Your search keyword '"Barque JP"' showing total 32 results

1. Purification and characterisation of a breast-cancer-associated glycoprotein not expressed in normal breast and identified by monoclonal antibody 83D4

Author

Pancino, G, primary, Osinaga, E, additional, Charpin, C, additional, Mistro, D, additional, Barque, JP, additional, and Roseto, A, additional

Published

1991

2. Constitutive overexpression of immunoidentical forms of PCP-induced Euglena gracilis CYP-450.

Author

Barque JP, Abahamid A, Flinois JP, Beaune P, and Bonaly J

Subjects

Animals, Antibodies immunology, Cell Line, Cross Reactions, Euglena gracilis drug effects, Euglena gracilis growth & development, Immunoblotting, Isoenzymes biosynthesis, Isoenzymes immunology, Protozoan Proteins biosynthesis, Protozoan Proteins immunology, Rats, Cytochrome P-450 Enzyme System biosynthesis, Cytochrome P-450 Enzyme System immunology, Environmental Pollutants pharmacology, Euglena gracilis enzymology, Pentachlorophenol pharmacology

Abstract

Environmental pollutants are classically associated with increased drug metabolism. In this report, antibodies that are able to detect mammalian CYP proteins, namely the CYP1A1, CYP1A2, CYP2B1/B2, and CYP3A4 proteins, were used to investigate the expression of CYP-related proteins in Euglena gracilis (EG) cells under normal and PCP-treated conditions and in a EG-cell line adapted to PCP. Compared to normal conditions, the presence of PCP in the culture medium induced elevated levels of EG CYP-like proteins. With the exception of CYP3A4, this overexpression was correlated with expression of additional forms of CYP proteins having, respectively, the same molecular weight but slightly different pIs. Even in EG cells which had lost their PCP-adapted property after having been cultured without PCP, these additional forms were continuously expressed. This observation raised the question about the definition of a biomarker of pollution.

Published

2002

3. In Euglena gracilis, a heat-shock protein related to hsc73 is constitutive and stress inducible.

Author

Barque JP, Schedler P, Floch E, and Bonaly J

Subjects

Animals, Antibodies, Monoclonal, Blotting, Western, Cadmium pharmacology, Drug Resistance, Electrophoresis, Gel, Two-Dimensional, Euglena gracilis drug effects, HSC70 Heat-Shock Proteins, Heat-Shock Proteins immunology, Heat-Shock Proteins isolation & purification, Hot Temperature, Protozoan Proteins immunology, Protozoan Proteins isolation & purification, Euglena gracilis metabolism, HSP70 Heat-Shock Proteins, Heat-Shock Proteins metabolism, Protozoan Proteins metabolism

Abstract

Using monoclonal antibodies directed against different cytoplasmic isoforms of hsp70 proteins, namely, the constitutive hsc73 and the inducible hsp72 isoforms, we found that one isoform related to hsc73 was present in Euglena gracilis. This hsc73-like protein is expressed with a higher rate of synthesis in cells growing under heat shock than in control cells. Moreover, in cadmium-resistant cells, cultured at normal growth temperature, the rate of synthesis of this protein is constitutively increased. These results indicate that a heat-shock protein related to hsc73 is present in an ancestral eukaryote, Euglena gracilis, and that this protein may be constitutive and stress inducible as well.

Published

2000

4. Gene expression of a protein, JB70, related to rat alpha1-acid glycoprotein in Euglena gracilis.

Author

Durand G, Delranc C, Bonaly J, Chacun H, Porquet D, and Barque JP

Subjects

Animals, Blotting, Northern, Blotting, Western, Cloning, Molecular, DNA Probes, DNA, Complementary, Orosomucoid immunology, RNA, Messenger genetics, Rats, Antigens immunology, Euglena gracilis genetics, Orosomucoid genetics

Abstract

Antibodies directed against rat alpha1-acid glycoprotein (AGP) recognize a 70 kDa antigen, designated JB70, present in extracts of achlorophyllous Euglena gracilis cells as well as in their culture medium. By using 2-dimensional electrophoresis, JB70 appears to be composed of two acidic polypeptides. Additionally, Northern blot analysis reveals the presence in E. gracilis cells of a 2.3 kb mRNA hybridizing with a cDNA probe specific for rat AGP mRNA. Moreover, elevated mRNA levels are detected in dexamethasone-treated E. gracilis cells, indicating a response to this inducer similar to that observed for hepatic AGP. These results strongly suggest that polypeptides closely related to hepatic rat AGP are expressed in E. gracilis cells. They also indicate that, like other gene families implicated in natural defense processes such as heat-shock protein and metallothionein genes, the AGP gene appears to be conserved down to this early diverging eucaryote.

