Flow Cytometry methods, Humans, Neoplasm Metastasis, Carcinoma, Renal Cell diagnosis, Carcinoma, Renal Cell genetics, DNA analysis, Kidney Neoplasms diagnosis, Kidney Neoplasms genetics, Ploidies

Abstract

Objectives: The common subtypes of renal tumors are conventional or clear cell carcinoma, papillary carcinoma, chromophobe carcinoma and oncocytoma. Each subtype has its distinct histogenesis and clinical evolution. DNA ploidy is viewed as a marker of gross genomic aberrations. The aim of this study is to evaluate the DNA ploidy in the common subtypes of renal tumors to increase our understanding of renal tumor biology and to broaden clinical application of DNA ploidy., Methods: 38 renal tumor samples (13 clear cell RCCs, 12 papillary RCCs, 7 chromophobe RCCs, and 6 oncocytomas) were studied. Five biopsies of different parts of each fresh tumor were subjected to a flow cytometric analysis of DNA ploidy., Results: All tumors except one papillary RCC generated interpretable DNA histograms. Flow cytometric analysis of oncocytomas showed the diploid pattern (29/30 frequencies) while the chromophobe RCC never showed the diploid pattern (0/55 frequencies) (p<0.01). 3/7 chromopbobe RCCs possessed the hypodiploid stemline. The hypodiploid stemline appeared neither in conventional RCCs (0/63 frequencies) nor in papillary RCCs (0/50 frequencies). The diploid pattern was dominant in conventional and papillary RCCs. 10/13 (76.9%) of clear cell RCCs and 9/11 (81.8%) of papillary RCCs possessed a homogeneous DNA ploidy pattern while only 1/7 (14.3%) has a homogeneous DNA ploidy pattern. 6/7 chromophobe RCCs had multiple aneuploid stemlines., Conclusions: Flow cytometric analysis reveals that conventional and papillary RCCs are more homogeneous than chromophobe RCC. Each subtype of renal tumors possesses a specific DNA ploidy pattern. The analysis of DNA ploidy is useful for the differentiation of common subtypes of renal tumors in morphologically difficult cases.

Published

2005

59. Differential production of immunoglobulin classes and subclasses by mucosal-type human B-lymphocytes exposed in vitro to CpG oligodeoxynucleotides.

Author

Cognasse F, Acquart S, Beniguel L, Sabido O, Chavarin P, Genin C, and Garraud O

Subjects

Animals, Antigens, CD metabolism, B-Lymphocytes drug effects, B-Lymphocytes immunology, CD40 Ligand genetics, CD40 Ligand immunology, Coculture Techniques methods, Cytokines genetics, Fibroblasts cytology, Gene Expression drug effects, Humans, Immunoglobulins, Lymphocyte Activation immunology, Membrane Glycoproteins genetics, Mice, Mucous Membrane immunology, NF-kappa B metabolism, Palatine Tonsil cytology, Palatine Tonsil immunology, Receptors, Cell Surface genetics, Toll-Like Receptor 9, Toll-Like Receptors, B-Lymphocytes metabolism, Immunoglobulin Isotypes biosynthesis, Mucous Membrane cytology, Oligodeoxyribonucleotides pharmacology

Abstract

As B-lymphocytes play an important role in innate and adaptive immunity, we aimed to examine the effects of CpG oligodeoxynucleotides (ODNs) on purified tonsil-originating CD19+ B-cells, representing mucosal B-cells. We screened various K-type ODNs, reactive with human B-cells, and tested for the production of immunoglobulins in vitro. Using one CpG-ODN, DSP30, we observed that it could upregulate not only Toll-like receptor 9 (TLR9) mRNA expression in activated B-cells, but also the early expression of CD69 followed by the sequential expression of CD80, CD86 and the nuclear factor (NF)-kappaB pathway. Furthermore, mRNA expression of certain B-cell-derived cytokines was influenced by exposure to DSP30, with a strong upregulation of interleukin 6 (IL-6) and downregulation of IL1-beta. Stimulation of B-cells, co-stimulated with IL-2, IL-10 and soluble CD40 ligand (sCD40L) with different CpG-ODNs, had differing effects on the terminal differentiation in vitro of B-cells into immunoglobulin-secreting cells. TLR9 is involved in innate immunity and the recognition of bound CpG DNA from invading bacterial pathogens. As tonsillar B-cells are mucosal-type B-lymphocytes, this study suggests that CpG-ODNs show promise as mucosal adjuvants in modulating the local production of immunoglobulins of certain classes and subclasses, a crucial issue in vaccine perspectives.

Published

2005

60. In vitro and in vivo evaluation of the influence of type III NaPi co-transporter activity during apoptosis on 99mTc-(V)DMSA uptake in the human leukaemic cell line U937.

Author

Denoyer D, Perek N, Jeune NL, Frere D, Sabido O, Clotagatide A, and Dubois F

Subjects

Animals, Cell Line, Tumor, Dose-Response Relationship, Drug, Humans, Leukemia diagnostic imaging, Leukemia drug therapy, Metabolic Clearance Rate, Mice, Mice, Nude, Organ Specificity, Radionuclide Imaging, Radiopharmaceuticals pharmacokinetics, Sodium-Phosphate Cotransporter Proteins, Tissue Distribution, Antineoplastic Agents pharmacology, Apoptosis drug effects, Etoposide administration & dosage, Leukemia metabolism, Symporters metabolism, Technetium Tc 99m Dimercaptosuccinic Acid pharmacokinetics

Abstract

Purpose: Pentavalent 99mTc-dimercaptosuccinic acid [99mTc-(V)DMSA or (V)DMSA] is a marker of phosphate transport, entering cells specifically through type III NaPi co-transporters. Phosphate ion is known to be involved in cell metabolism, including the apoptotic cell death process. As phosphate accumulation decreases during apoptosis, we investigated the influence of type III NaPi co-transporter activity on (V)DMSA uptake during this type of cell death., Methods: Uptake of (V)DMSA and phosphate was compared in a leukaemic cell line (U937) in vitro model after induction of apoptosis by a chemotherapeutic agent, etoposide (VP16). (V)DMSA biodistribution in nude mice during apoptosis was also investigated in a U937 xenograft in vivo model. The percentage of apoptosis in vitro and ex vivo was determined with annexin V fluorescein by flow cytometry., Results: The in vitro results showed that, in parallel with the decrease in phosphate uptake during apoptosis, (V)DMSA accumulation is negatively correlated with the percentage of apoptosis. Biodistribution studies showed decreased accumulation of (V)DMSA in tumours after treatment with VP16. Animal studies also confirmed an inverse correlation between percentage of apoptosis in tumours and (V)DMSA uptake., Conclusion: The activity of type III NaPi co-transporter is inhibited during the early stages of apoptosis, leading to differential incorporation of (V)DMSA in viable cells and apoptotic cells both in vitro and in vivo.

