Your search keyword '"Bergé-Lefranc JL"' showing total 37 results

1. Early-onset haemochromatosis caused by a novel combination of TFR2 mutations(p.R396X/c.1538-2 A>G) in a woman of Italian descent.

Author

Gérolami V, Le Gac G, Mercier L, Nezri M, Bergé-Lefranc JL, and Férec C

Subjects

Adult, Age of Onset, DNA Mutational Analysis, Female, Ferritins biosynthesis, Hemochromatosis ethnology, Heterozygote, Humans, Iron metabolism, Italy, Cation Transport Proteins genetics, Hemochromatosis diagnosis, Hemochromatosis genetics, Mutation, Receptors, Transferrin genetics

Published

2008

2. hOGG1(326), XRCC1(399) and XRCC3(241) polymorphisms influence micronucleus frequencies in human lymphocytes in vivo.

Author

Mateuca RA, Roelants M, Iarmarcovai G, Aka PV, Godderis L, Tremp A, Bonassi S, Fenech M, Bergé-Lefranc JL, and Kirsch-Volders M

Subjects

Adult, DNA Damage, Genotype, Humans, Lymphocytes chemistry, Male, Micronucleus Tests, Occupational Exposure, Smoking, X-ray Repair Cross Complementing Protein 1, DNA Glycosylases genetics, DNA-Binding Proteins genetics, Micronuclei, Chromosome-Defective, Polymorphism, Genetic

Abstract

A pooled analysis of five biomonitoring studies was performed to assess the influence of hOGG1(326), XRCC1(399) and XRCC3(241) gene polymorphisms on micronuclei (MN) frequency in human peripheral blood lymphocytes, as measured by the ex vivo/in vitro cytokinesis-block micronucleus (CBMN) assay. Each study addressed a type of occupational exposure potentially able to induce DNA strand breakage (styrene, ionising radiation, cobalt/hard metal, welding fumes and inorganic arsenite compounds), and therefore MN, as a result of base excision repair and double-strand break repair deficiencies. The effect of genotype, age, exposure to genotoxic agents and smoking habit on MN induction was determined using Poisson regression analysis in 171 occupationally exposed male workers and in 132 non-exposed male referents. The analysis of genotype-genotype, genotype-smoking and genotype-exposure interactions by linear combinations of parameters showed significantly higher MN frequencies in the following subsets: (i) occupationally exposed workers carrying either the Thr/Thr or the Thr/Met XRCC3(241) genotypes compared to their referent counterparts (P < 0.001) and (ii) carriers of the Met/Met XRCC3(241) genotype compared to Thr/Thr XRCC3(241) carriers, as far as they are non-exposed and bear the variant (Ser/Cys or Cys/Cys) hOGG1(326) genotype (P < 0.01). Significantly lower MN frequencies were observed in carriers of the variant hOGG1(326) genotype compared to Ser/Ser hOGG1(326) carriers in the subgroup of non-smokers with Thr/Thr XRCC3(241) genotype (P < 0.01). Stratified analysis by occupational exposure showed a significant MN increase with smoking in occupationally exposed carriers of the Arg/Gln XRCC1(399)genotype (P < 0.001). In contrast, a significant MN decrease with smoking was observed in referents carrying the Ser/Ser hOGG1(326) genotype (P < 0.01). These findings provide evidence that the combination of different DNA repair genes and their interaction with environmental genotoxic agents may modulate MN induction. Understanding the complexity of the relationships between exposure, DNA repair and MN frequencies require larger scale studies and complementary biomarkers.

Published

2008

3. DNA-repair and carcinogen-metabolising enzymes genetic polymorphisms as an independent risk factor for hepatocellular carcinoma in Caucasian liver-transplanted patients.

Author

Borentain P, Gérolami V, Ananian P, Garcia S, Noundou A, Botta-Fridlund D, Le Treut YP, Bergé-Lefranc JL, and Gérolami R

Subjects

Carcinogens metabolism, Carcinoma, Hepatocellular enzymology, Carcinoma, Hepatocellular surgery, DNA Repair Enzymes metabolism, Electrophoresis, Agar Gel, Female, Gene Amplification, Humans, Liver Neoplasms enzymology, Liver Neoplasms surgery, Liver Transplantation, Male, Middle Aged, Risk Factors, X-ray Repair Cross Complementing Protein 1, Carcinoma, Hepatocellular genetics, DNA Repair, DNA-Binding Proteins genetics, Glucuronosyltransferase genetics, Glutathione Transferase genetics, Liver Neoplasms genetics, Polymorphism, Genetic

Abstract

We studied polymorphisms of three genes, UDP-glucuronosyltransferase1A7 (UGT1A7), Glutathione-S-transferaseM1 (GSTM1) and X-Ray Cross Complementing group 1 (XRCC1), involved in detoxification of xenobiotics or DNA-repair in a population of 133 liver-transplanted patients, including 56 patients with hepatocellular carcinoma (HCC) and 77 without HCC, and in 89 healthy controls originating from the south of France. Multiple logistic regression analysis showed that, among liver-transplanted patients, interactions between XRCC1-G/G or -G/A and GSTM1-nul polymorphisms were independently associated with hepatocellular carcinoma (p interaction=0.027) concurrently with increasing age (p<0.001), male sex (p=0.037) and chronic hepatitis B or C virus infection (p=0.018 and p=0.001 respectively). On the contrary, no relationship was observed between UGT1A7 polymorphisms considered alone or in interaction with GSTM1 or XRCC1 polymorphisms and HCC. This suggests that concomitant impaired metabolism of carcinogenic compounds and impaired DNA-repair function play an important role in liver carcinogenesis in high-risk cirrhotic patients originating from the south of France.

Published

2007

4. Increased expression of adenosine A2A receptors in patients with spontaneous and head-up-tilt-induced syncope.

Author

Carrega L, Saadjian AY, Mercier L, Zouher I, Bergé-Lefranc JL, Gerolami V, Giaime P, Sbragia P, Paganelli F, Fenouillet E, Lévy S, and Guieu RP

Subjects

Adenosine metabolism, Adolescent, Adult, Aged, Case-Control Studies, Female, Humans, Male, Middle Aged, Receptor, Adenosine A2A genetics, Syncope blood, Gene Expression Regulation, Receptor, Adenosine A2A metabolism, Syncope etiology, Syncope metabolism

Abstract

Background: Adenosine may play a role in the triggering of neurocardiogenic syncope, but no information on adenosine receptors is available at the present time., Objective: The purpose of this study was to investigate whether adenosine A2A receptors expression is altered in patients with neurocardiogenic syncope., Methods: Adenosine plasma levels (APLs), the expression of A2A receptors, were measured (mean +/- standard error of the mean) during tilt testing. Expression of receptors was assessed on mononuclear cells using a selective receptor ligand., Results: At baseline, the APLs of 16 patients with a positive test were higher than those of 17 patients with a negative test and of those of a control group (2.10 +/- 0.30 vs. 0.40 +/- 0.05 and 0.41 +/- 0.06 muM, respectively; P <.0001). The number of receptors was higher in patients tested positive than in patients tested negative or in the control group (122 +/- 10 vs. 38 +/- 4 and 44 +/- 4 fmol/g of proteins, respectively; P <.0001). No difference was found in the affinity or synthesis among the three groups., Conclusion: This study showed an increased number and an up-regulation of adenosine A2A receptors in patients with spontaneous syncope and a positive head-up tilt, which in the context of high APLs may play a role in the recurrence of syncopal episodes.