Published

1997

5. Immunodetection of a protein related to mammalian arrestin in Euglena gracilis.

Author

Razaghi A, Bonaly J, Chacun H, Faure JP, Mirshahi M, and Barque JP

Subjects

Amino Acid Sequence, Animals, Antibodies, Monoclonal, Arrestin chemistry, Arrestin genetics, Cattle, Conserved Sequence, Cross Reactions, Epitopes chemistry, Epitopes genetics, Evolution, Molecular, Immunoblotting, Isoelectric Point, Microscopy, Fluorescence, Molecular Weight, Protozoan Proteins chemistry, Retina chemistry, Retina immunology, Signal Transduction, Arrestin immunology, Euglena gracilis immunology, Protozoan Proteins immunology

Abstract

Six monoclonal antibodies directed against different epitopes of bovine retinal arrestin recognized a single polypeptide in extracts of achlorophyllous Euglena gracilis cells. This polypeptide had an apparent molecular weight slightly lower: 45kDa vs. 48 kDa, and a more basic isoelectric point compared to that of bovine visual arrestin. It was located in an insoluble cytoplasmic fraction. Immunofluorescence assays show a cytoplasmic punctuated pattern suggesting a cluster distribution or a linkage to some cell structure. The presence of arrestine-like molecules in achlorophyllous Euglena gracilis cells suggests that these proteins might be involved in a peculiar step of chemical signal transduction processes.

Published

1997

6. Different heat-shock proteins are constitutively overexpressed in cadmium and pentachlorophenol adapted Euglena gracilis cells.

Author

Barque JP, Abahamid A, Chacun H, and Bonaly J

Subjects

Animals, Drug Resistance, Electrophoresis, Gel, Two-Dimensional, Electrophoresis, Polyacrylamide Gel, Euglena gracilis drug effects, Gene Expression Regulation, Plant drug effects, HSP70 Heat-Shock Proteins biosynthesis, HSP90 Heat-Shock Proteins biosynthesis, Heat-Shock Proteins isolation & purification, Molecular Weight, Cadmium pharmacology, Euglena gracilis metabolism, Heat-Shock Proteins biosynthesis, Pentachlorophenol pharmacology

Abstract

To determine whether cellular resistance to a given stressor is related to induction of specific stress-proteins, responses of two adapted Euglena gracilis cell lines, one adapted to cadmium, the other adapted to pentachlorophenol, were analyzed. Our experiments showed that two sets of heat-shock proteins (hsps) were constitutively overexpressed in each cell line: while hsp90, hsp70, hsp55, and hsp40 were induced in cadmium-resistant cells, only hsp40 was induced in pentachlorophenol-adapted cells.

Published

1996

7. Chromosomal localization and expression pattern of the RNase L inhibitor gene.

Author

Aubry F, Mattéi MG, Barque JP, and Galibert F

Subjects

Amino Acid Sequence, Base Sequence, Blotting, Northern, Chromosome Banding, Chromosome Mapping, DNA, Complementary, Endoribonucleases antagonists & inhibitors, Enzyme Inhibitors, Female, Genome, Human, Humans, In Situ Hybridization, Male, Molecular Sequence Data, Organ Specificity, Pregnancy, Protein Biosynthesis, RNA, Messenger analysis, Transcription, Genetic, ATP-Binding Cassette Transporters, Chaperonins, Chromosomes, Human, Pair 4, Proteins genetics, RNA, Messenger biosynthesis

Abstract

2-5A-Dependent RNase (RNase L), an important component of the 2-5A pathway, is directly implicated in the molecular mechanism of interferon action. We have cloned and sequenced following immunoscreening, a full-length cDNA that encodes the RNase L inhibitor (RLI). Northern blot analysis from a variety of human tissues revealed that two transcript forms (3.8 kb and 2.4 kb) are ubiquitously expressed but differences in levels of expression suggest a tissue-specific regulation. The RLI gene was localized to locus 4q31 by in situ hybridization indicating that this gene and other enzymes of the 2-5A pathway are not organized in cluster in the human genome.

Published

1996

8. Protein synthesis in cadmium- and pentachlorophenol-tolerant Euglena gracilis.

Author

Barque JP, Abahamid A, Bourezgui Y, Chacun H, and Bonaly J

Subjects

Animals, Cell Line, Dose-Response Relationship, Drug, Euglena gracilis drug effects, Euglena gracilis genetics, Euglena gracilis growth & development, Gene Expression, Proteins genetics, Cadmium pharmacology, Environmental Pollutants pharmacology, Euglena gracilis metabolism, Pentachlorophenol pharmacology, Protein Biosynthesis

Abstract

This work is a preliminary characterization of two adapted Euglena gracilis cell lines, one to cadmium and the other to pentachlorophenol. Growth curve analyses indicate that tolerance to one pollutant did not protect against the second pollutant. These suggest that metabolic pathways that are induced by one pollutant are specific for this pollutant. This specificity is detectable at the level of gene expression.