Published

2004

61. Mitochondrial-dependent regulation of myoblast proliferation.

Author

Duguez S, Sabido O, and Freyssenet D

Subjects

Animals, Antioxidants pharmacology, Cell Differentiation drug effects, Cell Division drug effects, Cell Division genetics, Cell Line, Cyclin-Dependent Kinase Inhibitor p21, Cyclins drug effects, Cyclins metabolism, Down-Regulation drug effects, Down-Regulation genetics, Energy Metabolism drug effects, G1 Phase drug effects, Gene Expression Regulation drug effects, Gene Expression Regulation genetics, Hypertrophy chemically induced, Hypertrophy metabolism, Mitochondria drug effects, Mitochondria genetics, Muscle, Skeletal cytology, Muscle, Skeletal growth & development, Muscle, Skeletal metabolism, Myoblasts drug effects, Myoblasts ultrastructure, Oxidants pharmacology, Proliferating Cell Nuclear Antigen drug effects, Proliferating Cell Nuclear Antigen metabolism, Pyruvic Acid metabolism, Pyruvic Acid pharmacology, Rats, Reactive Oxygen Species metabolism, Regeneration drug effects, Regeneration genetics, Cell Differentiation genetics, Energy Metabolism genetics, Mitochondria metabolism, Myoblasts metabolism

Abstract

The aim of the present study was to determine whether mitochondrial activity could regulate myoblast proliferation. We demonstrate that an increase in mitochondrial activity of L6E9 myoblasts can be easily obtained by simply raising extracellular pyruvate concentration in the culture dish. Under this condition, L6E9 myoblasts underwent a rapid growth arrest in G1 + S phases concomitant to a marked cellular hypertrophy. No sign of myoblast fusion was evident. This was accompanied by the down-regulation of proliferating cell nuclear antigen expression and an increase in p21 expression. Mitochondrial biogenesis was also stimulated, as indicated by a twofold increase in mitochondrial content. These cells exhibited a large increase in the production of reactive oxygen species that could contribute to the observed phenotypic alterations. However, exposure of pyruvate-treated cells to antioxidants did not reverse growth arrest. Similarly, exposure of control cells to oxidants did not induce growth arrest. Our observations suggest that mitochondrial activity appears to play a central role in regulating myoblast proliferation. They also argue strongly in favor of a retrograde communication establishing a mitochondrial control of nuclear gene expression that could be modulated by mitochondrial activity.

Published

2004

62. HIV-1 infection of Langerhans cells in a reconstructed vaginal mucosa.

Author

Sivard P, Berlier W, Picard B, Sabido O, Genin C, and Misery L

Subjects

Anti-HIV Agents pharmacology, Antigens, CD34 analysis, Antiviral Agents pharmacology, Chemokine CCL5 pharmacology, Chemokine CXCL12, Chemokines, CXC pharmacology, Coculture Techniques, Culture Techniques, DNA, Viral isolation & purification, Female, HIV-1 drug effects, HIV-1 isolation & purification, Hematopoietic Stem Cells cytology, Humans, Langerhans Cells metabolism, Leukocytes, Mononuclear virology, Mucous Membrane, Proviruses isolation & purification, Receptors, CCR5 metabolism, Receptors, CXCR4 metabolism, Vagina metabolism, Zidovudine pharmacology, HIV-1 growth & development, Langerhans Cells virology, Receptors, HIV metabolism, Vagina cytology

Abstract

We have developed an in vitro reconstructed vaginal mucosa integrating Langerhans cells (LCs), obtained by differentiation of umbilical cord blood CD34(+) hematopoietic progenitor cells, and, in this model, we have investigated the infection of LCs by human immunodeficiency virus type 1 (HIV-1). Proviral DNA of X4 (LAI and NL4-3) and R5 (Ba-L) HIV-1 strains were detected in LCs integrated in the reconstituted mucosa. Infection of LCs could be specifically inhibited by the chemokines stromal cell-derived factor 1 (SDF-1) and RANTES (regulated on activation, normally T cell-expressed and -secreted), confirming the presence of functional coreceptors on LCs generated in vitro. A complete inhibition of LCs, by use of azidothymidine, a reverse-transcriptase inhibitor, was also observed. Moreover, HIV-1-infected LCs of the reconstructed mucosa were able to transmit R5 or X4 HIV-1 strains to activated peripheral blood mononuclear cells. Such a model could be a useful tool to study the mechanisms involved in transmission of HIV in the female genital tract.

Published

2004

63. Cryopreservation induces an apoptosis-like mechanism in bull sperm.

Author

Martin G, Sabido O, Durand P, and Levy R

Subjects

Animals, Caspases metabolism, Cell Line, Cell Membrane ultrastructure, Cell Nucleus ultrastructure, Cell Survival, Chromatin ultrastructure, Coloring Agents, DNA Fragmentation, Humans, Male, Membrane Potentials, Mitochondria physiology, Propidium, Spermatozoa enzymology, Spermatozoa ultrastructure, Apoptosis, Cattle physiology, Cryopreservation, Spermatozoa physiology

Abstract

Cryopreservation induces many changes in sperm cells, including membrane disorders and cell death. We tested the hypothesis that apoptosis, a form of programmed cell death, can contribute to the fatal effect of cryopreservation on sperm cells. A multiparametric study of apoptosis on bovine sperm is proposed, using flow cytometry, including mitochondrial membrane potential (DeltaPsi(m)), caspase activation, membrane permeability, nucleus condensation, DNA fragmentation, and phosphatidylserine (PS) externalization. The relevance of each test was first validated on a human somatic cell line, U937. Cryopreservation and/or thawing induced significant changes in all apoptotic markers in living bull sperm cells except those concerning the nucleus. After cryopreservation, 44.9% +/- 17% (vs. 11.3% +/- 10.6% before cryopreservation) of sperm cells showed low DeltaPsi(m), 12% +/- 6.3% (vs. 2.2% +/- 1.0% before) contained active caspases, and 10.8% +/- 5.8% (vs. 1.4% +/- 1.1% before) exhibited high membrane permeability. However, cryopreservation had no effect on DNA fragmentation (9.1% +/- 7.7% before vs. 11.1% +/- 5.7% after cryopreservation) or on nucleus condensation (46% +/- 12.7% before vs. 43.8% +/- 13.1% after). Cryopreservation acts as an apoptotic mechanism inducer in bovine sperm cells, where the earliest but not the latest features of cells undergoing apoptosis occur. We have named this abortive process an apoptosis-like phenomenon.

Published

2004

64. Physiological strains remodel extracellular matrix and cell-cell adhesion in osteoblastic cells cultured on alumina-coated titanium alloy.

Author

Di Palma F, Chamson A, Lafage-Proust MH, Jouffray P, Sabido O, Peyroche S, Vico L, and Rattner A

Subjects

Base Sequence, DNA Primers, Enzyme-Linked Immunosorbent Assay, Microscopy, Electron, Scanning, Osteoblasts metabolism, Protein Biosynthesis, Alloys, Aluminum Oxide, Cell Adhesion, Extracellular Matrix, Osteoblasts cytology, Titanium

Abstract

The effects of mechanical strains on cellular activities were assessed in an in vitro model using human osteoblastic MG-63 cells grown on titanium alloy discs coated with porous alumina and exposed to chronic intermittent loading. Strain was applied with a Dynacell device for three 15-min sequences per day for several days with a magnitude of 600 microepsilon strain and a frequency of 0.25 Hz. We have previously demonstrated that this regimen increased alkaline phosphatase activity in confluent cultures on ceramic coated titanium (alumina and hydroxyapatite) (Biomaterials 24 (2003) 3139). In this study, we analysed the production of bone matrix proteins. Osteocalcin secretion quantified by ELISA between day 5 and 11 was not affected by mechanical strain. Strain had even no quantifiable effect on collagen production from day 1 to 5 as measured by carboxy terminal collagen type I propeptide release. On the other hand, stress stimulation resulted in increased expression of fibronectin (FN) measured by Western blot after 1 day stretching. This upregulation of FN production was followed by reorganisation of the FN network after 5 days stretching observed by immunostaining. The receptors for collagen and FN, alpha2beta1, alpha5beta1 and beta1 integrins were not quantitatively affected by the strains as measured by flow cytometry. A modification of cell morphology was seen after 5 days of loading that appeared to increase cell spreading, implying consequences on intercellular contacts. For this reason, N, C11 and E-adherins were examined. We noted a selective effect characterised by increased expression of N-cadherin using both RT-PCR and Western blot analyses. We concluded that reinforcement of cell-cell adhesion and remodelling of the FN network are important adaptive responses to physiological strains for human osteoblasts grown on alumina-coated biomaterials.

