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1. VGLL3expression is associated with a tumor suppressor phenotype in epithelial ovarian cancer

Author

Karen Gambaro, Paulina M. Wojnarowicz, Michael C.J. Quinn, Jean Sébastien Ripeau, Mario Chevrette, Manon de Ladurantaye, Anne Marie Mes-Masson, Ann M. Killary, Suzanna L. Arcand, Elaine C. Davis, Véronique Barrès, Josée N. Lavoie, Patricia N. Tonin, and Diane Provencher

Subjects
Cancer Research, Stromal cell, Tumor suppressor gene, Population, Mice, Nude, Mice, SCID, Carcinoma, Ovarian Epithelial, Mice, 03 medical and health sciences, 0302 clinical medicine, Nude mouse, Cell Line, Tumor, Gene expression, Genetics, Animals, Humans, Genes, Tumor Suppressor, Neoplasms, Glandular and Epithelial, education, Cell Proliferation, 030304 developmental biology, Ovarian Neoplasms, 0303 health sciences, education.field_of_study, biology, Ovary, General Medicine, biology.organism_classification, Candidate Tumor Suppressor Gene, Molecular biology, Clone Cells, Gene Expression Regulation, Neoplastic, Phenotype, Oncology, Chromosome 3, 030220 oncology & carcinogenesis, Papers, Microcell-mediated chromosome transfer, Molecular Medicine, Female, Transcription Factors
Abstract

Previous studies have implicated vestigial like 3 (VGLL3), a chromosome 3p12.3 gene that encodes a putative transcription co‐factor, as a candidate tumor suppressor gene (TSG) in high‐grade serous ovarian carcinomas (HGSC), the most common type of epithelial ovarian cancer. A complementation analysis based on microcell‐mediated chromosome transfer (MMCT) using a centric fragment of chromosome 3 (der3p12‐q12.1) into the OV‐90 ovarian cancer cell line haploinsufficient for 3p and lacking VGLL3 expression was performed to assess the effect on tumorigenic potential and growth characteristics. Genetic characterization of the derived MMCT hybrids revealed that only the hybrid that contained an intact VGLL3 locus exhibited alterations of tumorigenic potential in a nude mouse xenograft model and various in vitro growth characteristics. Only stable OV‐90 transfectant clones expressing low levels of VGLL3 were derived. These clones exhibited an altered cytoplasmic morphology characterized by numerous single membrane bound multivesicular‐bodies (MVB) that were not attributed to autophagy. Overexpression of VGLL3 in OV‐90 was achieved using a lentivirus‐based tetracycline inducible gene expression system, which also resulted in MVB formation in the infected cell population. Though there was no significant differences in various in vitro and in vivo growth characteristics in a comparison of VGLL3‐expressing clones with empty vector transfectant controls, loss of VGLL3 expression was observed in tumors derived from mouse xenograft models. VGLL3 gene and protein expression was significantly reduced in HGSC samples (>98%, p

Published
2013

2. Radiation Hybrid Maps of Medaka Chromosomes LG 12, 17, and 22

Author

Nobuyoshi Shimizu, Hisato Kondoh, Yumi Osada, Mario Chevrette, Takao Sasado, Shuichi Asakawa, Robert Geisler, Takashi Sasaki, Aiko Shiohama, Makoto Furutani-Seiki, Atsushi Shimizu, Toshiyuki Yamanaka, Marc Ekker, Hiroshi Mitani, and Feng Su

Subjects
Genetic Markers, Genetics, Radiation Hybrid Mapping, Bacterial artificial chromosome, Genome, Short Communication, Oryzias, General Medicine, Biology, Genetic recombination, Medaka, Chromosomes, Chromosome 17 (human), Gene mapping, Animals, Radiation hybrid mapping, genetic mapping, Molecular Biology, Gene, Chromosome 12, BAC
Abstract

The Medaka is an excellent genetic system for studies of vertebrate development and disease and environmental and evolutionary biology studies. To facilitate the mapping of markers or the cloning of affected genes in Medaka mutants identified by forward-genetic screens, we have established a panel of whole-genome radiation hybrids (RHs) and RH maps for three Medaka chromosomes. RH mapping is useful, since markers to be mapped need not be polymorphic and one can establish the order of markers that are difficult to resolve by genetic mapping owing to low genetic recombination rates. RHs were generated by fusing the irradiated donor, OLF-136 Medaka cell line, with the host B78 mouse melanoma cells. Of 290 initial RH clones, we selected 93 on the basis of high retention of fragments of the Medaka genome to establish a panel that allows genotyping in the 96-well format. RH maps for linkage groups 12, 17, and 22 were generated using 159 markers. The average retention for the three chromosomes was 19% and the average break point frequency was approximately 33 kb/cR. We estimate the potential resolution of the RH panel to be approximately 186 kb, which is high enough for integrating RH data with bacterial artificial chromosome clones. Thus, this first RH panel will be a useful tool for mapping mutated genes in Medaka.