Published

2007

5. Molecular characterization of myophosphorylase deficiency (McArdle disease) in 34 patients from Southern France: identification of 10 new mutations. Absence of genotype-phenotype correlation.

Author

Aquaron R, Bergé-Lefranc JL, Pellissier JF, Montfort MF, Mayan M, Figarella-Branger D, Coquet M, Serratrice G, and Pouget J

Subjects

Adolescent, Adult, Aged, DNA Mutational Analysis methods, Female, France epidemiology, Genotype, Glycogen Storage Disease Type V epidemiology, Humans, Male, Middle Aged, Pedigree, Phenotype, Retrospective Studies, Genetic Heterogeneity, Glycogen Phosphorylase, Muscle Form genetics, Glycogen Storage Disease Type V genetics, Mutation

Abstract

We report on 31 patients and 3 affected siblings (17 males and 17 females) from Southern France with McArdle disease (two from Spanish and three from Portuguese background). Molecular analysis revealed the presence of five previously described mutations: the common p.R50X nonsense mutation, the p.R94W and p.V456M missense mutations, the p.K609K conservative mutation which generates an aberrant splicing, and the p.K754fs frameshift mutation; and 10 new molecular defects: eight missense mutations at homozygous (p.G136D) or heterozygous state (p.T379M, p.G449R, p.T488I, p.R490Q, p.R570Q, p.R590H, and p.R715W), one nonsense mutation p.R650X and one deletion (p.delK170). Our results confirm that the p.R50X nonsense mutation is also the most common associated with myophosphorylase deficiency in the Southern French population: 21 of 25 French unrelated patients (15 homozygous and six heterozygous, i.e., 72% of the mutated alleles). Two patients, one from Algeria and one from Tunisia, were homozygous for a previously identified missense mutation p.V456M in a Moroccan subject. Our findings further demonstrate molecular heterogeneity of myophosphorylase deficiency, absence of genotype-phenotype correlation and expand the already crowded map of mutations within the myophosphorylase gene. Our study also provides evidence for increased medical interest of malignant hyperthermia susceptibility (MHS) because of 34 McArdle disease patients, three and two affected siblings were contracture-tested and found to be positive.

Published

2007

6. Evolution of DNA strand-breaks in cultured spermatocytes: the Comet Assay reveals differences in normal and gamma-irradiated germ cells.

Author

Perrin J, Lussato D, De Méo M, Durand P, Grillo JM, Guichaoua MR, Botta A, and Bergé-Lefranc JL

Subjects

Animals, Antimetabolites, Bromodeoxyuridine, Caspases metabolism, Cell Survival radiation effects, Cells, Cultured, Coculture Techniques, Comet Assay, Germ Cells ultrastructure, Kinetics, Male, Rats, Rats, Wistar, Sertoli Cells radiation effects, Sertoli Cells ultrastructure, Spermatocytes ultrastructure, DNA Damage radiation effects, Gamma Rays, Germ Cells radiation effects, Spermatocytes radiation effects

Abstract

In reproductive toxicity assessment, in vitro systems can be used to determine mechanisms of action of toxicants. However, they generally investigate the immediate effects of toxicants, on isolated germ cells or spermatozoa. We report here the usefulness of in vitro cultures of rat spermatocytes and Sertoli cells, in conjunction with the Comet Assay to analyze the evolution of DNA strand-breaks and thus to determine DNA damage in germ cells. We compared cultures of normal and gamma-irradiated germ cells. In non-irradiated spermatocytes, the Comet Assay revealed the presence of DNA strand-breaks, which numbers decreased with the duration of the culture, suggesting the involvement of DNA repair mechanisms related to the meiotic recombination. In irradiated cells, the evolution of DNA strand-breaks was strongly modified. Thus our model is able to detect genotoxic lesions and/or DNA repair impairment in cultured spermatocytes. We propose this model as an in vitro tool for the study of genotoxic injuries on spermatocytes.

Published

2007

7. Oculocutaneous albinism type 2 (OCA2) with homozygous 2.7-kb deletion of the P gene and sickle cell disease in a Cameroonian family. Identification of a common TAG haplotype in the mutated P gene.

Author

Aquaron R, Soufir N, Bergé-Lefranc JL, Badens C, Austerlitz F, and Grandchamp B

Subjects

Albinism, Oculocutaneous metabolism, Cameroon, Case-Control Studies, Female, Genotype, Globins genetics, Globins metabolism, Homozygote, Humans, Pedigree, Polymorphism, Single Nucleotide, Albinism, Oculocutaneous genetics, Anemia, Sickle Cell genetics, Gene Deletion, Haplotypes, Membrane Transport Proteins genetics, Mutation

Abstract

In this study, we report on a Cameroonian family from the Ewondo ethnic group, presenting with three oculocutaneous albinism type 2 (OCA2) patients homozygous for the 2.7-kb deletion of the P gene. In one of these patients OCA2 was associated with sickle cell anaemia and in two with the sickle cell trait. We took this opportunity to determine single nucleotide polymorphism (SNP) haplotypes within the P gene in this family in comparison with a group of 53 OCA2 patients homozygous for the same mutation and with a matched unrelated full-coloured control group of 49 subjects, originating from seven different ethnic groups of Southern Cameroon including Ewondo. A combination of five exonic and intronic SNPs in the OCA2 gene was genotyped by sequencing PCR products. We found 3 different haplotypes (TAGCT, TAGTT and TAGCC with frequencies of 0.66, 0.28 and 0.06, respectively) associated with the mutation in the 53 OCA2 patients, while 11 different haplotypes were observed in the control group. These observations suggest that the mutation appeared on the relatively frequent haplotype TAGCT, and that the two other haplotypes are derived from two independent recombination events. These haplotypic data, associated with a value of 1/15,000 for the prevalence of the 2.7-kb mutation, a present effective population size of 10,000,000 for Cameroon and a recombination rate of 0.0031, allowed us to estimate that this mutation originated 4,100-5,645 years ago.

Published

2007

8. Assessment of occupational exposure to welding fumes by inductively coupled plasma-mass spectroscopy and by the alkaline Comet assay.