Published

2004

65. Identification of germinal center B cells in blood from HIV-infected drug-naive individuals in Central Africa.

Author

Béniguel L, Bégaud E, Cognasse F, Gabrié P, Mbolidi CD, Sabido O, Marovich MA, DeFontaine C, Frésard A, Lucht F, Genin C, and Garraud O

Subjects

Adult, Antigens, CD20 analysis, Blood Donors, Female, Humans, Immunophenotyping, Lymph Nodes immunology, Male, Middle Aged, Trihexosylceramides analysis, Tumor Necrosis Factor Receptor Superfamily, Member 7 analysis, B-Lymphocytes immunology, Germinal Center immunology, HIV Infections immunology

Abstract

To better understand the pathophysiology of B cell populations-the precursors of antibody secreting cells-during chronic human immunodeficiency virus (HIV) infection, we examined the phenotype of circulating B cells in newly diagnosed Africans. We found that all African individuals displayed low levels of naive B cells and of memory-type CD27+ B cells, and high levels of differentiated B cells. On the other hand, HIV-infected African patients had a population of germinal center B cells (i.e. CD20+, sIgM-, sIgD+, CD77+, CD138(+/-)), which are generally restricted to lymph nodes and do not circulate unless the lymph node architecture is altered. The first observations could be linked to the tropical environment whereas the presence of germinal center B cells may be attributable to chronic exposure to HIV as it is not observed in HIV-negative African controls and HAART treated HIV-infected Europeans. It may impact the management of HIV infection in countries with limited access to HIV drugs and urges consideration for implementation of therapeutic vaccines.

Published

2004

66. A flow cytometry technique to study nuclear factor-kappa B (NFkappaB) translocation during human B cell activation.

Author

Cognasse F, Sabido O, Béniguel L, Genin C, and Garraud O

Subjects

Antigens, CD19 immunology, Humans, Lymphocyte Activation, Palatine Tonsil cytology, Signal Transduction, B-Lymphocytes metabolism, Flow Cytometry methods, NF-kappa B metabolism

Abstract

We aimed at examining NFkappaB translocation in B lymphocytes during in vitro activation through the specific receptor for antigen using a technique convenient in most laboratories such as flow cytometry. We present here an original, convenient, and reproducible technique to study B cell activation events through NFkappaB translocation by means of a novel, specific flow cytometry assay. Intranuclear translocation of NFkappaB p65 was induced after a 45min stimulation; the highest signal was detected for a 10 ng/ml stimulus compared to the unstimulated condition (P< 0.05). Purified CD19+ B cells--cultured in the presence of optimal concentrations of anti-micro fragment Abs (10ng/ml) for 45min at 37 degrees C--induced a mean 60% (range: 45-67%) MFI-- and thus, nuclear NFkappaB translocation-increase. We observed a one-pike profile of NFkappaB staining in PBMC B cells and a two-pike profile of NFkappaB staining in using tonsil B cells. B cells are susceptible to various dysregulations leading to minor to severe pathology (including immunoproliferative disorders). Studies of signal transduction carried out specifically in human B cells, using a novel technique gave considerable advantages: feasibility, sensitivity, reproducibility, ease.

Published

2003

67. Age-related changes in the mitotic and metabolic characteristics of muscle-derived cells.

Author

Barani AE, Durieux AC, Sabido O, and Freyssenet D

Subjects

Aging pathology, Animals, Caspase 3, Caspases metabolism, Citrate (si)-Synthase metabolism, Cysteine Endopeptidases metabolism, Down-Regulation, Extracellular Matrix metabolism, L-Lactate Dehydrogenase metabolism, Male, Matrix Metalloproteinases metabolism, Multienzyme Complexes metabolism, Muscle Fibers, Skeletal cytology, Muscle Fibers, Skeletal metabolism, Muscular Atrophy pathology, Plasminogen Activators metabolism, Proliferating Cell Nuclear Antigen metabolism, Proteasome Endopeptidase Complex, Proto-Oncogene Proteins c-met metabolism, Rats, Rats, Sprague-Dawley, Satellite Cells, Skeletal Muscle cytology, Satellite Cells, Skeletal Muscle metabolism, Aging metabolism, Mitosis physiology, Muscle, Skeletal cytology, Muscle, Skeletal metabolism, Muscular Atrophy metabolism

Abstract

Age-related sarcopenia could partly result from cumulative repeated episodes of incomplete repair and regeneration. We hypothesized that mitotic and metabolic events associated with satellite cell activation and proliferation could be altered with aging. Muscle-derived cells (mdc) were isolated from gastrocnemius and quadriceps muscles of young (3 wk old), adult (9 mo old), and old (24 mo old) Sprague-Dawley male rats (n = 10/group). The mdc from young growing rats started to proliferate earlier compared with adult and old animals. Cell cycle duration was significantly reduced with aging from 36.5 +/- 3.2 to 28.0 +/- 2.2 h. However, the proportion of noncycling (G0 phase) and cycling (G1 + S + G2 + M phases) cultured mdc was statistically unchanged among the three age groups. Significantly lower increase in c-met and proliferating cell nuclear antigen expression were observed in cultured mdc of old rats upon serum stimulation. Major changes in the expression of citrate synthase, lactate dehydrogenase, proteasome, caspase 3, plasminogen activators (PAs), and matrix metalloproteinase 2-9 (MMP2-9) were observed upon serum stimulation, but no age-related difference was noted. However, when measured on crushed muscle extracts, PAs and MMP2-9 enzyme activities were significantly decreased with aging. Our results show that cellular and biochemical events associated with the control of mdc activation and proliferation occur with aging. These alterations may participate in the accumulation of repeated episodes of incomplete repair and regeneration throughout the life span, thus contributing to the loss of skeletal muscle mass and function with aging.

Published

2003

68. Macrophages from cancer patients: analysis of TRAIL, TRAIL receptors, and colon tumor cell apoptosis.

Author

Herbeuval JP, Lambert C, Sabido O, Cottier M, Fournel P, Dy M, and Genin C

Subjects

Adenocarcinoma pathology, Apoptosis Regulatory Proteins, Colonic Neoplasms pathology, Confidence Intervals, Culture Media, Conditioned, Enzyme-Linked Immunosorbent Assay, Flow Cytometry, Gene Expression Regulation, Neoplastic, Heart Failure pathology, Humans, In Situ Nick-End Labeling, Interferon-alpha analysis, Pleural Effusion, Malignant etiology, RNA, Messenger analysis, Recombinant Proteins metabolism, Reverse Transcriptase Polymerase Chain Reaction, TNF-Related Apoptosis-Inducing Ligand, Tumor Cells, Cultured, Adenocarcinoma chemistry, Apoptosis, Colonic Neoplasms chemistry, Macrophages chemistry, Membrane Glycoproteins analysis, Pleural Effusion, Malignant pathology, Receptors, Tumor Necrosis Factor analysis, Tumor Necrosis Factor-alpha analysis