Published

1995

9. Growth responses of achlorophyllous Euglena gracilis to selected concentrations of cadmium and pentachlorophenol.

Author

Barque JP, Abahamid A, Bourezgui Y, Chacun H, and Bonaly J

Subjects

Animals, Euglena gracilis growth & development, Time Factors, Cadmium pharmacology, Euglena gracilis drug effects, Pentachlorophenol pharmacology

Abstract

The growth response of a wild achlorophyllous Euglena gracilis mutant was studied during exposure to cadmium and pentachlorophenol (PCP). Cadmium gradually reduced the growth rate and terminal cell density; PCP only lengthened the initial lag phase relative to control cultures. Flow cytometry showed that cadmium altered the cell cycle by delaying late S and G2/M phases; PCP did not disturb the cell cycle, but markedly affected DNA staining: the intercalating dyes ethidium bromide and propidium iodide showed little staining compared to controls. However, replication and transcription processes were not altered by PCP, as cell division occurred normally. Cells surviving after PCP treatment apparently developed an adaptative response during the lag phase.

Published

1995

10. Cadmium resistance of achlorophyllous Euglena gracilis cells: constitutive overexpression of two heat-shock proteins.

Author

Barque JP, Chacun H, Marouby S, and Bonaly J

Subjects

Animals, Electrophoresis, Gel, Two-Dimensional, Electrophoresis, Polyacrylamide Gel, Euglena gracilis metabolism, Heat-Shock Proteins isolation & purification, Molecular Weight, Cadmium toxicity, Drug Resistance physiology, Euglena gracilis drug effects, Heat-Shock Proteins biosynthesis

Abstract

The heat-shock response of Euglena gracilis was studied by cell labeling at both the normal growth temperature (23 degrees C) and an elevated temperature (35 degrees C). Analysis of the labeled proteins by two-dimensional polyacrylamide gel electrophoresis indicated that the rate of synthesis of two polypeptides p55 (55 kDa) and p40 (40 kDa) increased in cells labeled at the highest temperature studied. These polypeptides are also overexpressed in Cadmium-resistant Euglena gracilis cells labeled at the normal growth temperature (23 degrees C). On the basis of these results, p55 and p40 appear to be heat-shock proteins involved in some steps of the acquired Cd-resistance process in Euglena gracilis cells.

Published

1994

11. A novel 43-kDa glycoprotein is detected in the nucleus of mammalian cells by autoantibodies from dogs with autoimmune disorders.

Author

Soulard M, Barque JP, Della Valle V, Hernandez-Verdun D, Masson C, Danon F, and Larsen CJ

Subjects

Animals, Antibody Specificity, Cell Fractionation, Dogs, HeLa Cells, Humans, Immunologic Techniques, Lupus Erythematosus, Systemic immunology, Molecular Weight, RNA, Heterogeneous Nuclear immunology, Antibodies, Antinuclear immunology, Dog Diseases immunology, Glycoproteins immunology, Lupus Erythematosus, Systemic veterinary, Nuclear Proteins immunology, Ribonucleoproteins immunology

Abstract

We have characterized a new antibody specificity in a panel of sera from dogs developing systemic lupus erythematosus (SLE) or clinically related autoimmune disorders. This antibody stains in a speckled fashion the nucleus of cells of different mammalian origins. The target antigen is a basic (pI 9.2) nuclear polypeptide with an apparent molecular weight of 43 kDa (p43) which is detected in various mammalian cell nuclei. p43, as studied in HeLa cells, appears to be cell cycle-independent. It is released from nuclei by salts (0.5 M NaCl or 0.25 M ammonium sulfate). Upon subfractionation of nuclear components, p43 is found in the fraction containing HnRNPs and is recovered in immunoprecipitates obtained with 4F4 monoclonal antibody to HnRNP C proteins. Immunoelectron microscopy revealed that p43 is concentrated over the dense chromatin periphery and interchromatin granule clusters. Another important feature of p43 is its ability to specifically bind wheat germ agglutinin lectin but not concanavalin A nor Ulex europaeus I, supporting the notion that p43 is a glycoprotein bearing an N-acetyl-glucosamine moiety. Consistent with this result, a radio-active p43 band is specifically immunoprecipitated by canine anti-p43 autoantibodies from HeLa cells metabolically labeled with [14C]glucosamine. Finally, anti-p43 antibodies do not immunoprecipitate SnRNA, indicating that p43 has no apparent association with SnRNPs.

Published

1991

12. [Production of a monoclonal antibody (B1N) recognizing human nuclear antigen associated with cell proliferation].