Author

Botta C, Iarmarcovai G, Chaspoul F, Sari-Minodier I, Pompili J, Orsière T, Bergé-Lefranc JL, Botta A, Gallice P, and De Méo M

Subjects

Adult, Air Pollutants, Occupational blood, Air Pollutants, Occupational urine, Comet Assay, Environmental Monitoring, Humans, Lymphocytes drug effects, Male, Mass Spectrometry methods, Metals blood, Metals urine, Middle Aged, Air Pollutants, Occupational toxicity, DNA Damage, Metals toxicity, Occupational Exposure, Welding

Abstract

Welding fumes are classified as possibly carcinogenic to humans (Group 2B) by the International Agency for Research on Cancer. In the current study, blood and urine concentrations of aluminum (Al), cadmium (Cd), cobalt (Co), chromium (Cr), manganese (Mn), nickel (Ni), lead (Pb), and zinc (Zn) were monitored by inductively coupled plasma-mass spectrometry (ICP-MS) in 30 welders and in 22 controls. In addition, DNA damage was examined in the lymphocytes of these subjects by the alkaline Comet assay. Two biological samples were taken from the welders at the beginning (BW) and at the end (EW) of a work week. In controls, collection of samples was limited to BW. Blood concentrations of Cd, Co, Cr, Ni, and Pb were higher in the welders than in the control group while higher concentrations of Al, Cd, Co, Cr, Ni, and Pb were detected in welder urines. There was no significant difference in the metal concentrations for the BW and EW welder samples. Increased levels of DNA damage were found in lymphocytes from welders as compared to the controls, and 20/30 welders had higher levels of DNA lesions in the EW than in the BW samples. Age had a significant effect on DNA damage in the control group. Spearman's rank correlation analysis indicated that there were positive correlations between blood concentrations of Al, Co, Ni, and Pb and the levels of DNA damage. A negative correlation was found between DNA damage and Mn in blood, while there was a positive correlation between urinary Mn concentration and DNA damage. These data indicate that occupational exposure to welding fumes increases DNA damage in lymphocytes., (Copyright (c) 2006 Wiley-Liss, Inc.)

Published

2006

9. A combined analysis of XRCC1, XRCC3, GSTM1 and GSTT1 polymorphisms and centromere content of micronuclei in welders.

Author

Iarmarcovai G, Sari-Minodier I, Orsière T, De Méo M, Gallice P, Bideau C, Iniesta D, Pompili J, Bergé-Lefranc JL, and Botta A

Subjects

Adult, Humans, In Situ Hybridization, Fluorescence, Male, Mutagens, Smoking, Welding, X-ray Repair Cross Complementing Protein 1, Centromere ultrastructure, DNA-Binding Proteins genetics, Glutathione Transferase genetics, Micronucleus Tests methods, Occupational Exposure, Polymorphism, Genetic

Abstract

The aims of the present study were to assess clastogenic and aneugenic properties of welding fumes using fluorescent in situ hybridization (FISH) with a human pancentromeric DNA probe. The involvement of genetic polymorphisms in DNA repair genes (p.Arg399Gln of XRCC1 and p.Thr241Met of XRCC3) and in detoxification genes (GSTM1 and GSTT1) on the centromere content of micronuclei (MN) was also evaluated. This study included 27 male welders working without any collective protection device and a control group (n = 30). The welders showed significantly higher levels of chromosome/genome damage compared to the controls. The frequencies of MN and centromere-positive MN (C+MN) per 1,000 binucleated cells were significantly higher in the exposed group than in the control group (7.1 per thousand +/- 3.7 versus 4.9 per thousand +/- 1.8; P = 0.012 and 3.5 per thousand +/- 1.8 versus 2.4 per thousand +/- 1.2; P = 0.018, respectively, Mann-Whitney U-test). The centromere-negative MN (C-MN) frequency was higher in the exposed subjects than in the controls (3.6 per thousand +/- 3.4 versus 2.5 per thousand +/- 1.4), but the Mann-Whitney U-test did not yield a significant result. In the total population, the GSTM1 and GSTT1 polymorphisms significantly affected the frequencies of C-MN and C+MN defined by FISH. GSTM1 positive subjects showed an increased C-MN frequency and GSTT1 null subjects showed an elevated C+MN frequency. When GSTM1 and GSTT1 genotypes were included in multiple regression analysis, the effect of the occupational exposure could better be demonstrated; both C+MN and C-MN were significantly increased in the welders. Our results suggest that the combined analysis of genetic polymorphisms and centromeres in MN may improve the sensitivity of the micronucleus assay in detecting genotoxic effects.

Published

2006

10. Risk assessment of welders using analysis of eight metals by ICP-MS in blood and urine and DNA damage evaluation by the comet and micronucleus assays; influence of XRCC1 and XRCC3 polymorphisms.

Author

Iarmarcovai G, Sari-Minodier I, Chaspoul F, Botta C, De Méo M, Orsière T, Bergé-Lefranc JL, Gallice P, and Botta A

Subjects

Adult, Case-Control Studies, Comet Assay, DNA Damage genetics, Genotype, Humans, Male, Metals adverse effects, Metals pharmacology, Micronucleus Tests, Regression Analysis, Risk Assessment, Spectrophotometry, Atomic, X-ray Repair Cross Complementing Protein 1, DNA Damage drug effects, DNA-Binding Proteins genetics, Metals blood, Metals urine, Polymorphism, Genetic genetics, Welding

Abstract

The aims of the present study were to assess the occupational risk of welders using analysis of metals in biological fluids, DNA damage evaluation by complementary genotoxic endpoints and the incidence of polymorphisms in DNA repair genes. A biomonitoring study was conducted that included biometrology (blood and urinary concentrations of aluminium, cadmium, chromium, cobalt, lead, manganese, nickel, zinc by ICP-MS), comet and cytokinesis-block micronucleus assays in peripheral lymphocytes and genetic polymorphisms of XRCC1 (p.Arg399Gln) and XRCC3 (p.Thr241Met). This study included 60 male welders divided into two groups: group 1 working without any collective protection device and group 2 equipped with smoke extraction systems. A control group (n = 30) was also included in the study. Higher chromium, lead and nickel blood and urinary concentrations were detected in the two groups of welders compared to controls. Statistically differences between welders of group 1 and group 2 were found for blood concentration of cobalt and urinary concentrations of aluminium, chromium, lead and nickel. The alkaline comet assay revealed that welders had a significant increase of OTMchi2 distribution at the end of a work week compared to the beginning; a significant induction of DNA strand breaks at the end of the week was observed in 20 welders out of 30. The cytokinesis-block micronucleus assay showed that welders of group 1 had a higher frequency of chromosomal damage than controls. The XRCC1 variant allele coding Gln amino acid at position 399 was found to be associated with a higher number of DNA breaks as revealed by the comet assay. Increased metal concentrations in biological fluids, DNA breaks and chromosomal damage in lymphocytes emphasized the need to develop safety programmes for welders.

Published

2005

11. PAP IB, a new member of the Reg gene family: cloning, expression, structural properties, and evolution by gene duplication.

Author

Laurine E, Manival X, Montgelard C, Bideau C, Bergé-Lefranc JL, Erard M, and Verdier JM

Subjects

Amino Acid Sequence, Animals, Base Sequence, Bayes Theorem, CHO Cells, Cloning, Molecular, Consensus Sequence, Cricetinae, DNA Primers, Gene Duplication, Genome, Human, Humans, Lectins, C-Type chemistry, Models, Molecular, Molecular Sequence Data, Pancreatitis-Associated Proteins, Phylogeny, Protein Conformation, Proteins, Sequence Alignment, Sequence Homology, Amino Acid, Evolution, Molecular, Lectins, C-Type genetics, Multigene Family

Abstract

Reg proteins are expressed in various organs and are involved in cancers and neurodegenerative diseases. They display a typical C-type lectin-like domain but possess additional highly conserved amino acids. By studying human databases and Expressed Sequence Tags library, we identified a new member called PAP IB. Using probabilistic approaches, we established a phylogenetic tree of eighteen Reg proteins. The dendogram showed that they constitute a superfamily composed of three distinct families (FI to FIII) of paralogues that resulted from duplication. We therefore focused on two proteins, REG Ialpha and PAP IB, belonging to the more closely related FI and FII families, respectively. REG Ialpha and PAP IB share 50% sequence identity. After cloning PAP IB, however, we found that it was expressed almost only in pancreas, unlike REG Ialpha, whose expression is ubiquitous. In addition, by building a model of the structure of PAP IB based on the X-ray structure of REG Ialpha, we observed that the two proteins displayed distinctive surface charge distribution, which may lead to different ligands binding. In spite of their common fold that should result in closely related functions, REG Ialpha and PAP IB are a good example of duplication and divergence, probably with the acquisition of new functions, thus participating in the evolution of the protein repertoire.