Abstract

Background: Tumor-infiltrating macrophages secrete cytokines, including Fas ligand, tumor necrosis factor-alpha (TNF-alpha), and TNF-related apoptosis-inducing ligand (TRAIL). TRAIL induces apoptosis in tumor cells but not in normal cells; however, regulation of TRAIL and its receptors in cancer patients is relatively uncharacterized. We investigated whether macrophages from cancer patients produce TRAIL and whether apoptosis in cultured colon adenocarcinoma cells involves TRAIL and its receptors., Methods: Macrophages isolated from pleural effusions of nine cancer patients and five control patients with congestive heart failure (whose effusions contained no tumor cells) were cultured. Levels of TRAIL, TNF-alpha, interferon alpha, and Fas ligand in conditioned medium were measured by enzyme-linked immunosorbent assays. Apoptosis of human colon adenocarcinoma cell lines, including Colo 205, was determined by the Annexin V method and terminal deoxynucleotidyltransferase-mediated deoxyuridine 5'-triphosphate nick-end labeling (TUNEL). Cell-surface TRAIL receptors were measured by flow cytometry., Results: Conditioned culture medium from macrophages isolated from pleural effusions containing 1%-5% tumor cells (CM-A) contained TRAIL at 980-1300 pg/mL, whereas that from macrophages from pleural effusions containing more than 50% tumor cells or containing no tumor cells (CM-B) contained TRAIL at 0-50 pg/mL. When cultured with medium containing 50% CM-A, 40% (95% confidence interval [CI] = 30% to 50%) of Colo 205 cells underwent apoptosis; when cultured with 50% CM-B, 8% (95% CI = 3% to 13%) underwent apoptosis. When Colo 205 cells were cultured with 50% CM-A, cell-surface expression of TRAIL death receptors DR5 and DR4 increased 13-fold and sixfold, respectively, compared with that of untreated Colo 205 cells. Recombinant TRAIL induced 90% (95% CI = 85% to 95%) of Colo 205 cells to undergo apoptosis and acted synergistically with TNF-alpha to induce apoptosis., Conclusion: Macrophages from cancer patients appear to be activated by tumor cells to produce TRAIL and to increase the expression of TRAIL death receptors DR4 and DR5 on tumor cells.

Published

2003

69. Technique for obtaining highly enriched, quiescent immature Langerhans cells suitable for ex vivo assays.

Author

Tchou I, Sabido O, Lambert C, Misery L, Garraud O, and Genin C

Subjects

Antibodies, Monoclonal, Antigens, CD immunology, Antigens, CD metabolism, Biopsy, Cell Lineage, Epidermal Cells, Epidermis immunology, Epidermis metabolism, Flow Cytometry methods, HLA Antigens immunology, HLA Antigens metabolism, Humans, Langerhans Cells immunology, Langerhans Cells metabolism, Phenotype, Immunomagnetic Separation methods, Langerhans Cells cytology

Abstract

Epidermis and surface epithelium-dendritic cells comprise of immature cells termed Langerhans cells (LCs), which express characteristically the Birbeck granules, along with surface markers such as CD1a. These cells can capture a pathogen and then migrate and differentiate to a more mature stage. During this maturation process, dentritic cells express surface markers differentially. In physio-pathological models of infection where LCs are involved, it is critically important to ensure that the LCs tested in vitro are still immature and are not artefactually matured-dentritic cells. For experimental purposes, LCs were isolated from skin epidermis obtained from patients undergoing plastic surgery. This work thus aimed at collecting fresh LCs ex vivo and at testing the cells for phenotypic and functional characteristics of the immature stage. After mechanic disruption of the epidermis and proceeding for single cell suspension obtaining, two methods for purification were tested in parallel: (a) a positive immuno-magnetic separation by anti-CD1a-coated beads and (b) a purely mechanic purification system based on a three-step Ficoll floatation process. Both systems were equally efficient in terms of purification and yield. By using flow cytometry phenotyping, we have demonstrated that the use of magnetic beads led to some degree of maturation of CD1a(+) LCs, contrary to the repeated Ficoll floatation. This work calls attention for the use of certain monoclonal antibodies such as anti-CD1a to purify immature dendritic cells as they pre-activate these cells. Pre-activation would render a number of assays on the early events of LC physiology invalid, contrary to the purification of fresh skin epidermis LCs by means of a repeated Ficoll floatation.

Published

2003

70. Mitotic activity of rat muscle satellite cells in response to serum stimulation: relation with cellular metabolism.

Author

Barani AE, Sabido O, and Freyssenet D

Subjects

Animals, Cell Division, DNA analysis, Energy Metabolism, Enzymes metabolism, Male, Metabolism drug effects, Myoblasts cytology, Proliferating Cell Nuclear Antigen analysis, Proto-Oncogene Proteins c-met analysis, RNA analysis, Rats, Rats, Sprague-Dawley, Satellite Cells, Skeletal Muscle drug effects, Mitosis drug effects, Satellite Cells, Skeletal Muscle cytology, Satellite Cells, Skeletal Muscle metabolism, Serum Albumin pharmacology

Abstract

Cellular and molecular adaptations of satellite cells isolated from rat hindlimb muscles (n = 10) were investigated in response to serum stimulation. Flow cytometry analysis of the amounts of DNA and RNA indicated that 97.7 +/- 0.7% of satellite cells were in G0 at the end of the isolation procedure, whereas 93.2 +/- 2.0% of cells were cycling after serum exposure. The length of cell division was 34.0 +/- 2.8 h. Myoblast proliferation was asynchronous, suggesting the existence of heterogeneous cell populations in skeletal muscle. Myoblast proliferation was also accompanied by a significant increase in c-met expression, and major adaptations of energetic and proteolytic metabolisms, including an increase in the relative contribution of glycolytic metabolism for energy production, an increase in proteasome and matrix metalloproteinases 2 and 9 activities, and a decrease in plasminogen activator activities. Our data suggest that, along with molecular adaptations leading to cell cycle activation itself, adaptations in energetic and proteolytic metabolisms are crucial events involved in satellite cell activation and myoblast proliferation., (Copyright 2003 Elsevier Science (USA))

Published

2003

71. The in vivo DNA aneuploidization during expansion of conventional renal cell carcinoma.

Author

Li G, Cottier M, Sabido O, Gentil-Perret A, Lambert C, Passebosc-Faure K, Genin C, and Tostain J

Subjects

Carcinoma, Renal Cell pathology, Disease Progression, Female, Flow Cytometry, Humans, Kidney Neoplasms pathology, Male, Middle Aged, Aneuploidy, Carcinoma, Renal Cell genetics, DNA, Neoplasm genetics, Kidney Neoplasms genetics

Abstract

Although numerous studies on the prognostic value of DNA aneuploidy in RCC have been reported, the in vivo DNA aneuploidization during RCC expansion has not been revealed. The present study was undertaken to observe the DNA aneuploidization during RCC expansion. We studied prospectively 67 consecutive conventional RCCs. The ploidy status was determined by analyzing five fresh tumor tissues from different areas by flow cytometry. The diploid, heterogeneous aneuploid tumors and homogeneous aneuploid tumors could be detected, respectively, in 44.8%, 23.9% and 31.3% of cases. The diploid tumors decreased significantly and aneuploid tumors increased significantly as the tumor expanded. The similar DNA content distribution was found between the heterogeneous aneuploid tumors and homogeneous aneuploid tumors. The hypertriploid clone was the most frequent in aneuploid tumors. The tumors of multiple aneuploid clones (16.4%) were mainly found in large-sized tumors. These results suggested that some RCCs underwent DNA aneuploidization during the tumor expansion and that a major route of aneuploidiztion (hypertriploidization) and several pathways existed. Our results also supported the idea that the progressive chromosomal instability was associated with continued tumor growth of RCC. The molecular mechanism and the clinical significance of aneuploidy phenotypes need to be further investigated.

