Your search keyword '"Sylvie Mazoyer"' showing total 7 results

1. The 185delAG mutation (c.68_69delAG) in theBRCA1 gene triggers translation reinitiation at a downstream AUG codon

Author

Sylvie Mazoyer, Almoutassem B. Zetoune, Monique Buisson, Olga Anczuków, and Mark D. Ware

Subjects

endocrine system diseases, Blotting, Western, Nonsense-mediated decay, Population, Codon, Initiator, Biology, Transfection, Start codon, Genetics, Protein biosynthesis, Humans, Coding region, education, Genetics (clinical), Sequence Deletion, Translation reinitiation, education.field_of_study, Base Sequence, Models, Genetic, BRCA1 Protein, Blotting, Northern, Molecular biology, Codon, Nonsense, Protein Biosynthesis, Mutation, Mutation (genetic algorithm), HeLa Cells, Plasmids

Abstract

The 185delAG mutation (c.68_69delAG; ter39) in the BRCA1 gene is a founder Jewish Ashkenazi mutation that is carried by 1% of this population and has been identified in thousands of breast or ovarian cancer patients. We have previously described that transcripts bearing this mutation, as well as transcripts bearing the 188del11 mutation (c.71_81del; ter36), are not degraded by nonsense-mediated mRNA decay (NMD), contrary to our observations of other truncating mutations that introduce premature termination codons (PTCs) farther downstream in the coding sequence [Perrin-Vidoz et al., 2002]. To test the hypothesis that these two mutations fail to trigger NMD because of translation reinitiation, we have constructed BRCA1 minigenes and studied their protein expression after transient expression in HeLa cells. We show here that in the presence of a (PTC) at position 36 or 39, translation reinitiation occurs in the BRCA1 minigenes at position 128.

Published

2006

2. Genomic rearrangements in theBRCA1 andBRCA2 genes

Author

Sylvie Mazoyer

Subjects

Genotype, endocrine system diseases, Genes, BRCA2, Molecular Sequence Data, Genes, BRCA1, Breast Neoplasms, Biology, Exon, Germline mutation, Genetics, Genetic predisposition, Humans, Genetic Predisposition to Disease, Genetic Testing, skin and connective tissue diseases, Gene, Germ-Line Mutation, Genetics (clinical), Chromosome Aberrations, Ovarian Neoplasms, Point mutation, Breakpoint, Founder Effect, Female, Founder effect

Abstract

Mutations in the BRCA1 and BRCA2 genes predispose women to breast and ovarian cancer. BRCA1 and BRCA2 are 83 and 86 kb long, with coding sequences of 5.7 and 10.2 kb, scattered over 22 and 26 coding exons, respectively. The large majority of the alterations identified in these genes are point mutations and small insertions/deletions. However, an increasing number of large genomic rearrangements are being identified, especially in BRCA1. This review gives a brief overview of the techniques used to screen the BRCA1 and BRCA2 genes for large rearrangements, and describes those for which the breakpoints have been characterized. The principal mechanisms that are thought to lead to their formation, founder effects, and recombination hotspots, are also discussed.

Published

2005

3. Guidelines for splicing analysis in molecular diagnosis derived from a set of 327 combined in silico/in vitro studies on BRCA1 and BRCA2 variants

Author

Florent Soubrier, Dominique Stoppa-Lyonnet, Françoise Bonnet, Sylvie Mazoyer, Monique Buisson, Joanna Sokolowska, Brigitte Bressac-de Paillerets, Françoise Révillion, Mario Tosi, Agnès Hardouin, Etienne Rouleau, Myriam Bronner, Danielle Muller, Claude Houdayer, Olga M. Sinilnikova, Cédrick Lefol, Violaine Bourdon, Hagay Sobol, Pascaline Gaildrat, Sophie Krieger, Florence Coulet, Michel Barrois, Nicolas Sevenet, Virginie Caux-Moncoutier, Audrey Remenieras, Jean-Philippe Vert, Rosette Lidereau, and Mélanie Léoné