Published
2007

3. Chromosome 18 suppresses tumorigenic properties of human prostate cancer cells

Author

Jean-Sébastien Ripeau, Mario Chevrette, Valerii Zvieriev, and Audrey Gagnon

Subjects
Male, PCA3, Cancer Research, Chromosome Transfer, Transplantation, Heterologous, Mice, Nude, Hybrid Cells, Biology, Mice, Prostate cancer, Cancer stem cell, Chromosome 18, Cell Line, Tumor, Genetics, medicine, Animals, Chromosomes, Human, Humans, Neoplasm Invasiveness, Prostatic Neoplasms, Cancer, Chromoplexy, medicine.disease, Cancer cell, Cancer research, Chromosomes, Human, Pair 18, Neoplasm Transplantation
Abstract

Although prostate cancer is still the most diagnosed cancer in men, most genes implicated in its progression are yet to be identified. Chromosome abnormalities have been detected in human prostate tumors, many of them associated with prostate cancer progression. Indeed, alterations (including deletions or amplifications) of more than 15 human chromosomes have been reported in prostate cancer. We hypothesized that transferring normal human chromosomes into human prostate cancer cells would interfere with their tumorigenic and/or metastatic properties. We used microcell-mediated chromosome transfer to introduce human chromosomes 10, 12, 17, and 18 into highly tumorigenic (PC-3M-Pro4) and highly metastatic (PC-3M-LN4) PC-3-derived cell lines. We tested the in vitro and in vivo properties of these hybrids. Introducing chromosome 18 into the PC-3M-LN4 prostate cancer cell line greatly reduced its tumorigenic phenotype. We observed retarded growth in soft agar, decreased invasiveness through Matrigel, and delayed tumor growth into nude mice, both subcutaneously and orthotopically. This phenotype is associated with a marker in the 18q21 region. Combined with the loss of human chromosome 18 regions often seen in patients with advanced prostate cancer, our results show that chromosome 18 encodes one or more tumor-suppressor genes whose inactivation contributes to prostate cancer progression. © 2005 Wiley-Liss, Inc.

Published
2005

4. Radiation hybrid mapping of the zebrafish genome

Author

Frank Ning Li, Leonard I. Zon, Patricia Tellis, Lucille Joly, Thomas J. Hudson, Michael Tsang, Barry H. Paw, John H. Postlethwait, Igor B. Dawid, John Douglas Mcpherson, Marc Ekker, Jonathan A. Epstein, William B. Barbazuk, Mario Chevrette, Neil A. Hukriede, Jennifer Miles, and Stephen L. Johnson

Subjects
Genetic Markers, Candidate gene, Genotype, Genetic Linkage, DNA Mutational Analysis, Green Fluorescent Proteins, Biology, Polymerase Chain Reaction, Mice, Gene mapping, Animals, Radiation hybrid mapping, Cloning, Molecular, Simple sequence length polymorphism, Zebrafish, In Situ Hybridization, Expressed Sequence Tags, Genetics, Expressed sequence tag, Genome, Polymorphism, Genetic, Multidisciplinary, Breakpoint, Chromosome Mapping, Biological Sciences, Physical Chromosome Mapping, biology.organism_classification, Immunohistochemistry, Meiosis, Luminescent Proteins, Mutagenesis, Insertional, Phenotype, Genetic marker, Commentary, Microsatellite Repeats
Abstract

The zebrafish is an excellent genetic system for the study of vertebrate development and disease. In an effort to provide a rapid and robust tool for zebrafish gene mapping, a panel of radiation hybrids (RH) was produced by fusion of irradiated zebrafish AB9 cells with mouse B78 cells. The overall retention of zebrafish sequences in the 93 RH cell lines that constitute the LN54 panel is 22%. Characterization of the LN54 panel with 849 simple sequence length polymorphism markers, 84 cloned genes and 122 expressed sequence tags allowed the production of an RH map whose total size was 11,501 centiRays. From this value, we estimated the average breakpoint frequency of the LN54 RH panel to correspond to 1 centiRay = 148 kilobase. Placement of a group of 235 unbiased markers on the RH map suggests that the map generated for the LN54 panel, at present, covers 88% of the zebrafish genome. Comparison of marker positions in RH and meiotic maps indicated a 96% concordance. Mapping expressed sequence tags and cloned genes by using the LN54 panel should prove to be a valuable method for the identification of candidate genes for specific mutations in zebrafish.

Published
1999

5. Stable Transfer of Zebrafish Chromosome Segments into Mouse Cells

Author

Marc Ekker, Lucille Joly, C. Cristofre Martin, Mario Chevrette, Marsha D. Speevak, and Genny Giroux

Subjects
Genetic Markers, animal structures, Chromosomal translocation, Hybrid Cells, Biology, Mice, Gene mapping, Genetics, medicine, Animals, Zebrafish, In Situ Hybridization, Fluorescence, Repetitive Sequences, Nucleic Acid, Cloning, medicine.diagnostic_test, fungi, Genetic transfer, Chromosome Mapping, Chromosome, biology.organism_classification, Cell biology, genomic DNA, embryonic structures, Fluorescence in situ hybridization
Abstract

Whole-cell fusion between zebrafish fibroblast-like ZF4 cells and mouse B78 melanoma cells resulted in hybrids containing one or a few zebrafish chromosome segments in a murine chromosomal background. Fluorescence in situ hybridization to hybrid cell metaphases with a zebrafish genomic DNA probe revealed that many hybrids contained zebrafish chromosome segments that were either inserted or translocated to a mouse chromosome, whereas other hybrids contained zebrafish chromosomes with no evidence of insertion or translocation. We have assigned hybrids to 17 linkage groups of the genetic map of the zebrafish genome. Our results demonstrate the feasibility of producing somatic cell hybrids between distantly related species. Zebrafish/mouse cell hybrids will provide a useful tool for the physical mapping of the zebrafish genome and for the cloning of genes affected in zebrafish mutants.