Author

Baville F, Ammouri O, Charpin C, Della-Valle V, Soulard M, Guillemin MC, Osinaga E, Pancino G, Roseto A, and Barque JP

Subjects

Animals, Cervix Uteri ultrastructure, Female, Humans, Lymphocytes immunology, Mice, Mice, Inbred BALB C, Nuclear Proteins immunology, Protein Methyltransferases, tRNA Methyltransferases, Antibodies, Monoclonal immunology, Antigens isolation & purification, Cell Division, Cell Nucleus immunology

Abstract

This report describes the preliminary characterization of a novel antigen reactive with a murine monoclonal antibody designated B1N produced in our laboratory. This antibody (IgM) reacts in IFI with mammals and also insect cells, by staining in a speckled fashion the nucleus of these cells. Immunoblotting analysis of Hela and murine D55 nuclear extracts revealed a polypeptide with an apparent molecular weight of 120kD (p120). In this work we demonstrated that: 1. this polypeptide appeared in human peripheral blood lymphocytes only when they were induced to proliferate in vitro after phytohemagglutinin stimulation; 2. this polypeptide was no longer detected in D55 resting cells, following serum deprivation; 3. the MAb B1N specifically revealed the nucleus of proliferating cells on frozen sections of uterine tissue. These data strongly suggest that the p120 nuclear antigen expression is associated with the proliferation state of cells.

Published

1991

13. Human autoantibodies identify a nuclear chromatin-associated antigen (PSL or p55) in human platelets.

Author

Barque JP, Karniguian A, Brisson-Jeanneau C, Della-Valle V, Grelac F, and Larsen CJ

Subjects

Aged, Antigens, Nuclear, Blood Platelets ultrastructure, Cell Nucleus immunology, Electrophoresis, Female, Fluorescent Antibody Technique, Humans, Immunoblotting, Microscopy, Electron, Autoantibodies immunology, Autoantigens analysis, Blood Platelets immunology, Chromatin immunology, Nuclear Proteins analysis

Published

1990

14. [Production and characterization of hybrid monoclonal antibodies with IgG1/IgG3 double isotype].

Author

Lebègue V, Joron L, Barque JP, Pancino G, and Roseto A

Subjects

Antibodies, Monoclonal genetics, Antibodies, Monoclonal immunology, Cell Fusion, Chlamydia immunology, Clone Cells, Cytomegalovirus immunology, Enzyme-Linked Immunosorbent Assay, Antibodies, Monoclonal biosynthesis, Hybrid Cells immunology, Immunoglobulin G immunology, Immunoglobulin Isotypes immunology

Abstract

In order to obtain bispecific monoclonal antibodies, two hybridoma cell lines were fused: E13 producing an IgG1 anti-Cytomegalovirus, and 70B12 producing an IgG3 anti-Chlamydia. This experimental model was chosen to test the possibility of association between gamma 1 gamma 3 heavy chains. This association was shown by using an ELISA.

Published

1990

15. [Serum antibodies in dogs with autoimmune disorders recognize 40 kd glycoprotein in the nucleus of mammalian cells].

Author

Soulard M, Barque JP, Della Valle V, Danon F, and Larsen CJ

Subjects

Animals, Dogs, Glycoproteins classification, HeLa Cells, Immunoglobulin G immunology, Molecular Weight, Antibodies, Antinuclear immunology, Autoimmune Diseases immunology, Glycoproteins immunology, Lupus Erythematosus, Systemic immunology, Mammals immunology

Abstract

We report a new antibody specificity in 15 sera recovered from a group of dogs developing systemic lupus erythematosus (SLE) or clinically related disorders. This antibody stains in a speckled fashion the nucleus of human Hep-2 cells. Immunodiffusion tests with saline extracts of rabbit thymus showed that all 15 sera generate a common precipitation line which crosses the lines from reference sera to Sm, SS-A/ro, SS-B/La, and RNP antigens. The target nuclear antigen is a 40 kD polypeptide (p40). An important property of p40 resides in its ability to bind specifically Wheat Germ Agglutinin lectin but not Concanavalin A, supporting the notion that the antigen is a glycoprotein bearing a N-acetylglucosamine moiety.

Published

1990

16. [Effect of toyocamycin on the biosynthesis of viral glycoproteins in a cell line chronically infected with a murine retrovirus].