Published

2005

12. Low-level arsenite activates the transcription of genes involved in adipose differentiation.

Author

Salazard B, Bellon L, Jean S, Maraninchi M, El-Yazidi C, Orsière T, Margotat A, Botta A, and Bergé-Lefranc JL

Subjects

3T3 Cells, 3T3-L1 Cells, Adipocytes cytology, Animals, CCAAT-Enhancer-Binding Protein-alpha genetics, Cell Line, Cell Proliferation drug effects, Cell Survival drug effects, Dose-Response Relationship, Drug, Gene Expression genetics, Heme Oxygenase (Decyclizing) genetics, Heme Oxygenase-1, Hypoxia-Inducible Factor 1, alpha Subunit, Kruppel-Like Transcription Factors, Membrane Proteins, Mice, PPAR gamma genetics, Reverse Transcriptase Polymerase Chain Reaction, Teratogens pharmacology, Trans-Activators genetics, Transcription Factors genetics, Adipocytes drug effects, Arsenites pharmacology, Cell Differentiation genetics, Gene Expression drug effects

Abstract

In this study we analyzed gene expression in 3T3-F442A pre-adipocyte cells that differentiate in the presence of micro-molar arsenate concentration. Two concentrations of arsenite (As2O3, 0.25 micromol/L and 0.5 micromol/L) were applied for three days with and without insulin (170 nmol/L) and gene expressions were evaluated by quantitative RT-PCR. The genes included genes of oxidative-stress responses: heme-oxygenase-1 (HO1) and the hypoxia inducible factor 1a (HIF1alpha), genes of cell-cycle: c-jun and Kruppel like factor 5 (KLF5), and genes that play important roles in adipose determination: a peroxisome proliferator-activated receptor (PPARgamma) and a CCAAT/ enhancer binding protein (C/EBPalpha). Arsenite induced the expression of HO1, HIF1alpha, KLF5, PPARgamma and C/EBPalpha. These results suggest that under condition of oxidative stress arsenite induces genes that are required for adipose differentiation.

Published

2004

13. Patterns of gene expressions induced by arsenic trioxide in cultured human fibroblasts.

Author

Burnichon V, Jean S, Bellon L, Maraninchi M, Bideau C, Orsière T, Margotat A, Gérolami V, Botta A, and Bergé-Lefranc JL

Subjects

Arsenic Trioxide, Cell Division drug effects, Cell Survival drug effects, Cells, Cultured, Dose-Response Relationship, Drug, Fibroblasts, Humans, Time Factors, Arsenicals pharmacology, Gene Expression Regulation drug effects, Oxides pharmacology

Abstract

Arsenic exposure is associated with several human diseases and particularly, with neoplasia. Although the mechanism of arsenic toxicity is not fully understood, several recent works pointed out the involvement of oxidative stress in arsenic-induced DNA damage that, in living cells, correlates with changes in gene expressions. In cultured human fibroblasts exposed for 24 h to micromolar arsenic concentrations, we studied, using real-time RT-PCR, the expression profile of a limited number of genes: genes coding for a stress protein (HSP70), transcription factors (cJUN, cFOS, ETR103, ETR101 and TTP) and cell cycle or DNA repair proteins (P21, GADD153). We observed that the expression profile of genes followed individual different patterns that can be summed up in early-transient gene expression by contrast to delayed gene expression.

Published

2003

14. The expression of genes induced in melanocytes by exposure to 365-nm UVA: study by cDNA arrays and real-time quantitative RT-PCR.

Author

Jean S, Bideau C, Bellon L, Halimi G, De Méo M, Orsière T, Dumenil G, Bergé-Lefranc JL, and Botta A

Subjects

Cell Differentiation, Cell Division, DNA Repair, Gene Expression Regulation radiation effects, Humans, Melanocytes metabolism, Oligonucleotide Array Sequence Analysis, Polymerase Chain Reaction methods, Reverse Transcriptase Polymerase Chain Reaction, Genes, Melanocytes radiation effects, Ultraviolet Rays

Abstract

Ultraviolet A radiation (UVA; 320-400 nm) constitutes more than 90% of the terrestrial UV solar energy. This type of radiation generates reactive oxygen species and consequently induces DNA damage. UVA irradiation is now considered to be an important carcinogen agent especially in the development of melanoma. UVA radiation is known to activate several pathways in mammalian cells. We have used cDNA arrays to analyze differential gene expression in primary cultures of human melanocytes in response to 365-nm UVA. Among 588 genes studied, 11 were overexpressed. These genes included genes involved in cell cycle regulation (GADD45, CIP1/WAF1), in stress response (HSP70, HSP40, HSP86), in apoptosis (GADD153, tristetraproline) and genes encoding transcription factors (EGR-1, ETR-101, c-JUN, ATF4). This coordinate gene regulation was confirmed by real-time quantitative RT-PCR.

Published

2001

15. Association of APOE promoter but not A2M polymorphisms with risk of developing Alzheimer's disease.

Author

Halimi G, Duplan L, Bideau C, Iniesta D, Berthézène P, Oddoze C, Verdier JM, Michel B, and Bergé-Lefranc JL

Subjects

Aged, Alleles, Apolipoprotein E4, France, Gene Frequency, Genetic Predisposition to Disease, Genotype, Humans, Linkage Disequilibrium, Reference Values, Risk Factors, White People, Alzheimer Disease genetics, Apolipoproteins E genetics, Polymorphism, Genetic, Promoter Regions, Genetic, alpha-Macroglobulins genetics

Abstract

The APOE4 allele is widely accepted as a major risk factor for late-onset Alzheimer's disease (AD). Recently, it has been reported that polymorphisms in the APOE promoter and in the alpha2-macroglobulin gene (A2M) are associated with AD. We have analyzed the distribution of APOE alleles, -219T/G APOE promoter polymorphism, and A2M/A2Mdel polymorphism in a large case-control study. Our results showed that APOE genotype was the only informative marker of AD risk contrary to -219T/G and A2M/A2Mdel polymorphism. In AD patients however, a strong linkage disequilibrium was observed between the T allele of -219T/G polymorphism and APOE4 allele. This result indicates that -219T/G APOE promoter polymorphism is a risk factor for AD by increasing the APOE4-associated risk.

Published

2000

16. ARP3beta, the gene encoding a new human actin-related protein, is alternatively spliced and predominantly expressed in brain neuronal cells.