Published
1996

6. Mermaid,a Family of Short Interspersed Repetitive Elements, Is Useful for Zebrafish Genome Mapping

Author

Yutaka Kikuchi, Mario Chevrette, Nobuyoshi Shimoda, Yoshiki Hotta, Hitoshi Okamoto, and Marc Ekker

Subjects
Genetic Markers, Genome evolution, animal structures, Molecular Sequence Data, Biophysics, Computational biology, Hybrid Cells, Biology, Biochemistry, Genome, Evolution, Molecular, Mice, chemistry.chemical_compound, Gene density, Animals, Humans, Molecular Biology, Zebrafish, DNA Primers, Repetitive Sequences, Nucleic Acid, Genetics, Polymorphism, Genetic, Base Sequence, Oligonucleotide, fungi, Chromosome Mapping, DNA, Cell Biology, Genome project, biology.organism_classification, chemistry, embryonic structures, Human genome
Abstract

A family of short interspersed repetitive elements (SINEs), designated mermaid, is present in the genomes of fish, amphibian and primates, but absent in the mouse genome. We have demonstrated that the sequences of the mermaid family are highly polymorphic in the zebrafish genome as in the human genome. We have also shown that the mermaid sequence can be used to recover zebrafish specific DNA from zebrafish–mouse cell hybrids by using mermaid -specific oligonucleotides as PCR primers. Thus, the mermaid family serves as a valuable genetic tool for the zebrafish genome mapping.

Published
1996

7. Identification of chromosomes implicated in suppression of apoptosis in somatic cell hybrids

Author

Marsha D. Speevak and Mario Chevrette

Subjects
Male, Phosphonoacetic Acid, Melanoma, Experimental, Apoptosis, Tumorigenic cell, Hybrid Cells, Biology, Polymerase Chain Reaction, Biochemistry, Mice, Tumor Cells, Cultured, Animals, Chromosomes, Human, Humans, Molecular Biology, Aspartic Acid, Somatic Cell Hybrids, Cell Cycle, In vitro exposure, DNA, Cell Biology, Fibroblasts, Flow Cytometry, Genes, p53, Clone Cells, Cell biology, Karyotyping, Identification (biology)
Abstract

In vitro exposure of tumorigenic cell lines to the chemotherapeutic agent PALA (N-(phosphonoacetyl)-L-aspartate) usually results in cell death (shown here to be apoptosis), followed by clonal growth of rare survivors. On the other hand, normal diploid cells respond to PALA by arresting in G1 and G2 of the cell cycle. It was previously suggested that growth control mechanisms might exist to prevent cells from entering S phase under toxic conditions and that genes involved in such mechanisms were mutated or deleted in tumor cells. Interestingly, the tumor suppressor gene p53, a putative G1 control gene, was shown to mediate PALA-induced growth arrest. However, growth arrest occurs in cells that lack wild-type p53, suggesting that other genes are involved as well. To identify these genes, we have generated whole cell hybrids between mouse melanoma and normal human fibroblast cells. At early passage, a whole cell hybrid (BHF12) responds to PALA with growth arrest, while at later passage, the same hybrid undergoes apoptosis. To determine which human chromosomes are required for the PALA-induced growth arrest phenotype, we isolated subclones of the hybrid and tested them for their PALA response. FISH (fluorescence in situ hybridization) and PCR (polymerase chain reaction) amplification have been used to identify the human chromosome content of BHF12 and its subclones. Several human chromosomes, in addition to chromosome 17 (the location of p53), are consistently associated with the growth arrest phenotype. These findings provide evidence that one or more genes in addition to p53 may be involved in the suppression of a drug-induced apoptosis pathway and may lie on one or more of these chromosomes.Key words: apoptosis, growth arrest, N-(phosphonoacetyl)-L-aspartate, somatic cell hybrids.

Published
1994

8. Generation of region– and species–specific expressed gene probes from somatic cell hybrids

Author

Michael H. Shapero, Mario Chevrette, Keith W. Jones, and R. E. K. Fournier

Subjects
Male, Genetic Linkage, Molecular Sequence Data, Hybrid Cells, Biology, Cell Line, Mice, Liver Neoplasms, Experimental, Tubulin, Sequence Homology, Nucleic Acid, Complementary DNA, Tumor Cells, Cultured, Genetics, Animals, Humans, Gene, Cells, Cultured, Gene Library, Cloning, Base Sequence, cDNA library, Chromosome Mapping, Chromosome, Fibroblasts, Molecular biology, Chromosome Banding, Rats, Chromosome 17 (human), Oligodeoxyribonucleotides, Suppression subtractive hybridization, Human genome, DNA Probes, Chromosomes, Human, Pair 17
Abstract

Human genes expressed in interspecific somatic cell hybrids can be cloned specifically by subtractive cDNA hybridization. This approach is based on the observation that cDNA fragments from noncoding segments of mature human transcripts do not form stable heteroduplexes with their rodent homologues under high-stringency hybridization conditions. Thus, small, oligo-dT primed cDNAs from a rat/human hybrid retaining a fragment of human chromosome 17 were enriched for human sequences by hybridization with RNA from a sister clone containing a smaller human chromosome fragment. The enriched probe was used to screen a human cDNA library, and nine expressed genes from within the non-overlap region were obtained. This method should be useful for cloning active human genes from defined chromosome segments.