Author

Mathieu-Mahul D, Barque JP, Mauchauffe M, Peraudeau L, and Larsen CJ

Subjects

Animals, Cell Line, Membranes metabolism, Mice, Friend murine leukemia virus metabolism, Glycoproteins biosynthesis, Ribonucleosides pharmacology, Toyocamycin pharmacology, Viral Proteins biosynthesis

Abstract

Toyocamycin (TMC), an adenosine analog has been previously reported to inhibit both number and infectivity of retrovirus particles released by chronically infected cells (Bonar et al., 1970; Riman, 1971; Mauchauffé et al., 1979). We have previously shown that loss of infectivity could result from the incorporation of TMC in place of adenosine in the genomic 35S RNA (Larsen et al., 1979). This phenomenon is likely to impair the structure of the viral genome in such a way that reverse transcriptase cannot properly copy the template. Another consequence of the Toyocamycin action on the retrovirus particles released by analog-treated cells was their reduced content in envelope glycoprotein or gp70 (Mathieu - Mahul et al., 1979). In order to find the origin of this defect, which could also explain the loss of infectivity, viral polypeptides present in the cytoplasm of Toyocamycin-treated cells were analyzed by immunoprecipitation with specific antisera. The results indicated a diminution of the biosynthesis of the envelope glycoprotein and other GAG gene-related polypeptides. However, the gpr85env precursor was normally synthesized and processed into its final products (gp70 + p15E), which accumulated in the cells. These result make it likely that Toyocamycin has no specific effect on the virus replicative process in chronically infected cells but acts by deteriorating cellular functions, which are necessary to virus assembly. Indeed, it was found that a membrane fraction corresponding to smooth endoplasmic reticulum and Golgi apparatus was severely reduced if not totally suppressed in TMC-treated cells.

Published

1981

17. Characterization by human antibodies of two HeLa cell proteins which are related to Xenopus laevis transcription factor TFIIIA.

Author

Lagaye S, Barque JP, le Maire M, Denis H, and Larsen CJ

Subjects

Animals, Antibody Specificity, Cell Compartmentation, Cytoplasm metabolism, HeLa Cells, Humans, Molecular Weight, Xenopus laevis, Autoantibodies immunology, Autoimmune Diseases immunology, Nuclear Proteins immunology, RNA, Ribosomal metabolism, RNA, Ribosomal, 5S metabolism, Ribonucleoproteins immunology, Transcription Factors immunology

Abstract

The sera of two patients with autoimmune disorders recognize in HeLa cell extracts two proteins with apparent molecular masses of 37,000 (p37) daltons and 32,000 daltons (p32). These proteins are non covalently associated with 5S RNA and sediment as 7-10 S particles in sucrose density gradients. Both proteins are antigenetically related to TFIIIA, a previously described protein of Xenopus laevis, which is known as a 5S RNA transcription factor and occurs in oocytes as a noncovalent complex with 5S RNA. Like TFIIIA, HeLa cell proteins p37 binds in vitro to 5S RNA and to cloned 5S RNA genes. These results suggest that protein p37 fulfils in HeLa cells a function similar to that of TFIIIA in amphibian oocytes, ie control of 5S RNA transcription.

Published

1988

18. [A cytoplasmic antigen related to the cell cycle identified by a human autoimmune serum].

Author

Lagaye S, Barque JP, Péraudeau L, Danon F, and Larsen CJ

Subjects

Cell Cycle, HeLa Cells, Humans, Interphase, Antigens isolation & purification, Autoantibodies immunology, Cytoplasm immunology

Abstract

A human serum from a patient with an autoimmune disorder, previously characterized for its ability to specifically recognize a chromatin-associated PSL or p55 antigen, was found also to detect a 30-32 K polypeptide in the cytoplasm of human HeLa cells. This molecule is strictly cytoplasmic, does not cross react with nuclear PSL and is synthesized only during the S phase of the cell cycle.

Published

1984

19. Enzyme-substrate interaction in lipid monolayers. I. Experimental conditions and fundamental kinetics.

Author

Dervichian DG and Barque JP

Subjects

Adsorption, Animals, Kinetics, Membranes, Artificial, Pancreas enzymology, Protein Binding, Surface Properties, Swine, Diglycerides, Glycerides, Lipase metabolism

Abstract

A systematic study has shown the importance of the different factors which are concerned with the action of lipase on a substrate (1,3-didecanoylglycerol). These consist of a) the process of adsorption of lipase to the surface, b) the necessity of limited stirring to reach equilibrium, and c) the persistence during the reaction process of the enzyme molecules adsorbed on the monolayer. On the basis of this preliminary investigation, a technique was established to analyze the mechanism of lipase action with defined quantities of enzyme and lipid segregated in the monolayer. Thus, the process of the reaction itself is separated from the adsorption process, and it is demonstrated that the quantity of substrate hydrolyzed per minute depends only on the quantity of initially adsorbed lipase and not on the quantity of substrate or on the surface concentration of the enzyme. An appropriate new definition of the rate is consequently adopted.

Published

1979

20. [Characterization of a new nuclear antigen using a human serum containing antinuclear antibodies (author's transl)].