Subjects

Genetics, BRCA2 Protein, BRCA1 Protein, In silico, RNA Splicing, Large series, Context (language use), Exons, Biology, Set (abstract data type), Unknown Significance, RNA splicing, Humans, splice, Female, Pathology, Molecular, Enhancer, Genetics (clinical)

Abstract

Assessing the impact of variants of unknown significance (VUS) on splicing is a key issue in molecular diagnosis. This impact can be predicted by in silico tools, but proper evaluation and user guidelines are lacking. To fill this gap, we embarked upon the largest BRCA1 and BRCA2 splice study to date by testing 272 VUSs (327 analyses) within the BRCA splice network of Unicancer. All these VUSs were analyzed by using six tools (splice site prediction by neural network, splice site finder (SSF), MaxEntScan (MES), ESE finder, relative enhancer and silencer classification by unanimous enrichment, and human splicing finder) and the predictions obtained were compared with transcript analysis results. Combining MES and SSF gave 96% sensitivity and 83% specificity for VUSs occurring in the vicinity of consensus splice sites, that is, the surrounding 11 and 14 bases for the 5' and 3' sites, respectively. This study was also an opportunity to define guidelines for transcript analysis along with a tentative classification of splice variants. The guidelines drawn from this large series should be useful for the whole community, particularly in the context of growing sequencing capacities that require robust pipelines for variant interpretation.

Published

2011

4. Does the nonsense-mediated mRNA decay mechanism prevent the synthesis of truncated BRCA1, CHK2, and p53 proteins?

Author

Olga Anczuków, Olga M. Sinilnikova, Monique Buisson, Almoutassem B. Zetoune, Sylvie Mazoyer, Mark D. Ware, and Dominique Stoppa-Lyonnet

Subjects

RNA Stability, Mutant, Cell, Nonsense-mediated decay, Biology, Protein Serine-Threonine Kinases, medicine.disease_cause, Mutant protein, Cell Line, Tumor, Genetics, medicine, Humans, RNA, Messenger, Allele, Gene, Genetics (clinical), Alleles, Mutation, BRCA1 Protein, RNA, Molecular biology, Androstadienes, Checkpoint Kinase 2, medicine.anatomical_structure, Codon, Nonsense, Tumor Suppressor Protein p53, Wortmannin, HeLa Cells

Abstract

The nonsense-mediated mRNA decay (NMD) mechanism is an evolutionarily conserved process ensuring the degradation of transcripts carrying premature termination codon(s). NMD is believed to prevent the synthesis of truncated proteins that could be detrimental to the cell. However, although numerous studies have assessed the efficiency of this mechanism at the mRNA level, data are lacking in regard to whether NMD fulfills its expected goal at the protein level. In this study, we have investigated whether endogenous alleles of breast cancer predisposing genes carrying nonsense codons were able to produce detectable amounts of truncated proteins in lymphoblastoid cell lines. A total of 20 truncating BRCA1 mutations were analyzed, along with the 1100delC CHEK2 and the 770delT TP53 mutations. All the studied alleles triggered NMD, the amount of mutant transcript ranging from 16 to 63% of that of the wild-type species. We found that BRCA1 and CHK2 truncated proteins could not be detected, even when NMD was inhibited. This suggests that BRCA1 and CHK2 truncated proteins are highly unstable. Conversely, the p53 protein encoded by the 770delT allele is as abundant as the wild-type protein, as removal of the C-terminal p53 domain leads to a stabilized mutant protein, whose abundance is markedly increased when NMD is inhibited. Therefore, our results show that it is not possible to infer the presence of truncated proteins in cells from carriers of a truncated mutation without experimental verification, as each case is expected to be different.