Published
1992

9. Transfer of chromosome 3 fragments suppresses tumorigenicity of an ovarian cancer cell line monoallelic for chromosome 3p

Author

Mario Chevrette, Veronique Ouellet, P. Tellis, D. Provencher, Emily N. Manderson, A. Filali-Mouhim, Magdalena Zietarska, Michael C.J. Quinn, Neal A.L. Cody, Anne Marie Mes-Masson, and Patricia N. Tonin

Subjects
Cancer Research, Tumor suppressor gene, Chromosome Transfer, Mice, Nude, Biology, Adenocarcinoma, medicine.disease_cause, Loss of heterozygosity, Transcriptome, Mice, Cell Line, Tumor, Genetics, medicine, Animals, Humans, Genes, Tumor Suppressor, Molecular Biology, Chromosome Aberrations, Ovarian Neoplasms, Microarray analysis techniques, Gene Expression Profiling, Gene Transfer Techniques, medicine.disease, Xenograft Model Antitumor Assays, Chromosome 3, Cancer research, Female, Chromosomes, Human, Pair 3, Ovarian cancer, Carcinogenesis
Abstract

Multiple chromosome 3p tumor suppressor genes (TSG) have been proposed in the pathogenesis of ovarian cancer based on complex patterns of 3p loss. To attain functional evidence in support of TSGs and identify candidate regions, we applied a chromosome transfer method involving cell fusions of the tumorigenic OV90 human ovarian cancer cell line, monoallelic for 3p and an irradiated mouse cell line containing a human chromosome 3 in order to derive OV90 hybrids containing normal 3p fragments. The resulting hybrids showed complete or incomplete suppression of tumorigenicity in nude mouse xenograft assays, and varied in their ability to form colonies in soft agarose and three-dimensional spheroids in a manner consistent with alteration of their in vivo tumorigenic phenotypes. Expression microarray analysis identified a set of common differentially expressed genes, such as SPARC, DAB2 and VEGF, some of which have been shown implicated in ovarian cancer. Genotyping assays revealed that they harbored normal 3p fragments, some of which overlapped candidate TSG regions (3p25-p26, 3p24 and 3p14-pcen) identified previously in loss of heterozygosity analyses of ovarian cancers. However, only the 3p12-pcen region was acquired in common by all hybrids where expression microarray analysis identified differentially expressed genes. The correlation of 3p12-pcen transfer and tumor suppression with a concerted re-programming of the cellular transcriptome suggest that the putative TSG may have affected key underlying events in ovarian cancer.

Published
2006

10. Over-expression of CD9 does not affect in vivo tumorigenic or metastatic properties of human prostate cancer cells

Author

Jia-Chi Wang, Mario Chevrette, and Valerii Zvieriev

Subjects
PCA3, Male, Time Factors, Molecular Sequence Data, Biophysics, Mice, Nude, Biology, Biochemistry, Tetraspanin 29, Injections, Prostate cancer, Mice, Tetraspanin, Cancer stem cell, Prostate, In vivo, Antigens, CD, medicine, Tumor Cells, Cultured, Animals, Humans, Neoplasm Metastasis, Molecular Biology, Membrane Glycoproteins, Base Sequence, Prostatic Neoplasms, Cell Biology, medicine.disease, medicine.anatomical_structure, Gene Expression Regulation, Cell culture, Lymphatic Metastasis, embryonic structures, Cancer cell, Cancer research, Neoplasm Transplantation
Abstract

Expression of tetraspanin CD9 protein is downregulated in many tumors. CD9 over-expression also reduces the tumorigenicity of some human cancer cells. Here, we determined if exogenous expression of CD9 affects the properties of human prostate cancer cells. Highly metastatic prostate cancer cells PC-3M-LN4 over-expressing exogenous CD9 were orthotopically injected into the prostate of nude mice. CD9 expression was determined in tumors using PCR and Western immunoblotting techniques. Over-expression of CD9 increased invasiveness of prostate cancer cells in vitro. Animals injected with either parental PC-3M-LN4 or CD9-transfected cells developed tumor and harbored lymph node metastasis. There was no statistical difference in tumor growth between the two cell lines. CD9 did not suppress tumorigenic or metastatic properties of PC-3M-LN4 cells. Our data contrast with published results in other tumor types and likely indicate that other proteins (CD9 partners) are needed for CD9 full anti-tumorigenic action.