Author

Barque JP, Yéni P, Péraudeau L, Signoret Y, Danon F, and Larsen CJ

Subjects

Animals, Humans, Immune Sera, Mice, Rabbits, Antibodies, Antinuclear immunology, Antigens analysis, Autoimmune Diseases immunology, Nucleoproteins immunology, Ribonucleoproteins immunology

Published

1982

21. Analysis of viral RNA and proteins expressed by a non producer Friend erythroleukemia cell line (HFL/b cell line).

Author

Mathieu-Mahul D, Robert J, Barque JP, and Larsen CJ

Subjects

Animals, Cell Line, Cell Transformation, Viral, Defective Viruses analysis, Friend murine leukemia virus genetics, Genes, Viral, Mice, Nucleic Acid Hybridization, Friend murine leukemia virus analysis, Leukemia, Erythroblastic, Acute microbiology, Peptides analysis, RNA, Viral analysis, Viral Proteins analysis

Published

1981

22. Enzyme-substrate interaction in lipid monolayers. II. Binding and activity of lipase in relation to enzyme and substrate concentration and to other factors.

Author

Barque JP and Dervichian DG

Subjects

Adsorption, Animals, Kinetics, Mathematics, Membranes, Artificial, Pancreas enzymology, Protein Binding, Surface Properties, Swine, Diglycerides, Glycerides, Lipase metabolism

Abstract

With the limited stirring procedure used in the present work, substrate and enzyme together form a segregated and well-defined system on the surface. The lipase molecules responsible for the lipolysis are only those that are adsorbed on the glyceride monolayer. After a study of the stirring procedure, two series of systematic experiments were done: a) the bulk concentration of the enzyme was varied with different constant surface concentrations of the substrate, and b) the surface concentration of the substrate was varied with different constant bulk concentrations of the enzyme. The influence of the surface concentration of substrate on a) the rate of lipolysis, V,; b) the enzyme activity, a,; and c) the enzyme adsorption, Ze, were each determined by a different procedure. The values obtained verify the enzymic activity equation (a = V/Ze). The roles of other factors (Ca2+ ions, and pH) which govern the adsorption of the enzyme and its specific activity were also studied in preliminary experiments.

Published

1979

23. PSL, an S phase-related p55 nuclear antigen, associates transiently with chromatin.

Author

Barque JP, Lagaye S, Bendayan M, Puvion-Dutilleul F, Danon F, and Larsen CJ

Subjects

Animals, Chemical Precipitation, Colchicine pharmacology, Fluorescent Antibody Technique, HeLa Cells, Humans, Immunochemistry, Liver immunology, Liver ultrastructure, Metaphase drug effects, Microscopy, Electron methods, Protein Binding, Rats, Rats, Inbred Strains, Antigens analysis, Autoantigens analysis, Cell Nucleus immunology, Chromatin analysis, Interphase drug effects, Nuclear Proteins, Nucleoproteins analysis

Abstract

An S phase-related nuclear 55K antigen, also designated PSL, has been characterized in various mammalian cells, using a human serum from a patient with autoimmune disorders (Barque et al., EMBO j 2 (1983) 743). In this report, we show by immunoelectron microscopy that the p55 protein associates in situ with the chromatin of rat hepatocytes. This association is a transient one, as indirect immunofluorescence studies show that PSL does not bind to individualized metaphase chromosomes. Furthermore, immunoprecipitation tests indicate that the majority of PSL is in the non-chromosomal cell fraction. These results suggest that this nuclear antigen is directly involved in the DNA replication process.

Published

1985

24. Nuclear ribonucleoproteins recognized by human antinuclear antibodies in retrovirus-infected cells.

Author

Barque JP, Yeni P, Peraudeau L, Danon F, and Larsen CJ

Subjects

Animals, Cell Nucleus analysis, Electrophoresis, Polyacrylamide Gel, Friend murine leukemia virus, Humans, Leukemia, Experimental immunology, Lupus Erythematosus, Systemic immunology, Mice, RNA, Viral isolation & purification, Antibodies, Antinuclear immunology, Nucleoproteins immunology, Retroviridae Infections immunology, Ribonucleoproteins immunology

Published

1981

25. [A variety of human autoantibodies recognizes in HeLa cells 2 proteins related to the TFIIIA factor of Xenopus laevis which regularizes the transcription of ribosomal 5S RNA].

Author

Lagaye S, Barque JP, Della Valle V, Danon F, Le Maire M, Denis H, and Larsen CJ

Subjects

Animals, Chemical Precipitation, HeLa Cells, Humans, Molecular Weight, Transcription Factor TFIIIA, Transcription Factors immunology, Xenopus laevis, Autoantibodies immunology, Transcription Factors analysis

Abstract

Using the sera from two patients with autoimmune disorders, we have identified by immunoprecipitation of HeLa cell extracts two proteins with apparent molecular masses of 37 kDa (p 37) and 32 kDa (p 32). These proteins are associated with 5 S RNA. They are antigenetically related to Xenopus laevis 5 S RNA transcription factor TFIIIA, which is very abundant in early oocytes of this species. In contrast to what is observed in X. laevis oocytes, the TFIIIA-related proteins of HeLa cells are present in very small amounts. Our data suggest that proteins p 37 and p 32 are involved in the control of 5 S RNA transcription.