Published

2002

72. Expression of PGP9.5 on Langerhans' cells and their precursors.

Author

Hamzeh H, Gaudillère A, Sabido O, Tchou I, Lambert C, Schmitt D, Genin C, and Misery L

Subjects

Humans, Ubiquitin Thiolesterase, Antigens, Differentiation biosynthesis, Biomarkers, Tumor biosynthesis, Langerhans Cells metabolism

Abstract

Langerhans' cells are epidermal dendritic cells, derived from blood precursors. Their main function is antigen presentation to T-cells. They are able to express neuronal proteins, such as neuron-specific enolase or substance P-receptor. They are closely associated with nerve fibres. PGP9.5 is the most specific neuronal protein in the epidermis. Epidermal Langerhans' cells can express PGP9.5 if denervated. Using flow cytometry, we found that cultured CD34+ precursors did not express PGP9.5, whereas suspensions of fresh or cultured Langerhans' cells could express this neuronal protein. Precursors of Langerhans' cells are not able to express PGP9.5, suggesting that they are not mature enough or that the capacity to express PGP9.5 may be acquired only in the epidermis. The function of PGP9.5 on Langerhans' cells and mature dendritic cells remains unknown. PGP9.5 might be related to dendritic cell maturation or to the lack of contacts with nerve endings.

Published

2000

73. Expression of apoptosis-controlling proteins in acute leukemia cells.

Author

Campos L, Sabido O, Viallet A, Vasselon C, and Guyotat D

Subjects

Acute Disease, Adult, Caspase 2, Caspase 3, Flow Cytometry, HL-60 Cells, Humans, K562 Cells, Apoptosis, Caspase 1 biosynthesis, Caspases biosynthesis, Leukemia metabolism, Leukemia pathology, Proto-Oncogene Proteins c-bcl-2 biosynthesis

Abstract

The expression of Bcl-2 family proteins (Bcl-2, Bcl-X, Bcl-XL, Bcl-Xs, BAX, BAD, MCL-1) and of Interleukin-1 converting enzyme (ICE)-related proteins (ICE, CPP32, ICH- 1) was analyzed in acute leukemia cells by flow cytometry. Most proteins studied were detectable in cell lines such as KG1a, HL60, K562 (myeloblastic), REH, RAJI and MOLT4 (lymphoblastic) and VAL (B-cell lymphoma). However, BCL-Xs and BAK were weakly expressed in K562, as were Bcl-X, BAD and BAK in the VAL line. In acute myeloid leukemia (66 cases studied), the proteins were expressed in most cases in a high percentage of cells, especially BAX and CPP32, without correlation with hematological characteristics. However, Bcl-2 was expressed in a higher percentage of cells in FAB M1 and M5 cases, and in CD34-positive cases, whereas Bcl-Xs was more frequently expressed in M3 cases. No differences were observed regarding fluorescence intensity. Higher percentages of Bcl-2-positive cells were associated with low remission rate, while expression of Bcl-Xs was predictive of high remission rate. In acute lymphoblastic leukemia (36 cases), all proteins studied were expressed in a majority of cases. Bcl-Xs was more frequently detected in T-cell type, and was also associated with a higher remission rate. These results suggest that apoptosis-controlling proteins may have a role in the pathogenesis and response to therapy of acute leukemia.

Published

1999

74. Expression of beta1-integrins and pseudo-immunoglobulins on acute promyelocytic leukemia cells and its modifications during in vitro differentiation.

Author

Thomas X, Anglaret B, Campos L, Thiebaut A, Sabido O, Bailly M, and Archimbaud E

Subjects

Adolescent, Adult, Aged, Bone Marrow Cells metabolism, Bone Marrow Cells pathology, Cell Adhesion, Cell Adhesion Molecules biosynthesis, Cell Differentiation, Female, Humans, Male, Middle Aged, Tumor Cells, Cultured, Antigens, CD biosynthesis, Integrin beta1 biosynthesis, Leukemia, Promyelocytic, Acute metabolism, Leukemia, Promyelocytic, Acute pathology

Abstract

Adhesion molecules are involved in cell-cell interactions and therefore probably play a role in the differentiation and egress of cells from the bone marrow, which might be potentially important in the biology of acute promyelocytic leukemia (APL). All-trans retinoic acid (ATRA) is known to induce in vitro and in vivo differentiation of APL cells and to favor their release from the bone marrow into the blood at initiation of therapy. In order to determine whether these effects might be mediated in part by modifications of beta1-integrin and pseudoimmunoglobulin expression on APL cells, the expression of these adhesion molecules on bone marrow (BM) blast cells from 24 APL patients was assayed at diagnosis by an indirect immunofluorescence method. CD49b, CD49d, CD49e, CD49f, CD54, CD58, and CD56 were expressed respectively on 18%+/-20% (0-66%), 40%+/-31% (0-96%), 48%+/-32% (0-97%), 29%+29% (1-94%), 51%+/-30% (5-98%), 37%+/-24% (1-85%) and 32%+/-31% (0-97%) of APL cells, with respectively 39%, 71%, 79%, 50%, 70%, 70%, and 53% positive cases (> or = 20% positive cells). Despite a wide variability between individual samples, the expression of beta1-integrins and that of pseudo-immunoglobulins tended to be higher in APL in comparison with that of a cohort of 63 patients with other AML subtypes with significant differences for CD54 expression (51%+/-30% vs 28%+/-27%, P=0.006) and CD56 expression (37%+/-24% vs 17%+/-19%, P=0.0003). An in vitro differentiation assay was performed in nine cases. Cells were harvested after 4-7 days of culture and studied for the expression of adhesion molecules. Granulocytic differentiation was marked by persistence of CD15 expression. Antigen expression was decreased after culture with ATRA for all beta1-integrins (except CD49b and CD49f) and pseudoimmunoglobulins (except CD54) tested. However, changes were statistically significant only for CD56 (P=0.04), CD49d (P=0.02) and CD49e (P=0.01). The modifications in the expression of the beta1-integrins and pseudo immunoglobulins were not specific to ATRA-induced differentiation, but commonly observed with differentiation. Furthermore, the modifications in the adhesive properties of APL cells to extracellular matrix proteins, observed on adhesion assays, were not statistically significant after ATRA-induced differentiation. Overall, the level of expression of beta1-integrins and pseudo-immunoglobulins was higher in APL than in other AML subtypes, and appeared modified with induced differentiation. This was not specific of ATRA, but might be involved in the general differentiation phenomenon. The modulation of adhesion molecules does not seem a sufficient requisite for the development of the retinoic acid syndrome, but could nevertheless be part of the increase in leukocyte counts observed during the first days of ATRA therapy.

Published

1998

75. Effects of intermittent or continuous gravitational stresses on cell-matrix adhesion: quantitative analysis of focal contacts in osteoblastic ROS 17/2.8 cells.

Author

Guignandon A, Usson Y, Laroche N, Lafage-Proust MH, Sabido O, Alexandre C, and Vico L

Subjects

Animals, Antineoplastic Agents pharmacology, Cell Adhesion physiology, Cell Division drug effects, Cell Size physiology, Flow Cytometry, Image Cytometry, Microscopy, Confocal, Mitosis drug effects, Nocodazole pharmacology, Osteoblasts chemistry, Osteosarcoma, Rats, Tumor Cells, Cultured, Vinculin analysis, Extracellular Matrix metabolism, Gravity, Altered, Osteoblasts cytology, Osteoblasts metabolism

Abstract

The relationship between cell morphology and cell metabolism and the role of mechanical load in bone remodeling is well known. Mechanical stimulation induces changes in the shape of osteoblasts, probably mediated by reorganization of focal contacts. We studied the influence of gravity (Gz) variations occurring during parabolic flight on osteoblast focal adhesion of ROS 17/2.8 osteosarcoma cells subjected to 15 or 30 parabolic flights. Significant flight-induced shape changes consisted of decreased cell area associated with focal contact plaque reorganization. Identical durations of continuous mechanical stress induced by centrifugation (2 Gz) or clinorotation (Gz randomization) had no major effect on cell focal adhesion. ROS 17/2.8 G2/M synchronization by treatment with nocodazole inhibited the flight-induced decrease in adhesion parameters. We concluded that ROS 17/2.8 cells are sensitive to Gz switches and that their adaptation is at least dependent on microtubule function.