Published
2005

11. Potentiation of a dendritic cell vaccine for murine renal cell carcinoma by CpG oligonucleotides

Author

Fanny Chagnon, Simon Tanguay, Ozdem Levent Ozdal, Meng Guan, Zeynep Z. Ozen, Jean-Sébastien Ripeau, Mario Chevrette, Mostafa M. Elhilali, and Lu Ann Thompson-Snipes

Subjects
Cancer Research, Analysis of Variance, Mice, Inbred BALB C, T-Lymphocytes, Bone Marrow Cells, Dendritic Cells, Immunotherapy, Adoptive, Kidney Neoplasms, Mice, Treatment Outcome, Oncology, Adjuvants, Immunologic, Oligodeoxyribonucleotides, Cell Line, Tumor, Animals, CpG Islands, Carcinoma, Renal Cell, Neoplasm Transplantation
Abstract

Purpose: An ideal vaccine therapy for tumors should activate both effector and memory immune responses against tumor-specific antigens. Here we investigated the effect of CpG oligodeoxynucleotides (CpG-ODN) for their ability to potentiate the activity of tumor antigen–pulsed bone marrow–derived dendritic cells (DC) in a vaccine model for the treatment of murine renal cell carcinoma (RENCA).Experimental Design: First we evaluated the effects of a murine renal cell carcinoma (RENCA) on immune cell activity in a mouse model using in vitro assays for T-cell proliferation and natural killer cell activation. To overcome the immune suppression of the tumor, we s.c. injected groups of 10 mice with dendritic cells and tumor cells. We compared the effect of different conditioning regimens of the DCs with RENCA antigen and/or CpG-ODNs before injection by measuring tumor size twice a week.Results: Tumor growth was shown to negatively affect spleen cell and T-cell proliferation, IFN-γ production, natural killer cell activity, and NF-κB activation in T cells. In this model, we have shown that RENCA-pulsed CpG-ODN-treated DCs were able not only to significantly reduce tumor growth but also to prevent tumor implantation in 60% of mice. Tumor-free mice were resistant to tumor challenge and the immunity conferred by the vaccine was transferable and tumor specific.Conclusions: This data show that RENCA down-modulates the immune response, and DC vaccine therapy, in conjunction with CpG-ODN, can restore tumor-specific immunity.

Published
2005

12. Screen for genes differentially expressed during regeneration of the zebrafish caudal fin

Author

Marie-Andrée Akimenko, Puru Nanjappa, Marc Ekker, Lucille Joly, Mario Chevrette, Amanda C. Smith, Patricia A. Tellis, and Bhaja K. Padhi

Subjects
DNA, Complementary, Embryo, Nonmammalian, Molecular Sequence Data, In situ hybridization, Polymerase Chain Reaction, Amputation, Surgical, Fin regeneration, Gene expression, Animals, Regeneration, Genetic Testing, Zebrafish, In Situ Hybridization, Expressed Sequence Tags, Differential display, Wound Healing, biology, Base Sequence, Subtraction hybridization, Reverse Transcriptase Polymerase Chain Reaction, Regeneration (biology), fungi, Gene Expression Regulation, Developmental, Nucleic Acid Hybridization, Extremities, biology.organism_classification, Physical Chromosome Mapping, Molecular biology, Up-Regulation, Keratins, Blastema, Developmental Biology
Abstract

The zebrafish caudal fin constitutes an important model for studying the molecular basis of tissue regeneration. The cascade of genes induced after amputation or injury, leading to restoration of the lost fin structures, include those responsible for wound healing, blastema formation, tissue outgrowth, and patterning. We carried out a systematic study to identify genes that are up-regulated during “initiation” (1 day) and “outgrowth and differentiation” (4 days) of fin regeneration by using two complementary methods, suppression subtraction hybridization (SSH) and differential display reverse transcriptase polymerase chain reaction (DDRT-PCR). We obtained 298 distinct genes/sequences from SSH libraries and 24 distinct genes/sequences by DDRT-PCR. We determined the expression of 54 of these genes using in situ hybridization. In parallel, gene expression analyses were done in zebrafish embryos and early larvae. The information gathered from the present study provides resources for further investigations into the molecular mechanisms of fin development and regeneration. Developmental Dynamics 231:527–541, 2004. © 2004 Wiley-Liss, Inc.

Published
2004

13. Analysis of the conservation of synteny between Fugu and human chromosome 12

Author

Michael D. Wilson, Alexandre Montpetit, Daniel Sinnett, Ben F. Koop, and Mario Chevrette

Subjects
lcsh:QH426-470, lcsh:Biotechnology, Molecular Sequence Data, Locus (genetics), Takifugu, Synteny, Genome, Conserved sequence, 03 medical and health sciences, 0302 clinical medicine, Sequence Homology, Nucleic Acid, lcsh:TP248.13-248.65, Gene Order, Genetics, Animals, Humans, Gene, Conserved Sequence, 030304 developmental biology, 0303 health sciences, Chromosomes, Human, Pair 12, Base Sequence, Proto-Oncogene Proteins c-ets, biology, Fugu, fungi, Chromosome Mapping, DNA, Sequence Analysis, DNA, biology.organism_classification, DNA-Binding Proteins, Repressor Proteins, lcsh:Genetics, 030220 oncology & carcinogenesis, Human genome, Sequence Alignment, Research Article, Biotechnology
Abstract

Background The pufferfish Fugu rubripes (Fugu) with its compact genome is increasingly recognized as an important vertebrate model for comparative genomic studies. In particular, large regions of conserved synteny between human and Fugu genomes indicate its utility to identify disease-causing genes. The human chromosome 12p12 is frequently deleted in various hematological malignancies and solid tumors, but the actual tumor suppressor gene remains unidentified. Results We investigated approximately 200 kb of the genomic region surrounding the ETV6 locus in Fugu (fETV6) in order to find conserved functional features, such as genes or regulatory regions, that could give insight into the nature of the genes targeted by deletions in human cancer cells. Seven genes were identified near the fETV6 locus. We found that the synteny with human chromosome 12 was conserved, but extensive genomic rearrangements occurred between the Fugu and human ETV6 loci. Conclusion This comparative analysis led to the identification of previously uncharacterized genes in the human genome and some potentially important regulatory sequences as well. This is a good indication that the analysis of the compact Fugu genome will be valuable to identify functional features that have been conserved throughout the evolution of vertebrates.