Published

1987

26. Nucleolar proteins identified in human cells as antigens by sera from dogs with autoimmune disorders.

Author

Soulard M, Lagaye S, Della Valle V, Danon F, Larsen CJ, and Barque JP

Subjects

Animals, Autoimmune Diseases immunology, Cell Line, Cell Nucleolus ultrastructure, Dogs, Fluorescent Antibody Technique, HeLa Cells immunology, HeLa Cells ultrastructure, Humans, Immune Sera, Immunoblotting, Molecular Weight, Nuclear Proteins isolation & purification, Autoimmune Diseases veterinary, Cell Nucleolus immunology, Dog Diseases immunology, Nuclear Proteins immunology

Abstract

In the course of a systematic screening of sera from dogs suffering from autoimmune disorders, three sera were shown by indirect immunofluorescence to characteristically label the nucleoli and nucleoplasm of human cell lines (Hep-2 and HeLa). This pattern of staining persisted throughout the cell cycle, except for mitosis when the fluorescence was localized in extrachromosomal areas. By immunoblotting nuclear and subnuclear fractions, three polypeptides of 110,000, 95,000, and 45,000 Da apparent molecular weight were identified, which reacted with all three sera. By means of affinity purification, it was shown that an antibody specific for any one of the three proteins also reacts with the two others. This antigenic cross-reactivity suggested regions of structural homology shared by the three proteins. Indeed, treatment of nucleoli with high concentrations of DNase I containing residual proteolytic activity resulted in the disappearance of the 110- and 95-kDa proteins and the concomitant appearance of a doublet of 45-kDa proteins. Subnuclear localization studies indicated that all three polypeptides were located in both nucleoli and nucleoplasm. Significantly, the 110-kDa protein differs from the major nucleolar protein, nucleolin, by its electrophoretic mobility in two-dimensional gels, its location in nucleoli and in nucleoplasm, its absence in nucleolar organizer regions of chromosomes, and its differential solubility of DNase I. Therefore, the three antigenically related species reported in this study constitute a new class of nucleolar proteins.

Published

1989

27. [Change in the envelope of a murine retrovirus produced in the presence of toyocamycin].

Author

Mathieu-Mahul D, Barque JP, Samso A, Mauchauffé M, and Larsen CJ

Subjects

Animals, Glucosamine metabolism, Glycoproteins metabolism, Mice, Peptides metabolism, Retroviridae metabolism, Retroviridae ultrastructure, Viral Proteins metabolism, Antibiotics, Antineoplastic pharmacology, Retroviridae drug effects, Toyocamycin pharmacology

Abstract

Toyocamycin (TMC), an adenosine analog, impairs qualitatively and quantitatively virus production in a cellular system chronically infected by Friend Virus. Viral particles released by cell cultures treated with 0.2 microgram/ml of the drug have lost most of their glycoprotein (gp 70) content. This phenomenon is likely to modify the viral envelope and could explain the loss of infectivity of the virus.

Published

1979

28. Enzyme--substrate interaction in lipid monolayers. III. A study of the variation of the surface concentration with lipolysis.

Author

Barque JP and Dervichian DG

Subjects

Adsorption, Kinetics, Lipolysis, Surface Properties, Diglycerides metabolism, Glycerides metabolism, Lipase metabolism, Membranes, Artificial

Abstract

Monolayers of a diacylglycerol were submitted to the action of lipase, keeping the area constant. The variation of lipase, keeping the area constant. The variation of the surface concentration gamma of the substrate with time was derived from the recorded reduction of the surface pressure pi (the isotherm of the monolayer being previously established). The rate -d gamma/dt was determined both as a function of the surface concentration gamma of the substrate and as a function of the bulk concentration C of the enzyme in the underlying solution. The rate depends on the quantity of enzyme ze adsorbed on the monolayer and on the enzymatic specific activity alpha of these adsorbed enzyme molecules. Both ze and alpha vary with gamma. The two variations have been quantitatively dissociated. The curves of ze and of alpha as functions of gamma coincide with those previously established in the study of hydrolysis under constant surface pressure.