Published

1997

76. Simultaneous expression of P-glycoprotein and BCL-2 in acute myeloid leukemia blast cells.

Author

Campos L, Oriol P, Sabido O, and Guyotat D

Subjects

Adult, Aged, Cell Division, Humans, Leukemia, Myeloid, Acute mortality, Middle Aged, Prognosis, Survival Rate, ATP Binding Cassette Transporter, Subfamily B, Member 1 analysis, Leukemia, Myeloid, Acute metabolism, Proto-Oncogene Proteins c-bcl-2 analysis

Abstract

High expression of the multidrug resistance gene product P170, and of the oncoprotein bcl-2 have been associated with in vitro resistance to chemotherapeutic agents and with poor clinical outcome in acute myeloid leukemia (AML). More recently, it has been shown that autonomous proliferation of blast cells in liquid culture was also predictive of poor prognosis. In a series of 72 adult AML cases at diagnosis, we studied by flow cytometry the expression of P170 and bcl-2 proteins, together with autonomous growth of leukemic cells in liquid culture. Cases were classified as exhibiting no proliferation (N = 29), intermediate proliferation (N = 25) and high proliferation (N = 18). We observed a significant correlation between the percentage of cells in each sample expressing P170 and bcl-2. This was confirmed by double staining techniques showing that both antigens were present in the same cells. We also observed a significant association between growth pattern and P170 or bcl-2 expression. All patients were treated by intensive chemotherapy including an anthracycline drug and cytarabine. The blasts of patients achieving complete remission (N = 47) were less frequently positive for CD34, P170 and bcl-2 than those from patients who did not. Growth pattern also influenced significantly CR. In univariate analysis, CD34, P170 and bcl-2 expression, as well as growth pattern, significantly influenced survival. However, in multivariate analysis P170 expression remained the only significant factor, bcl-2 (or proliferation) having no independent value. Our study confirms the prognostic value of P170 and bcl-2 expression as well as the value of spontaneous proliferation and suggests that several drug-resistance mechanisms are implicated concomitantly in AML.

Published

1997

77. Expression of gastrin-releasing peptide receptor in human skin.

Author

Staniek V, Misery L, Peguet-Navarro J, Sabido O, Cuber JC, Dezutter-Dambuyant C, Claudy A, and Schmitt D

Subjects

Adult, Antigen-Presenting Cells ultrastructure, Blood Vessels ultrastructure, Coloring Agents, Dendritic Cells ultrastructure, Eccrine Glands ultrastructure, Epidermis immunology, Epidermis ultrastructure, Female, Flow Cytometry, Gene Expression, Hair ultrastructure, Humans, Immunohistochemistry, Langerhans Cells ultrastructure, Lymphocyte Activation, Lymphocytes immunology, Lymphocytes ultrastructure, Male, Microscopy, Electron, Microscopy, Immunoelectron, Middle Aged, Nerve Fibers ultrastructure, Receptors, Bombesin genetics, Sebaceous Glands ultrastructure, Skin blood supply, Skin innervation, Skin metabolism, T-Lymphocytes immunology, Receptors, Bombesin ultrastructure, Skin ultrastructure

Abstract

Bombesin-related peptides are expressed in the skin of batrachians and mammals. As gastrin-releasing peptide belongs to this family, we searched for the presence and distribution of gastrin-releasing peptide receptors (GRPr) in the skin of healthy human adults by immunohistochemistry, flow cytometry and electron microscopy. The results indicated that GRPr are expressed on nerves and vessels in the dermis, on eccrine sweat glands, sebaceous glands and erector pili muscle. Within epidermis, staining was localized only on basal and suprabasal layer cells, or in the whole epidermis, according to the samples studied. Interestingly, suprabasal epidermal dendritic cells occasionally showed a strong labelling. Some of these epidermal dendritic cells were identified as Langerhans' cells by immunoelectron microscopy studies. Flow cytometry analysis of crude epidermal cell suspensions resulted in the expression of GRPr on about 43% of the cells. Therefore, we investigated whether human GRPr could modulate Langerhans' cells antigen-presenting functions. For this purpose, we added increasing concentrations of GRP (10(-12) to 10(-5) M) to mixed epidermal cell lymphocyte reactions. Allogeneic T-cell proliferation was not significantly modified when added to GRP-pretreated epidermal cells. In conclusion, we demonstrated the presence of GRPr in human skin, suggesting that GRP may modulate epidermal cell functions but does not modify antigenic presentation.

Published

1996

78. Expression of BCL-2 proto-oncogene in adult acute lymphoblastic leukemia.

Author

Campos L, Sabido O, Sebban C, Charrin C, Bertheas MF, Fière D, and Guyotat D

Subjects

Adolescent, Adult, Aged, Antigens, Differentiation, Myelomonocytic metabolism, Apoptosis, Cell Survival, Chromosomes, Human, Pair 22, Chromosomes, Human, Pair 9, Flow Cytometry, Humans, Leukocyte Count, Linear Models, Middle Aged, Precursor Cell Lymphoblastic Leukemia-Lymphoma immunology, Precursor Cell Lymphoblastic Leukemia-Lymphoma pathology, Prognosis, Proportional Hazards Models, Proto-Oncogene Mas, Proto-Oncogene Proteins c-bcl-2, Translocation, Genetic, Tumor Cells, Cultured pathology, Gene Expression, Precursor Cell Lymphoblastic Leukemia-Lymphoma genetics, Proto-Oncogene Proteins genetics, Proto-Oncogenes genetics

Abstract

The products of the BCL-2 gene prolong survival of lymphohematopoietic cells by inhibition of programmed cell death. We studied bcl-2 protein expression in a series of 43 adult acute lymphoblastic leukemia (ALL) at diagnosis, using a specific monoclonal antibody and flow cytometry. All samples expressed bcl-2 with a mean percentage of positive cells of 77.9. The level of bcl-2 in positive cells expressed as mean equivalent of soluble fluorescence (MESF) was highly variable ranging from 5 x 10(3) to 552 x 10(3) (mean +/- s.d.: 96.5 +/- 109 x 10(3)). Neither the percentage of positive cells nor bcl-2 MESF levels were correlated with initial characteristics including blood counts, immunological phenotype, or cytogenetics. The survival of leukemic cells maintained in cytokine-free liquid culture was not correlated with bcl-2 expression. However, cells from ALL with higher white blood cell (WBC) counts, with t(9;22) translocation, or expressing myeloid surface antigens exhibited significantly longer survival in this culture system. The outcome after intensive chemotherapy did not differ according to bcl-2 expression. Factors associated with poor outcome included WBC counts, presence of t(9;22) translocation, presence of myeloid antigens and prolonged survival of cultured cells. These results indicate that high levels of bcl-2 are not associated with distinct clinical or biological characteristics in ALL.