Published
2003

14. Whole-cell and microcell fusion for the identification of natural regulators of telomerase

Author

Henriette, Gourdeau, Marsha D, Speevak, Lucie, Jetté, and Mario, Chevrette

Subjects
Melanoma, Experimental, Fibroblasts, Hybrid Cells, Avidin, Polymerase Chain Reaction, Gene Expression Regulation, Enzymologic, Chromosome Painting, Neoplasm Proteins, Cell Fusion, Repressor Proteins, Mice, Microscopy, Fluorescence, Species Specificity, Alu Elements, Neoplasms, Animals, Chromosomes, Human, Humans, Biotinylation, Telomerase, Cells, Cultured, Cellular Senescence
Published
2002

15. The LN54 radiation hybrid map of zebrafish expressed sequences

Author

Neil A. Hukriede, Jonathan I. Epstein, Lucille Joly, Laura Fenton-Noriega, Mario Chevrette, Brad Barbazuk, Daniel A.C. Fisher, Marc Ekker, Kristine Cox, Yi Zhou, Igor B. Dawid, Xiaoming Sheng, Patricia Tellis, John Douglas Mcpherson, Leonard I. Zon, Stephen L. Johnson, Candace Hersey, Anhua Song, Rick Waterman, and Jennifer Miles

Subjects
Genetics, Expressed Sequence Tags, Genetic Markers, Expressed sequence tag, Radiation Hybrid Mapping, Genetic Linkage, Gene Expression Profiling, Biology, biology.organism_classification, Resources, Gene expression profiling, Genetic marker, Genetic linkage, Complementary DNA, Animals, Radiation hybrid mapping, Zebrafish, Gene, Genetics (clinical)
Abstract

To increase the density of a gene map of the zebrafish, Danio rerio, we have placed 3119 expressed sequence tags (ESTs) and cDNA sequences on the LN54 radiation hybrid (RH) panel. The ESTs and genes mapped here join 748 SSLp markers and 459 previously mapped genes and ESTs, bringing the total number of markers on the LN54 RH panel to 4226. Addition of these new markers brings the total LN54 map size to 14,372 cR, with 118 kb/cR. The distribution of ESTs according to linkage groups shows relatively little variation (minimum, 73; maximum, 201). This observation, combined with a relatively uniform size for zebrafish chromosomes, as previously indicated by karyotyping, indicates that there are no especially gene-rich or gene-poor chromosomes in this species. We developed an algorithm to provide a semiautomatic method for the selection of additional framework markers for the LN54 map. This algorithm increased the total number of framework markers to 1150 and permitted the mapping of a high percentage of sequences that could not be placed on a previous version of the LN54 map. The increased concentration of expressed sequences on the LN54 map of the zebrafish genome will facilitate the molecular characterization of mutations in this species.

Published
2001

16. Characterization of a zebrafish/mouse somatic cell hybrid panel

Author

Jennifer Miles, Mario Chevrette, Mark C. Fishman, Lucille Joly, Marc Ekker, Patricia Tellis, and Ela W. Knapik

Subjects
Genetics, Genetic Markers, biology, Somatic cell, Genetic Linkage, Chromosome, Hybrid Cells, biology.organism_classification, Genome, Polymerase Chain Reaction, Cell Line, Somatic fusion, Mice, Gene mapping, Genetic marker, Animals, Zebrafish, Gene, In Situ Hybridization, Fluorescence, Microsatellite Repeats
Abstract

We have characterized a collection of zebrafish/mouse somatic cell hybrids with 211 genes and markers chosen from the 25 zebrafish linkage groups. Most of the zebrafish genome is represented in this collection with 88% of genes/markers present in at least one hybrid cell line. Although most hybrids contain chromosomal fragments, there are a few instances where a complete or nearly complete zebrafish chromosome has been maintained in a mouse background, based on multiple markers covering the entire chromosome. In addition to their use in mapping studies, this collection of somatic cell hybrids should constitute an important tool as a source of specific chromosome fragments and for assessing the function of genome regions.