Published

2007

5. Characterisation of a 161 kb deletion extending from the NBR1 to the BRCA1 genes in a French breast-ovarian cancer family

Author

Sophie, Gad, Ivan, Bièche, Michel, Barrois, Federica, Casilli, Sabine, Pages-Berhouet, Catherine, Dehainault, Marion, Gauthier-Villars, Aaron, Bensimon, Alain, Aurias, Rosette, Lidereau, Brigitte, Bressac-de Paillerets, Mario, Tosi, Sylvie, Mazoyer, and Dominique, Stoppa-Lyonnet

Subjects

Family Health, Ovarian Neoplasms, Base Sequence, BRCA1 Protein, DNA Mutational Analysis, Molecular Sequence Data, Intracellular Signaling Peptides and Proteins, Proteins, Breast Neoplasms, Humans, Female, France, Gene Deletion, Chromosomes, Human, Pair 17

Abstract

A large germline deletion removing exons 1 to 22 of the BRCA1 gene has been previously detected using quantitative PCR based methods (QMPSF and real time PCR gene dosage assay) in a woman affected with breast and ovarian cancer. Here, we report its characterisation by using colour bar code on combed DNA of the BRCA1 region. The 5' boundary is located in a Alu Y sequence in NBR1 intron 18 whereas the 3' boundary is located in a Alu Sc sequence in BRCA1 intron 22. This 161 kb deletion encompassing the NBR1, PsiBRCA1, NBR2 and BRCA1 genes is the largest BRCA1 deletion reported so far. No specific phenotype was associated with the hemizygosity of these four genes.

Published

2004

6. Characterisation of a 161 kb deletion extending from the NBR1 to the BRCA1 genes in a French breast-ovarian cancer family

Author

Sabine Pagès-Berhouet, Dominique Stoppa-Lyonnet, Sylvie Mazoyer, Brigitte Bressac-de Paillerets, Catherine Dehainault, Mario Tosi, Marion Gauthier-Villars, Rosette Lidereau, Alain Aurias, Federica Casilli, Sophie Gad, Ivan Bièche, Michel Barrois, and Aaron Bensimon

Subjects

Genetics, endocrine system diseases, Intron, Hemizygosity, Biology, Molecular biology, Gene dosage, Phenotype, Germline, Exon, Real-time polymerase chain reaction, skin and connective tissue diseases, Gene, Genetics (clinical)

Abstract

A large germline deletion removing exons 1 to 22 of the BRCA1 gene has been previously detected using quantitative PCR based methods (QMPSF and real time PCR gene dosage assay) in a woman affected with breast and ovarian cancer. Here, we report its characterisation by using colour bar code on combed DNA of the BRCA1 region. The 5' boundary is located in a Alu Y sequence in NBR1 intron 18 whereas the 3' boundary is located in a Alu Sc sequence in BRCA1 intron 22. This 161 kb deletion encompassing the NBR1, PsiBRCA1, NBR2 and BRCA1 genes is the largest BRCA1 deletion reported so far. No specific phenotype was associated with the hemizygosity of these four genes.

Published

2003

7. Characterisation of a 161 kb deletion extending from the NBR1 to the BRCA1 genes in a French breast-ovarian cancer family(Communicated by Richard G.H. Cotton)Online Citation: Human Mutation, Mutation in Brief #619 (2003) Online http://www.interscience.wiley.com/humanmutation/pdf/mutation/619.pdf)

Author

Sophie Gad, Ivan Bièche, Michel Barrois, Federica Casilli, Sabine Pages-Berhouet, Catherine Dehainault, Marion Gauthier-Villars, Aaron Bensimon, Alain Aurias, Rosette Lidereau, Brigitte Bressac-de Paillerets, Mario Tosi, and Sylvie Mazoyer

Subjects

EXONS (Genetics), SPLIT genes, POLYMERASE chain reaction, GENES, GENETICS, CANCER

Abstract

A large germline deletion removing exons 1 to 22 of the BRCA1 gene has been previously detected using quantitative PCR based methods (QMPSF and real time PCR gene dosage assay) in a woman affected with breast and ovarian cancer. Here, we report its characterisation by using colour bar code on combed DNA of the BRCA1 region. The 5' boundary is located in a Alu Y sequence in NBR1 intron 18 whereas the 3' boundary is located in a Alu Sc sequence in BRCA1 intron 22. This 161 kb deletion encompassing the NBR1, ΨBRCA1, NBR2 and BRCA1 genes is the largest BRCA1 deletion reported so far. No specific phenotype was associated with the hemizygosity of these four genes. © 2003 Wiley-Liss, Inc. [ABSTRACT FROM AUTHOR]

Published

2003