Author

Jay P, Bergé-Lefranc JL, Massacrier A, Roessler E, Wallis D, Muenke M, Gastaldi M, Taviaux S, Cau P, and Berta P

Subjects

Actin-Related Protein 3, Actins physiology, Amino Acid Sequence, Animals, Base Sequence, Blotting, Northern, Brain embryology, Central Nervous System metabolism, Chromosomes, Human, Pair 7, DNA, Complementary metabolism, Exons, Humans, In Situ Hybridization, In Situ Hybridization, Fluorescence, Introns, Molecular Sequence Data, Neurons metabolism, Pseudogenes, RNA, Messenger metabolism, Rats, Reverse Transcriptase Polymerase Chain Reaction, Tissue Distribution, Actins biosynthesis, Actins genetics, Alternative Splicing, Brain metabolism, Cytoskeletal Proteins

Abstract

A cDNA encoding a new human actin-related protein (ARP) was cloned. The corresponding protein is highly conserved with the previously described ARP3 protein, suggesting that it represents a second isoform of the human ARP3 subfamily. This new actin-related protein was subsequently named ARP3beta and represents the second example of multiple isoforms of an actin-related protein in a single organism. The ARP3beta gene was mapped to chromosome band 7q34, centromeric to Sonic Hedgehog. Gene structure analysis revealed that at least part of the observed ARP3beta mRNA heterogeneity is caused by alternative splicing resulting in exon skipping. Transcripts produced after exon 2 skipping are predicted to encode truncated products, whose functionality is still unclear. An ARP3beta pseudogene was detected on chromosome 2p11 by database searching. Several ARP3beta mRNA species were detected by Northern blotting and their abundance varied importantly among tissues: the highest expression levels were detected in fetal and adult brain, whereas lower levels were observed in liver, muscle and pancreas. In contrast, ARP3 mRNAs were detected in all tissues tested. Using in situ hybridization, the expression of ARP3beta in brain was shown to be restricted to neurons and epithelial cells from choroid plexus. This suggests a specific function for ARP3beta in the physiology of the development and/or maintenance of distinct subsets of nerve cells.

Published

2000

17. The human growth factor-inducible immediate early gene, CYR61, maps to chromosome 1p.

Author

Jay P, Bergé-Lefranc JL, Marsollier C, Méjean C, Taviaux S, and Berta P

Subjects

Base Sequence, Chromosome Mapping, Cloning, Molecular, Cysteine-Rich Protein 61, Gene Expression, Humans, In Situ Hybridization, Fluorescence, Molecular Sequence Data, Proto-Oncogene Mas, RNA, Messenger genetics, Sequence Alignment, Sequence Homology, Amino Acid, Chromosomes, Human, Pair 1, Growth Substances genetics, Immediate-Early Proteins genetics, Intercellular Signaling Peptides and Proteins

Abstract

Complementary DNA encoding the human CYR61 protein was isolated from human embryonic tissues and mapped to chromosome 1p22-p31. We show that CYR61 encodes a 381 amino acid protein rich in cysteine and proline residues that is strongly conserved with the mouse homologue. Sequence analysis reveals the presence of several distinct protein domains which confer a mosaic structure to this protein and makes human CYR61 a member of a recently described growth regulator family that includes several proto-oncogene products. From our results we hypothesize that this new immediate early gene may play a role in cell commitment during embryogenesis and more generally in the control of cell proliferation.

Published

1997

18. Isolation and regional mapping of cDNAs expressed during early human development.

Author

Jay P, Diriong S, Taviaux S, Roeckel N, Mattéi MG, Audit M, Bergé-Lefranc JL, Fontès M, and Berta P

Subjects

Cloning, Molecular, Embryo, Mammalian, Humans, In Situ Hybridization, Fluorescence, Molecular Sequence Data, Chromosome Mapping, DNA, Complementary, Embryonic and Fetal Development genetics, Gene Expression

Abstract

A cDNA sequencing project was initiated with the aim of isolating and mapping new genes expressed during early human development. A human embryo cDNA library was constructed, and a prescreening procedure was used to select cDNAs corresponding to poorly transcribed genes. Partial sequences were generated from one or both ends of 231 cDNA clones, and sequence comparison with genetic databases revealed that 28% were already annotated genes, 42% matched with partial sequences expressed sequence tags that had already been detected, 3% contained no insert, 5% were highly similar to sequences from other species, and 23% of the cDNAs appeared to be unknown in genetic databases. All new sequences were deposited in public genetic databases, and most of the corresponding cDNAs were regionally mapped on human chromosome bands using both fluorescence and radioactive in situ hybridization. Several cDNAs colocalized with critical regions of the genome regarding mapped disorders, thus providing candidate genes for human genetic diseases.

Published

1997

19. Characterization of the human jumonji gene.

Author

Bergé-Lefranc JL, Jay P, Massacrier A, Cau P, Mattei MG, Bauer S, Marsollier C, Berta P, and Fontes M

Subjects

Amino Acid Sequence, Animals, Chromosome Mapping, Cloning, Molecular, DNA, Complementary analysis, Female, Gene Expression Regulation, Developmental, Humans, Mice, Molecular Sequence Data, Polycomb Repressive Complex 2, Pregnancy, Sequence Alignment, Sequence Analysis, Sequence Homology, Amino Acid, Chromosomes, Human, Pair 6, DNA, Complementary genetics, Nerve Tissue Proteins genetics

Abstract

While constructing a cDNA library of human embryos, we have isolated a clone homologous to jumonji, a mouse gene required for neural tube formation. We have determined the complete coding sequence of the human homologue (JMJ) and deduced the amino acid sequence of the putative protein. We show here that human and mouse jumonji putative proteins are homologous and present 90% identity. During human embryogenesis, JMJ mRNAs are predominantly expressed in neurons and particularly in dorsal root ganglion cells. They are also expressed in neurons of human adult cerebral cortex. In view of these observations, we propose JMJ as a candidate gene for developmental defects of the central nervous system in the human. The human JMJ gene maps at position 6p24-6p23.

Published

1996

20. Cloning of the human homologue of the TGF beta-stimulated clone 22 gene.

Author

Jay P, Ji JW, Marsollier C, Taviaux S, Bergé-Lefranc JL, and Berta P

Subjects

Amino Acid Sequence, Animals, Base Sequence, Chromosome Mapping, Chromosomes, Human, Pair 13, Cloning, Molecular, DNA, Complementary genetics, Gene Expression, Humans, Mice, Molecular Sequence Data, RNA, Messenger genetics, Rats, Sequence Alignment, Sequence Homology, Amino Acid, Swine, Genes, Immediate-Early, Proteins genetics, Repressor Proteins, Transforming Growth Factor beta pharmacology

Abstract

We have isolated the human homologue if the TGF beta-stimulated clone 22 gene from a human embryo cDNA library. This gene maps to the q14 region of chromosome 13. Its deduced amino acid sequence is almost 99% identical to that of mouse or rat proteins and includes a putative leucine zipper motif. An abundant major transcript of 1.8 kb and in some instances an additional 5 kb transcript were detected by Northern blotting of several human tissues. The TSC-22 protein has been shown to be well conserved across evolution as evidenced by the existence of a Drosophila homologue. These observations prompt discussion on the strong conservation of TSC-22 during evolution but also on its general function as a primary response gene expressed either when stimulated by several different factors during early human development, or in the adult in response to inducing differentiation signals.