Published
2000

17. Links between Fer tyrosine kinase expression levels and prostate cell proliferation

Author

Linh T. Nguyen, Mario Chevrette, Amina Zoubeidi, Sylvain Tessier, Armen Aprikian, Simon Tanguay, Simone Chevalier, and Pierre Allard

Subjects
Male, DNA, Complementary, Molecular Sequence Data, Prostatic Hyperplasia, Transfection, Biochemistry, Basal Cell Hyperplasia, Antibodies, Gene Expression Regulation, Enzymologic, Prostate cancer, Endocrinology, Dogs, DU145, Species Specificity, Prostate, Proto-Oncogene Proteins, LNCaP, medicine, Tumor Cells, Cultured, Animals, Humans, Amino Acid Sequence, Cloning, Molecular, Molecular Biology, DNA Primers, biology, Base Sequence, Sequence Homology, Amino Acid, Prostatic Neoplasms, Protein-Tyrosine Kinases, medicine.disease, medicine.anatomical_structure, Cancer research, biology.protein, Tyrosine kinase, Cortactin, Cell Division
Abstract

In our cloning strategy to identify tyrosine kinases implicated in the regulation of prostate growth, the dog fer cDNA was obtained and shown to be highly homologous to known fer cDNAs. Using a polyclonal Fer antibody directed against a C-terminal peptide, we studied its associations with cortactin, β-catenin and p120Cas in human prostate carcinoma PC-3 cells. In contrast to previous reports, no interactions were observed. To assess its functional role, fer cDNA constructs were transfected in PC-3 cells. Antisense clones exhibiting a marked diminution of Fer expression had a reduced growth rate (doubling time of 29 vs. 42 h) and were unable to form colonies in soft agar. In agreement with these results, Fer protein expression was linked to human prostatic proliferative diseases, with enhanced levels in extracts from cancer tissues as compared to those from normal and hyperplastic ones, and was also expressed in the human prostate carcinoma cell lines DU145 and LNCaP. In the dog model, Fer expression was up-regulated in dividing versus resting prostate epithelial cells in vitro, and also in vivo when basal cell hyperplasia and metaplasia was induced by estrogen after castration. Minimal effects were observed when renewing the luminal epithelium with androgens. Taken together, these results show that Fer expression is associated with prostate cell proliferation and enhanced in prostate cancer.

Published
2000

18. A microsatellite genetic linkage map for zebrafish (Danio rerio)

Author

Jonathan Delgado, Nobuyoshi Shimoda, Ela W. Knapik, Mark C. Fishman, Howard J. Jacob, Mario Chevrette, Marc Ekker, Stephan C.F. Neuhauss, Alec Goodman, and Wolfgang Driever

Subjects
Genetics, Genetic Markers, Genome, Positional cloning, biology, Genetic Linkage, fungi, Chromosome Mapping, Sequence Analysis, DNA, biology.organism_classification, Centimorgan, Gene mapping, Genes, Genetic linkage, Genetic marker, Microsatellite, Animals, Zebrafish, Microsatellite Repeats
Abstract

We have constructed a zebrafish genetic linkage map consisting of 705 simple sequence-length polymorphism markers (SSLPs). The map covers 2350 centimorgans (cM) of the zebrafish genome with an average resolution of 3.3 cM. It is a complete map in genetic mapping terms (there is one linkage group for each of the 25 chromosomes), and it has been confirmed by somatic-cell hybrids and centromere-mapping using half-tetrad analysis. The markers are highly polymorphic in the zebrafish strains used for genetic crosses and provide a means to compare genetic segregation of developmental mutations between laboratories. These markers will provide an initial infrastructure for the positional cloning of the nearly 600 zebrafish genes identified as crucial to vertebrate development,and will become the anchor for the physical map of the zebrafish genome.

Published
1998

19. Contribution of zebrafish-mouse cell hybrids to the mapping of the zebrafish genome

Author

Patricia Tellis, Lucille Joly, Mario Chevrette, and Marc Ekker

Subjects
animal structures, Genetic Linkage, Danio, Biology, Hybrid Cells, Biochemistry, Cell Line, Cell Fusion, Mice, biology.animal, Animals, Molecular Biology, Zebrafish, Zebrafish genome, Genetics, Genome, fungi, Vertebrate, Chromosome Mapping, Cell Biology, Fibroblasts, biology.organism_classification, Evolutionary biology, embryonic structures, Cell hybrids, %22">Fish
Abstract

The zebrafish, Danio rerio, is becoming an increasingly popular model for the study of vertebrate development. Indeed, the biology of the fish offers great advantages for such studies. The life cycle of the zebrafish is relatively short (2-3 months) and the embryos develop outside the mother, facilitating the visualization of any mutated phenotype. At present, more than 1000 embryonic mutations have been reported. However, until recently, there was no physical or genetic map for this organism. In an effort to generate such a map, we have produced and characterized a panel of zebrafish-mouse cell hybrids. We have used whole-cell fusion to transfer zebrafish chromosomes from two different zebrafish cell lines into mouse recipient cells, thus generating more than 100 hybrids. Using fluorescence in situ hybridization and polymerase chain reaction analysis, we have determined the zebrafish chromosome composition of these hybrids. Here we report that elements from the 25 linkage groups of the zebrafish genome are present in our hybrids. These hybrids could identify the chromosomal location of genes affected in zebrafish mutants.