Published

1996

79. Expression of N-CAM (CD56) on acute leukemia cells: relationship with disease characteristics and outcome.

Author

Thomas X, Vila L, Campos L, Sabido O, and Archimbaud E

Subjects

Acute Disease, Chromosome Aberrations metabolism, Chromosome Deletion, Chromosome Disorders, Female, Humans, Immunophenotyping, Leukemia, Myeloid diagnosis, Leukemia, Myeloid immunology, Male, Middle Aged, Precursor Cell Lymphoblastic Leukemia-Lymphoma diagnosis, Precursor Cell Lymphoblastic Leukemia-Lymphoma immunology, Translocation, Genetic, CD56 Antigen metabolism, Leukemia, Myeloid metabolism, Precursor Cell Lymphoblastic Leukemia-Lymphoma metabolism

Abstract

Expression of CD56 was analyzed by indirect immunofluorescence method on bone marrow samples from 94 newly diagnosed patients with acute leukemia (AL), including 59 acute myelogenous leukemias (AML) and 35 acute lymphoblastic leukemias (ALL). CD56 was expressed on 17 +/- 18% (range: 0-72%) of AML cells and 24 +/- 24% (range: 0-98%) of ALL cells, without significant differences between FAB subtypes in AML, nor immunologic subtypes in ALL. Expression of CD56 was not associated with any clinical or biological characteristic at diagnosis, nor with prognosis in AML or ALL. We do not confirm previously described relationships between CD56 expression and initial characteristics and evolution of acute leukemia.

Published

1995

80. Expression of VLA molecules on acute leukemia cells: relationship with disease characteristics.

Author

Vila L, Thomas X, Campos L, Sabido O, and Archimbaud E

Subjects

Adult, Aged, Antigens, CD analysis, Bone Marrow metabolism, Female, Flow Cytometry, Humans, Immunohistochemistry, Leukemia, Myeloid, Acute blood, Male, Middle Aged, Precursor Cell Lymphoblastic Leukemia-Lymphoma blood, Leukemia, Myeloid, Acute metabolism, Precursor Cell Lymphoblastic Leukemia-Lymphoma metabolism, Receptors, Fibronectin biosynthesis, Receptors, Very Late Antigen biosynthesis

Abstract

VLA molecules are involved in the adhesion of hematopoietic cells to the bone marrow stroma and play a role in the mediation of cellular interactions and migrations that are potentially important in the biology of acute leukemia (AL). We studied the expression of VLA-2 (CD49b), VLA-4 (CD49d), and VLA-5 (CD49e) by indirect immunofluorescence on leukemic cells from 67 patients with acute myelogenous leukemia (AML) and 40 patients with acute lymphoblastic leukemia (ALL). VLA-2, VLA-4, and VLA-5 were expressed, respectively, on 13 +/- 17%, 33 +/- 29%, and 36 +/- 30% of AML cells with 20, 54 and 61% positive cases and on 22 +/- 27%, 40 +/- 30%, and 39 +/- 29% of ALL cells with 29, 60, and 61% positive cases. Significant difference was neither noted between French-American-British (FAB) subtypes in AML or ALL nor between immunologic subtypes in ALL. There were highly significant correlations between the expression of the three beta 1-integrins tested in both AML and ALL. In AML, expression of both VLA-4 and VLA-5 was associated with that of CD14 (p = 0.003 and p = 0.01, respectively) and CD19 (p = 0.006 and p = 0.009, respectively). Expression of VLA-5 was correlated with that of CD15 (p = 0.004). Expression of VLA-4 was associated with both a high initial blast cell count (p = 0.01) and high percentage of bone marrow blast cell involvement (p = 0.003). In ALL, expression of VLA molecules was correlated neither with differentiation antigen nor with hematologic features. In AML, as in ALL, no significant correlation was noted between expression of VLA molecules and evolution of the disease.

Published

1995

81. Identification of two human sperm populations using flow and image cytometry.

Author

Pasteur X, Métézeau P, Maubon I, Sabido O, and Kiefer H

Subjects

Cell Separation, Chromatin metabolism, DNA metabolism, Deoxyribonuclease I, Fertility, Humans, Lasers, Male, Propidium, Spermatozoa metabolism, Staining and Labeling, Flow Cytometry, Spermatozoa cytology

Abstract

Flow cytometric studies of human sperm from fertile men display a constant and characteristic bimodal nonartifactual DNA pattern confirming the existence of two distinct populations. The main population is represented by a peak followed by a shoulder ("marginal population"). The appearance of this marginal population fluctuates with either freezing and thawing or with Percoll gradient centrifugation. We have analyzed both the main and marginal sperm populations by flow cytometry after cell sorting, laser scanning cytometry, light microscopic evaluation, and their sensitivity to DNase digestion. We have observed that the marginal population detected in fertile men represents a sperm group altered in the nuclear condensation, yielding unstable chromatin which appears more stainable with propidium iodide.

Published

1994

82. Over-expression of c-myc oncoprotein in B lymphocytes of renal transplant recipients with lymphoproliferative disorders.

Author

Sabido O, Alamartine E, Barthelemy JC, and Berthoux F

Subjects

Genes, myc genetics, Herpesvirus 4, Human, Humans, Leukemia, Promyelocytic, Acute genetics, Lymphoproliferative Disorders blood, Lymphoproliferative Disorders microbiology, Proto-Oncogene Proteins c-myc metabolism, T-Lymphocytes immunology, B-Lymphocytes physiology, Gene Expression genetics, Kidney Transplantation physiology, Lymphoproliferative Disorders genetics, Proto-Oncogene Proteins c-myc blood, Proto-Oncogene Proteins c-myc genetics

Published

1993

83. The low number of natural killer cells in renal transplant recipients with de novo malignancies.

Author

Alamartine E, Sabido O, and Berthoux FC

Subjects

Humans, Kidney Transplantation immunology, Kidney Transplantation pathology, Leukocyte Count, Neoplasms blood, Neoplasms pathology, Kidney Transplantation adverse effects, Killer Cells, Natural cytology, Neoplasms etiology

Published

1992

84. Comparison of the chromatin stainability of human spermatozoa separated by discontinuous Percoll gradient centrifugation. A flow cytometric contribution.

Author

Pasteur X, Maubon I, Sabido O, Cottier M, and Laurent JL

Subjects

Cell Separation methods, Centrifugation, Density Gradient, Flow Cytometry, Humans, Male, Statistics as Topic, Chromatin chemistry, DNA analysis, Fertilization in Vitro methods, Spermatozoa cytology

Abstract

Many clinical programs in in vitro fertilization (IVF) use the classic Percoll sperm preparation technique to obtain a subpopulation of highly mobile spermatozoa. This Percoll discontinuous gradient centrifugation technique (densities ranging from 1.042 to 1.116 g/mL) was used at room temperature to separate human spermatozoa fractions in order to determine differences in chromatin stainability. The stainability was measured by analysis of DNA fluorochrome uptake by flow cytometry using human peripheral blood lymphocytes as an internal standard. A significant difference in chromatin stainability was noted between the residual fraction (immobile spermatozoa remaining at the top of the Percoll gradient) (44.2%) and the selected one (highly mobile spermatozoa harvested in the 90% and 100% steps) (36.3%). The sperm DNA heterogeneity, as defined by the coefficient of variation (CV), was significantly lower for the selected fraction as compared to the residual one (CV = 12.8% versus 15.4%). A marginal population of spermatozoa adjacent to the germinal peak was also identified. The percentage of this marginal population was significantly lower for the selected fraction as compared to the residual one (7.4% versus 22%). Using a biochemical in vitro decondensation method, the chromatin stainability of the selected and residual fractions (56.9% versus 62.9%) was also determined, demonstrating that the chromatin of the selected fraction was less stainable. This study confirmed that Percoll centrifugation selects a germinal population that is denser and less stainable than with other techniques and analyzed the relation between density, high mobility and probable capacitation.