Published

1996

21. A limited genomic region contains the human REG and REG-related genes.

Author

Bartoli C, Dagorn JC, Fontes M, and Bergé-Lefranc JL

Subjects

Base Sequence, Chromosome Mapping, Chromosomes, Artificial, Yeast genetics, Cosmids, DNA Primers, Gene Expression, Humans, Lithostathine, Molecular Sequence Data, Pseudogenes, Calcium-Binding Proteins genetics, Nerve Tissue Proteins

Abstract

A glycoprotein expressed in exocrine pancreas (where it has been called lithostathine) and endocrine pancreas (where it has been called the regeneration protein) is encoded by a gene (REG) which maps to 2p12. A REG-related sequence (REGL) is also located in 2p12 and expressed in the pancreas. Here we describe the physical mapping of these genes within a 100-kb genomic region. A YAC clone was converted into an ordered cosmid contig. We constructed a restriction map of the cosmid contig and localized the loci corresponding to the genes. A third REG-related sequence also maps to this region. Although this sequence was previously described as a pseudogene, we show here that it is also expressed in the pancreas.

Published

1995

22. A gene homologous to the reg gene is expressed in the human pancreas.

Author

Bartoli C, Gharib B, Giorgi D, Sansonetti A, Dagorn JC, and Bergé-Lefranc JL

Subjects

Amino Acid Sequence, Base Sequence, Cloning, Molecular, DNA, Humans, Lithostathine, Liver metabolism, Molecular Sequence Data, RNA, Messenger metabolism, Sequence Homology, Amino Acid, Calcium-Binding Proteins genetics, Gene Expression, Nerve Tissue Proteins, Pancreas metabolism, Phosphoproteins genetics

Abstract

We have determined the nucleotide sequence of regl a human genomic DNA fragment homologous to the reg gene which is expressed in the exocrine pancreas and regenerating islets. Sequence comparisons of reg and regl suggested similar exon-intron organisation. Based on this assumption, specific oligonucleotides for regl exons were used to demonstrate expression of the regl gene in pancreas and liver. The proteins encoded by reg and regl comprise 166 amino acids and differ by 22 amino acids only.

Published

1993

23. Human ribosomal RNA gene repeats are localized in the dense fibrillar component of nucleoli: light and electron microscopic in situ hybridization in human Sertoli cells.

Author

Wachtler F, Schöfer C, Mosgöller W, Weipoltshammer K, Schwarzacher HG, Guichaoua M, Hartung M, Stahl A, Bergé-Lefranc JL, and Gonzalez I

Subjects

Cell Nucleolus chemistry, Humans, Male, Microscopy, Electron, Nuclear Matrix ultrastructure, Nucleic Acid Hybridization, Cell Nucleolus ultrastructure, DNA, Ribosomal analysis, Repetitive Sequences, Nucleic Acid, Sertoli Cells ultrastructure

Abstract

The distribution of the human ribosomal gene repeat within human Sertoli cell nucleoli was investigated with the help of DNA-DNA in situ hybridization at the light and electron microscopic level. Probes from both the transcribed part of the gene repeat and the "non-transcribed" spacer were found to hybridize predominantly to the dense fibrillar component of nucleoli. It therefore can be concluded that the dense fibrillar component of nucleoli is the major site of the intranucleolar location of the ribosomal DNA. This holds true not only for the dense fibrillar component adjacent to fibrillar centers, but also for the dense fibrillar component remote from the fibrillar centers.

Published

1992

24. Triiodothyronine control of ATP-citrate lyase and malic enzyme during differentiation of a murine preadipocyte cell line.

Author

Gharbi-Chihi J, Facchinetti T, Bergé-Lefranc JL, Bonne J, and Torresani J

Subjects

ATP Citrate (pro-S)-Lyase genetics, Adipose Tissue enzymology, Adipose Tissue physiology, Animals, Cell Differentiation drug effects, Cell Differentiation physiology, Cells, Cultured, Gene Expression Regulation, Enzymologic drug effects, Gene Expression Regulation, Enzymologic physiology, Malate Dehydrogenase genetics, Mice, RNA Processing, Post-Transcriptional genetics, RNA, Messenger genetics, RNA, Messenger metabolism, Stem Cells enzymology, Stem Cells physiology, ATP Citrate (pro-S)-Lyase metabolism, Adipose Tissue cytology, Malate Dehydrogenase metabolism, Stem Cells cytology, Triiodothyronine pharmacology

Abstract

In the Ob 17 preadipocyte cell line, during adipose differentiation, T3 amplified the progressive expression of two enzymes of the lipogenic pathway, ATP-citrate lyase (ATP-CL) and malic enzyme (ME) as previously described for fatty acid synthase (FAS) and fatty acid synthesis, and in the same time-period of development. However, the stimulation by T3 was sustained at late stages of differentiation whereas it declined in FAS studies. The stimulation was preceded by an increase in the relative abundance of the specific mRNAs. Two ME mRNA species were detected (21S and 27S) and found to be differently distributed. Their abundance was asynchronously increased by T3 with a predominant effect on the 21S species. Culture of the cells in a thyroid-hormone depleted medium prevented any significant increase of ME activity. Early inclusion of T3 largely restored ME development whereas late elimination of T3 only moderately impaired it. It is suggested that T3 plays a crucial role at an early step of adipose differentiation, this leading to an increased expression of a set of late adipose phenotypes such as several lipogenic enzymes.

Published

1991

25. The peculiar spectrum of beta-thalassemia genes in Tunisia.

Author

Chibani J, Vidaud M, Duquesnoy P, Bergé-Lefranc JL, Pirastu M, Ellouze F, Rosa J, and Goossens M

Subjects

Genetic Markers, Humans, Tunisia, Globins genetics, Mutation, Thalassemia genetics

Abstract

We have determined the spectrum of mutations producing beta-thalassemia (beta-thal) in Tunisia by direct DNA analysis using hybridization with allele-specific oligonucleotide probes and restriction endonuclease assay. In all, 34 unrelated beta-thal patients originating from different parts of the country were available for study. The beta-globin gene cluster of each was subjected to haplotype analysis, and on the basis of this analysis, we tested each patient's DNA for one or more mutations previously shown to be linked to that haplotype. We identified four previously unreported haplotypes and found that this population differs from others in Mediterranean areas in the frequency of the beta-thal haplotypes, the unexpected observation being the high frequency of haplotype IX. Six different point mutations were found, accounting for 62% of beta-thal genes in this Tunisian population. The molecular defects known to be the most frequent in Mediterraneans (nonsense codon 39, IVS1 nt 110, IVS1 nt 6) only make up 37% of the mutant genes. One as yet undescribed mutation (IVS1 nt 2 T----G) was identified by molecular cloning and sequencing. Our results should help the implementation of a prenatal diagnosis program for beta-thal in Tunisia.