Published

1979

29. Genetic analysis of myeloproliferative leukemia virus, a novel acute leukemogenic replication-defective retrovirus.

Author

Penciolelli JF, Wendling F, Robert-Lezenes J, Barque JP, Tambourin P, and Gisselbrecht S

Subjects

Animals, Cloning, Molecular, DNA Restriction Enzymes, Leukemia, Experimental genetics, Mice, Nucleic Acid Hybridization, Virus Replication, DNA Replication, Friend murine leukemia virus genetics, Genes, Viral, Helper Viruses genetics, Retroviridae genetics

Abstract

The myeloproliferative leukemia virus (MPLV) is a new acute leukemogenic, nonsarcomatogenic retroviral complex that is generated during the in vivo passage of a molecularly cloned Friend ecotropic helper virus. Examination of viral RNA expression in MPLV-producing cells revealed the presence of two distinct molecular species that hybridized with a long terminal repeat or an ecotropic env-specific probe but not with a xenotropic mink cell focus-forming virus env-specific probe derived from a spleen focus-forming virus: an 8.2-kilobase species corresponding to a full-length Friend murine leukemia virus (F-MuLV) and a deleted species with a genomic size of 7.4 kilobases. This deleted virus was biologically cloned by limiting dilutions and single cell cloning in Mus dunni fibroblasts. Three nonproducer clones with normal morphologies and containing one single integrated copy of the deleted virus were superinfected with F-MuLV, Moloney murine leukemia virus, Gross murine leukemia virus, mink cell focus-forming virus (HIX), or the amphotropic 1504 murine leukemia virus. All pseudotypes caused macroscopic and microscopic abnormalities in mice that were similar to those seen in the parental stock. A comparison of the physical maps of F-MuLV and MPLV, which was deduced from the restriction enzyme digests of unintegrated proviral DNAs, indicated that the MPLV-defective genome (i) is probably derived from F-MuLV, (ii) has conserved the F-MuLV gag and pol regions, and (iii) is deleted and rearranged in the env region in a manner that is clearly distinct from that of Friend or Rauscher spleen focus-forming viruses.

Published

1987

30. PSL, a nuclear cell-cycle associated antigen is increased during retinoic acid-induced differentiation of HL-60 cells.

Author

Barque JP, Lagaye S, Ladoux A, Della Valle V, Abita JP, and Larsen CJ

Subjects

Humans, Isoelectric Point, Molecular Weight, Phosphoproteins metabolism, Phosphorylation, Tumor Cells, Cultured, Cell Cycle, Cell Differentiation drug effects, Nuclear Proteins metabolism, Tretinoin pharmacology

Abstract

PSL(p55) is a nuclear 55kD antigen present in various mammalian cell systems, which has been first identified by use of human autoimmune antibodies (Barque et al. 1983, EMBO J. 2, 743). It has been shown to be associated with interphase chromatine and to be synthesized in during the S phase of the cell cycle. In this work, we have analysed the status of PSL in promyelocytic HL-60 human cells in exponential or stationary growth, or undergoing granulocytic differentiation in presence of Retinoic acid. By use of 2-dimensional electrophoresis, PSL was found to be composed of two acidic proteins designated p55A and p55B. Unexpectedly, estimated 10-20 fold higher amounts of each species were found in cells treated for 5 days with 10(-6)M Retinoic acid, than in asynchronously growing cells or resting cells. Moreover, the p55A protein was phosphorylated during the process. On the basis of these results, PSL appears to be involved in some steps of the granulocytic differentiation process.

Published

1987

31. Characterization by human autoantibody of a nuclear antigen related to the cell cycle.

Author

Barque JP, Danon F, Peraudeau L, Yeni P, and Larsen CJ

Subjects

Animals, Cell Cycle, Centrifugation, Density Gradient, Fluorescent Antibody Technique, Microscopy, Fluorescence, Mink, Antigens immunology, Autoantibodies analysis, Autoimmune Diseases immunology

Abstract

Using a serum from a patient with an autoimmune disease, we have recently described a novel 55 000-dalton antigen (p55) in the nucleus of several animal cells including human ones. This antigen, designated PSL, was not related to the previously defined antigens recognized by sera from patients with systemic rheumatic diseases (Sm, n-RNP, SS-B, Scl-70). We have now found that p55 is associated with chromatin structures as it is released from the nucleus of mink cell fibroblasts by saline + DNase treatments. Analysis by sucrose gradient centrifugation of the nuclear material released in these conditions indicated that p55 co-migrated with core histones. Meanwhile, p55 was absent from the residual nuclear matrices (achromatinic nuclei). Localization of p55 in synchronized cells was performed by indirect immunofluorescence and immunoprecipitation. P55 appeared to accumulate in the nucleus during the S phase. Finally, it was not recognized by an anti-SV40 tumor serum that specifically precipitated the protein p53, which has been recently related to cell proliferation. Thus, PSL an p53, although apparently not antigenically related, appear to be implicated in the same step of the cell cycle.

Published

1983

32. [Demonstration of fixation of an enzyme on a superficial lipid layer].

Author

Dervichian DG, Préhu C, and Barque JP

Subjects

Adsorption, Binding Sites, Cholesterol, Models, Biological, Phosphatidylcholines, Surface Properties, Glycerides, Lipase, Phospholipases, Phospholipids

Published

1973