Published

1992

85. Monoclonal antibody specific for the cellular receptor of echoviruses.

Author

Mbida AD, Gaudin OG, Sabido O, Pozzetto B, and Le Bihan JC

Subjects

Animals, Antibodies, Viral, Antibody Specificity, Binding, Competitive, Cell Line, Enterovirus B, Human classification, Humans, KB Cells, Kinetics, Serotyping, Antibodies, Monoclonal, Enterovirus B, Human immunology, Receptors, Virus immunology

Abstract

Cell lines of primate origin carry membrane receptors which are specific for echoviruses (EV). The present report describes isolation and characterization of a monoclonal antibody (Mab 143) reacting with the membrane of KB cells. The Mab was selected for its protection of different cell lines from primate origin against the CPE of EV-11. This protection was found to extend to most EV serotypes and to coxsackievirus A9, while the replication of several other picornaviruses was not affected. The fluorecein isothiocyanate labelled Mab did not react with cell lines from bovine, canine, or rabbit origin, but bound specifically to the cell lines from human or simian origin. These results suggest that a unique receptor site is used by most EV serotypes for binding onto and penetration into susceptible cells.

Published

1992

86. Quantitative assessment of chromatin stability alteration in human spermatozoa induced by freezing and thawing. A flow cytometric study.

Author

Pasteur X, Sabido O, Maubon I, Perrin-Cottier M, and Laurent JL

Subjects

Flow Cytometry, Freezing, Humans, Male, Propidium, Semen physiology, Staining and Labeling, Chromatin ultrastructure, Cryopreservation, Spermatozoa ultrastructure

Abstract

The authors examined the effect of cryopreservation on chromatin stability in human spermatozoa from 21 ejaculates. Each ejaculate was divided into four aliquots: (1) fresh aliquot, (2) frozen and thawed aliquot, (3) fresh aliquot subjected to an in vitro decondensation method, and (4) frozen and thawed aliquot subjected to the same in vitro decondensation method; all were then fixed with an ethanol fixative agent. Chromatin stainability was quantified by flow cytometric measurement of fluorochrome uptake by DNA. Study of 21 fresh aliquots showed that 37.9% of the DNA was accessible to propidium iodide. The comparative stainability between the 21 fresh and 21 frozen-thawed, undecondensed aliquots demonstrated a low but significant increase in accessibility of DNA by propidium iodide for the thawed samples: 38.7 +/- 1.7% (mean +/- SD) versus 37.9 +/- 1.3%. The biochemical action of the nuclear decondensation solution increased the accessibility of propidium iodide, but in different ways: 57.2 +/- 12.9% versus 54.7 +/- 13.7%, respectively, for fresh and frozen-thawed aliquots. Analysis of the flow cytometric histograms revealed an intermediate population of spermatozoa adjacent to the main germinal peak. This population increased significantly: 9.6 +/- 1.9% for the fresh versus 12.3 +/- 4.9% for the frozen-thawed undecondensed aliquots and 8.6 +/- 3.5% versus 12.3 +/- 4.9%, respectively, for fresh and frozen-thawed, decondensed aliquots. Because the chromatin stability of thawed spermatozoa may be a critical factor in assisted procreation, the authors discuss the effect of thermal denaturation on the nucleoprotein structures and the origin of the intermediate population of spermatozoa.

Published

1991

87. Flow cytometric analysis of DNA content in colorectal polyps resected at endoscopy.

Author

Perrin-Cottier M, Jouffre C, Sabido O, Maubon I, Barthélémy C, Pasteur X, Audigier JC, and Laurent JL

Subjects

Adult, Aged, Aged, 80 and over, Aneuploidy, Colorectal Neoplasms genetics, Colorectal Neoplasms pathology, DNA, Neoplasm genetics, Endoscopy, Female, Flow Cytometry, Humans, Male, Middle Aged, Ploidies, Polyps genetics, Polyps pathology, Colorectal Neoplasms chemistry, DNA, Neoplasm analysis, Polyps chemistry

Abstract

Samples from 64 consecutive resected colorectal polyps were preserved in liquid nitrogen and analyzed by flow cytometry to assess the nuclear DNA content, which was compared to the histopathologic findings. The frequency of aneuploidy in these nonselected polyps was 17.2%. There was a significant correlation between the diameter of the polyp and the frequency of aneuploidy (P = .04), with all aneuploid polyps being greater than or equal to 10 mm. Similarly, aneuploidy was significantly more frequent for polyps that were both greater than or equal 20 mm and showed at least severe dysplasia (P = .02). On the other hand, there was no correlation between the ploidy and the gross histopathologic type (tubular, tubulovillous or villous), and the proliferation index did not correlate with any of the parameters studied.

Published

1991

88. Quantitative assessment of human spermatozoa chromatin stainability by flow cytometry: preliminary study.

Author

Pasteur X, Maubon I, Cottier M, Sorg P, Seffert P, Laurent JL, and Sabido O

Subjects

DNA chemistry, Ejaculation, Humans, Male, Spermatozoa physiology, Chromatin chemistry, Flow Cytometry, Spermatozoa chemistry, Staining and Labeling

Abstract

The authors report a human sperm suspension method to assess quantitatively the stainability of the spermatozoa chromatin. Analysis of 15 ejaculates demonstrated the existence of a constant percentage of stained DNA in different ejaculated spermatozoa. The condensed chromatin stainability was then compared to the in vitro decondensed chromatin stainability with the finding of an increased uptake of fluorochrome in relation with the nuclear chromatin decondensation. The quantitative spermatozoa chromatin stainability and its decondensation aptitude may be of importance in sperm physiology.

Published

1990

89. Relation between malignancies and viral infections with natural killer cells in renal transplant recipients.

Author

Alamartine E, Sabido O, Buisson V, Videcoq C, and Berthoux F

Subjects

Cytotoxicity, Immunologic, Humans, Neoplasms complications, Virus Diseases complications, Kidney Transplantation immunology, Killer Cells, Natural immunology, Neoplasms immunology, Virus Diseases immunology

Published

1990

90. [Phenotypic and functional study of natural killer lymphocytes in flow cytometry: application to renal transplantation].

Author

Alamartine E, Sabido O, Buisson V, Videcocq C, and Berthoux F

Subjects

Adult, Azathioprine pharmacology, Flow Cytometry, Humans, Interleukin-2 immunology, Kidney Failure, Chronic immunology, Killer Cells, Natural drug effects, Middle Aged, Phenotype, Kidney Transplantation immunology, Killer Cells, Natural immunology

Abstract

In order to define the best appraisal of Natural Killer cells, the authors performed a dual study, including both phenotypes and functional activities, and all the analyses were achieved with flow cytometric techniques. Results were applied to renal transplantation. Among the numerous clusters of differenciation, only CD16 and CD56 appeared to be well correlated with the functional properties of Natural Killer cells, and especially for CD3- cells. On the other hand, CD57 should no longer be considered as a NK marker. Functional properties of Natural Killer cells were evaluated by cytotoxicity assays of peripheral lymphocytes against K562 and Daudi tumor cells, either spontaneously, or after a 3-day activation with Interleukin 2 (LAK). The authors use carboxyfluoro-diacetate to label viable cells and avoid radioisotopes. They confirm the Natural Killer cells deficiency in renal transplant recipients, and show that this impairment also involves the LAK cytotoxicity. Azathioprine appeared to be responsible of such deficiency. During viral infections, Natural Killer cells raised and reached the normal values, while they were incapable of any response to fight against cancer. They suggest that the Natural Killer deficiency could explain the high incidence of malignancies during renal transplantation.

Published

1990