Published

1988

26. The mRNA transcripts from a mutant beta-globin gene derived from splicing at preferential cryptic sites.

Author

Lossi AM and Bergé-Lefranc JL

Subjects

Base Composition, Blotting, Southern, Cells, Cultured, DNA analysis, Erythrocytes analysis, Globins analysis, Homozygote, Humans, Introns, Molecular Probe Techniques, Mutation, Reticulocytes analysis, Thalassemia genetics, Globins genetics, RNA Splicing, RNA, Messenger analysis, Transcription, Genetic

Abstract

We have analyzed mRNA transcripts from beta-globin genes carrying a homozygous point mutation at the 5' splicing site of the first intron, using a method allowing in vivo analysis of mRNA transcripts. As expected, this mutation decreases normal splicing of mRNA when cryptic splicing are utilized. We have observed that, in reticulocytes, most mature mRNA transcribed from beta-globin genes derives from specific sites of abnormal splicing. Our results differ from those previously obtained using mutant beta-globin genes introduced in cultured cells and indicate a preferential processing of the abnormal globin mRNA species in red cell precursors.

Published

1989

27. Quantitative in situ hybridization of 3H-labeled complementary deoxyribonucleic acid (cDNA) to the messenger ribonucleic acid of thyroglobulin in human thyroid tissues.

Author

Bergé-Lefranc JL, Cartouzou G, Bignon C, and Lissitzky S

Subjects

Adenoma analysis, Goiter metabolism, Graves Disease metabolism, Humans, Thyroid Gland analysis, Thyroid Neoplasms analysis, Tritium, DNA, Nucleic Acid Hybridization, RNA, Messenger analysis, Thyroglobulin biosynthesis, Thyroid Diseases metabolism

Abstract

Thyroglobulin (Tgb) mRNA content was studied in human thyroid tissues using liquid hybridization and in situ hybridization. Liquid hybridization revealed no differences in mRNA content, except in the case of colloid adenoma in which a lower amount of Tgb mRNA was found. Conditions for quantitative in situ hybridization of [3H]DNA complementary to the mRNA of Tgb are described. In situ hybridization allowed correlation of the morpho-functional state of the follicles and their content of Tgb mRNA.

Published

1983

28. Localization of the thyroglobulin gene by in situ hybridization to human chromosomes.

Author

Bergé-Lefranc JL, Cartouzou G, Mattéi MG, Passage E, Malezet-Desmoulins C, and Lissitzky S

Subjects

Chromosome Banding, Humans, Chromosome Mapping, Chromosomes, Human, 6-12 and X ultrastructure, DNA, Recombinant, Genes, Nucleic Acid Hybridization, Thyroglobulin genetics

Abstract

The human thyroglobulin gene was mapped by in situ hybridization whereby a 3H-labeled recombinant plasmid DNA containing a fragment of 2.3 kilobases of human thyroglobulin gene was hybridized to human chromosome preparations. A high proportion (25%) of hybridized metaphases exhibited silver grains at the distal portion of the long arm of chromosome 8. Analysis of the grain position at this site indicated that the chromosomal localization of the human thyroglobulin gene was 8q242-8q243.

Published

1985

29. Precise in situ localization of NCAM, ETS1, and D11S29 on human meiotic chromosomes.

Author

Bello MJ, Salagnon N, Rey JA, Guichaoua MR, Bergé-Lefranc JL, Jordan BR, and Luciani JM

Subjects

Chromosome Mapping, DNA Probes, Glycoproteins genetics, Humans, Male, Meiosis, Nucleic Acid Hybridization, Testis ultrastructure, Chromosomes, Human, Pair 11, DNA genetics, Membrane Proteins genetics, Proto-Oncogenes genetics

Abstract

In order to sublocalize NCAM, ETS1, and the anonymous DNA fragment D11S29 within 11q23, in situ hybridization was performed on pachytene bivalents. Analysis of the grain distribution within the band 11q23 indicated that the chromosomal sublocalization of both NCAM and D11S29 was in 11q23.1, whereas ETS1 was found to be localized in 11q23.3. These results clearly demonstrate the usefulness of in situ hybridization applied to pachytene bivalents to obtain accurate gene sublocalization.

Published

1989

30. Structural basis for Robertsonian translocations in man: association of ribosomal genes in the nucleolar fibrillar center in meiotic spermatocytes and oocytes.

Author

Stahl A, Luciani JM, Hartung M, Devictor M, Bergé-Lefranc JL, and Guichaoua M

Subjects

Cell Nucleolus ultrastructure, DNA, Ribosomal, Female, Fetus physiology, Humans, Male, Microscopy, Electron, Oocytes ultrastructure, Pregnancy, Spermatocytes ultrastructure, Spermatogonia physiology, Spermatogonia ultrastructure, Cell Nucleolus physiology, DNA genetics, Meiosis, Oocytes physiology, Ovum physiology, Spermatocytes physiology, Spermatozoa physiology, Translocation, Genetic

Abstract

The spatial relationships of acrocentric chromosomes were studied during prophase I of meiosis in human oocytes and spermatocytes by using cytogenetic techniques, electron microscopy, and in situ hybridization. Ultrastructural investigations revealed an ordered arrangement of nucleolar bivalents at the zygotene and pachytene stages. The end of the bivalent corresponding to the cytological satellite was consistently attached to the nuclear envelope. The fibrillar center of the nucleolus always contained rDNA chromatin fibers emanating from the secondary constriction region. Association of ribosomal genes from two bivalents in the same fibrillar center was frequently observed. Ultrastructural studies demonstrated the close proximity of chromatids in the short arm region of the involved nonhomologous acrocentrics. A breakage/reunion model based on our data can explain the formation of all observed types of Robertsonian translocations: monocentrics and dicentrics with or without rDNA.

Published

1983

31. Thyroglobulin structure and function: recent advances.

Author

Malthièry Y, Marriq C, Bergé-Lefranc JL, Franc JL, Henry M, Lejeune PJ, Ruf J, and Lissitzky S

Subjects

Amino Acid Sequence, DNA isolation & purification, Gene Expression Regulation, Humans, Molecular Sequence Data, Protein Conformation, RNA, Messenger isolation & purification, Thyroglobulin genetics, Thyroglobulin physiology

Abstract

Thyroglobulin is a large-size iodoglycoprotein specific to thyroid tissue and is the substrate for the synthesis of thyroid hormones, thyroxine and 3,5,3'-triiodothyronine. Recent studies, which greatly benefited from recombinant DNA methodologies, improved the knowledge of several structural features of this dimeric protein and permitted insights into some structure-function relationships. Analysis-function of the primary structure of the human thyroglobulin monomer revealed several main characteristics: 1) 3 types of internal homologies; 2) extensive homology with the bovine thyroglobulin monomer and known partial sequences in the thyroglobulins of other mammalian species; 3) significant homologies with 2 other non-thyroid proteins (acetylcholinesterase and the invariant chain of the Ia class II histocompatibility antigen); 4) a terminal localization of the hormonogenic sites at both ends of the monomer. Current studies aim at determining conformational characteristics, understanding the molecular mechanisms of thyroid hormone formation and unraveling those interactions which in the thyroid cell and the thyroid follicle will permit this large pro-hormone to synthesize and release a few small thyroid hormone molecules. A more precise knowledge of this molecule in higher vertebrates and during evolution would impart valuable information concerning thyroid pathology, since thyroglobulin has been implicated in some genetic and in autoimmune thyroid diseases.

Published

1989

32. A further case of beta-thalassemia with an homozygous T----C substitution at the donor splice site of the first intervening sequence of the beta-globin gene.

Author

Lossi AM, Milland M, Bergé-Lefranc JL, Lena-Russo D, and Perrimond H

Subjects

Base Sequence, Child, Preschool, DNA Mutational Analysis, Female, Genes, Humans, Introns, Molecular Sequence Data, Globins genetics, Thalassemia genetics

Published

1989

33. Molecular weight of the thyroglobulin messenger RNA of sheep thyroid gland.

Author

Chebath J, Chabaud O, Bergé-Lefranc JL, Cartouzou G, and Lissitzky S

Subjects

Animals, Kinetics, Molecular Weight, Poly A analysis, Polyribosomes metabolism, RNA, Ribosomal metabolism, Sheep, Thyroglobulin biosynthesis, RNA, Messenger isolation & purification, RNA, Messenger metabolism, Thyroid Gland metabolism

Published

1977

34. Cloning of four DNA fragments complementary to human thyroglobulin messenger RNA.

Author

Bergé-Lefranc JL, Cartouzou G, Malthiéry Y, Perrin F, Jarry B, and Lissitzky S

Subjects

Biotransformation, Cloning, Molecular, DNA isolation & purification, DNA Restriction Enzymes metabolism, Endonucleases metabolism, Escherichia coli metabolism, Humans, Nucleic Acid Hybridization, Placental Hormones metabolism, Plasmids, RNA-Directed DNA Polymerase metabolism, Ribonucleases antagonists & inhibitors, Single-Strand Specific DNA and RNA Endonucleases, DNA, Recombinant isolation & purification, Deoxyribonucleases, Type II Site-Specific, Poly A genetics, RNA, Messenger genetics, Thyroglobulin genetics

Abstract

Human thyroglobulin mRNA was isolated from Graves' goitres by size selection of total poly(A)-rich RNA in a sucrose gradient. It sedimented at 33 S, as in other mammalian species, and showed a single component of approximately 8500 bases by gel electrophoresis. cDNA was synthesized from the 33-S RNA by using reverse transcriptase in the presence of human placenta ribonuclease inhibitor and in conditions allowing the formation of long transcripts. The latter was made double-stranded using reverse transcriptase and blunt-ended with nuclease S1. After tailing with dCTP and terminal transferase, the double-stranded cDNA was annealed to pBR322 DNA that had been cleaved at the endonuclease PstI site and tailed with dGTP. The resulting plasmids were used to transform Escherichia coli C600 cells and four cloned recombinants were selected. Each plasmid DNA was shown to contain a sequence complementary to human thyroglobulin mRNA by hybridization with a labeled 33-S mRNA, visualization of cDNA . mRNA hybrids by electron microscopy and filter hybridization selection of mRNA directing the synthesis of immunologically related thyroglobulin peptides in the reticulocyte lysate. The four inserted DNA sequences were 1400 - 1800 base pairs long, two of them showing an homologous sequence of 1100 base pairs. Together, the four cloned DNA fragments represented 63% of the 8500 bases of human thyroglobulin mRNA.

Published

1981

35. The association of the nucleolus and the short arm of acrocentric chromosomes with the XY pair in human spermatocytes: its possible role in facilitating sex-chromosome acrocentric translocations.

Author

Stahl A, Hartung M, Devictor M, and Bergé-Lefranc JL

Subjects

Cell Nucleolus ultrastructure, Chromosome Banding, Humans, Male, Microscopy, Electron, Spermatogenesis, Meiosis, Nucleolus Organizer Region, Translocation, Genetic, Y Chromosome

Abstract

Sex vesicle-nucleolus association was observed in 12% of zygotene and pachytene human spermatocytes using Giemsa and NOR-silver stained preparations. The silver-positive area of the nucleolus, corresponding to the nucleolus organizer (NOR), was usually close to the XY pair. C-banding frequently showed the terminal chromomere, formed by the condensed short arm of an acrocentric bivalent, attached to the sex vesicle. When a nucleolus produced by transcription of rDNA was connected to the short arm, it seemed to be secondarily associated with the sex vesicle. Non-transcribed ribosomal genes, which did not form a nucleolus, were revealed by in situ hybridization. Autoradiographs showed the rDNA-containing short arm of acrocentric bivalents associated with the sex vesicle in 18% of spermatocytes. The difference with the frequency of nucleolus-XY pair association was partially explained by the presence of inactive ribosomal genes. Moreover, electron microscopy showed that the dimensions of the newly formed nucleoli at early zygotene did not exceed 0.5 micron; they can be missed in light microscope investigations. From early zygotene to late pachytene, close relationships were observed between the sex vesicle chromatin and that of the associated acrocentric bivalent, especially in the short arm region. These relationships might explain the frequent involvement of acrocentrics in Y-autosome and X-autosome translocations occurring during male meiosis.

Published

1984

36. Oligonucleotide screening of beta thalassemia mutations in the south east of France.

Author

Milland M, Bergé-Lefranc JL, Lena D, and Cartouzou G

Subjects

Alleles, DNA genetics, Ethnicity, France, Gene Frequency, Humans, Nucleic Acid Hybridization, Oligodeoxyribonucleotides genetics, Mutation, Thalassemia genetics

Abstract

France is a non-endemic region for beta thalassemia. In this country, the sporadic cases of Cooley's disease encountered affect almost constantly subjects of Mediterranean origin. In this report, we have screened, using oligonucleotide probes, the distribution of the main beta thalassemia mutations present in the population of South-eastern France whose origins lie in the mixing of several Mediterranean ethnic groups. Among 105 beta thalassemia chromosomes, we have observed a limited number of alleles, since, by using oligonucleotide probes for six mutations, we have characterized the molecular defect in 90% of the chromosomes. The four main mutations were found in more than 85% of the chromosomes and the others in about 5%. The distribution of the beta thalassemia mutations within the various ethnic groups was determined.

Published

1987

37. Quantification of thyroglobulin messenger RNA by in situ hybridization in differentiated thyroid cancers. Difference between well-differentiated and moderately differentiated histologic types.

Author

Bergé-Lefranc JL, Cartouzou G, De Micco C, Fragu P, and Lissitzky S

Subjects

Autoradiography, Cell Differentiation, Cell Fractionation, DNA, Recombinant, Humans, Nucleic Acid Hybridization, Polyribosomes metabolism, Protein Biosynthesis, RNA, Neoplasm metabolism, Thyroid Neoplasms pathology, RNA, Messenger metabolism, Thyroglobulin genetics, Thyroid Neoplasms genetics

Abstract

Thyroglobulin messenger RNA (mRNA) was located and quantified in tissue sections of differentiated human thyroid cancers by in situ hybridization using cloned complementary DNA probes. The cells of the well-differentiated follicular and papillary forms contained similar levels of thyroglobulin mRNA, corresponding to about 2000 copies per cell. In contrast, cells of moderately differentiated thyroid cancers contained about two to three times less thyroglobulin mRNA. It was also found that thyroglobulin mRNA was present almost exclusively in polyribosomes under the form of heavy polyribosomes actively synthesizing thyroglobulin. It is suggested that in situ hybridization method allows localization of specific mRNA in differentiated thyroid cancers and correlation with the level of differentiation of the cells.

Published

1985