Published
1997

20. Mermaid: a family of short interspersed repetitive elements widespread in vertebrates

Author

Yutaka Kikuchi, Mario Chevrette, Nobuyoshi Shimoda, Marc Ekker, Hitoshi Okamoto, and Yoshiki Hotta

Subjects
Amphibian, Transposable element, Primates, Interspersed repeat, Molecular Sequence Data, Biophysics, Biochemistry, Genome, Polymerase Chain Reaction, Amphibians, Evolution, Molecular, Species Specificity, biology.animal, Sequence Homology, Nucleic Acid, Animals, Humans, Molecular Biology, Conserved Sequence, Phylogeny, DNA Primers, Repetitive Sequences, Nucleic Acid, Genetics, biology, Base Sequence, Fishes, Cell Biology, Evolutionary biology, Horizontal gene transfer, Vertebrates, DNA Transposable Elements, %22">Fish
Abstract

We have discovered a family of short interspersed repetitive elements (SINEs) that are present in the genomes of fish, amphibian and primates. The family of the SINEs, designated mermaid, is distinctive in each species except for a conserved region of approximately 80 bp. Some members of the mermaid family were found in transposon-like repetitive elements, including Tc1-like elements which are also distributed in the genomes of fish and amphibian. This raises the possibility of horizontal transfer of the mermaid family between vertebrates via transposons.

Published
1996

21. DNase I hypersensitivity and methylation of the 5'-flanking region of the α1-fetoprotein gene during developmental and glucocorticoid-induced repression of its activity in rat liver

Author

Mario Chevrette, Hélène LaRue, Bernard Turcotte, Michel Guertin, and Luc Bélanger

Subjects
Male, Aging, Transcription, Genetic, 5' flanking region, Biology, Methylation, Dexamethasone, chemistry.chemical_compound, Liver Neoplasms, Experimental, Transcription (biology), Genetics, Animals, Deoxyribonuclease I, Cloning, Molecular, Gene, Nucleotide Mapping, Brain, Rats, Inbred Strains, DNA Restriction Enzymes, Molecular biology, digestive system diseases, Liver Regeneration, Rats, Chromatin, Genes, Liver, chemistry, DNA methylation, alpha-Fetoproteins, DNA
Abstract

Three major regions of DNase I hypersensitivity (DH) were found in alpha 1-fetoprotein (AFP) chromatin of rat liver. DH site I is located at the transcription initiation site and associated with ongoing AFP transcription. DH site II is located 2.5 kb upstream from the cap site: it is developmental stage-dependent but dissociable from ongoing AFP transcription. DH site III, 3.7 kb upstream from the cap site, behaves as hepatocyte-constitutive. DH sites are present in similar regions of liver albumin chromatin. Dexamethasone-induced AFP gene repression is accompanied by the selective loss of AFP DH site I, a likely result of glucocorticoid receptors binding to a DNA recognition sequence located 5'-adjacent to DH site I. Sl nuclease-hypersensitive sites were found on naked superhelical AFP and albumin DNA, but do not appear to contribute DH sites in liver chromatin. The extent of hypomethylation of HpaII sites at the 5'-end of the AFP gene correlates positively with the level of potential and actual expression of the gene. We conclude that developmental and hormonal regulation of the AFP gene is confined within congruent to 4 kb of 5'-flanking DNA, and we discuss possible hierarchical interactions among DH sites, in relation to DNA methylation and replication.

Published
1986

22. Enhancer and Promoter Elements Directing Activation and Glucocorticoid Repression of the α1-Fetoprotein Gene in Hepatocytes

Author

Michel Guertin, Luc Bélanger, Marie-Claude Gingras, Mario Chevrette, O Wrange, Daniel Bernier, and Hélène LaRue

Subjects
Chloramphenicol O-Acetyltransferase, Transcriptional Activation, Molecular Sequence Data, Biology, Transfection, Dexamethasone, Chloramphenicol acetyltransferase, Glucocorticoid receptor, Cytosol, Liver Neoplasms, Experimental, Recognition sequence, Acetyltransferases, Genes, Regulator, Animals, Cloning, Molecular, Enhancer, Promoter Regions, Genetic, Molecular Biology, Tyrosine Transaminase, Regulation of gene expression, Nuclear factor I, Base Sequence, Point mutation, Cell Biology, Molecular biology, digestive system diseases, Rats, Enhancer Elements, Genetic, Gene Expression Regulation, Genes, Liver, Regulatory sequence, Enzyme Induction, alpha-Fetoproteins, Research Article, Plasmids
Abstract

Mutations were introduced in 7 kilobases of 5'-flanking rat ..cap alpha../sub 1/-fetoprotein (AFP) genomic DNA, linked to the chloramphenicol acetyltransferase gene. AFP promoter activity and its repression by a glucocorticoid hormone were assessed by stable and transient expression assays. Stable transfection assays were more sensitive and accurate than transient expression assays in a Morris 7777 rat hepatoma recipient (Hepa7.6), selected for its strong AFP repression by dexamethasone. The segment of DNA encompassing a hepatocyte-constitutive chromatin DNase I-hypersensitive site at -3.7 kilobases and a liver developmental stage-specific site at -2.5 kilobases contains interacting enhancer elements sufficient for high AFP promoter activity in Hepa7.6 or HepG2 cells. Deletions and point mutations define an upstream promoter domain of AFP gene activation, operating with at least three distinct promoter-activating elements, PEI at -65 base pairs, PEII at -120 base pairs, and DE at -160 base pairs. PEI and PEII share homologies with albumin promoter sequences, PEII is a near-consensus nuclear factor I recognition sequence, and DE overlaps a glucocorticoid receptor recognition sequence. An element conferring glucocorticoid repression of AFP gene activity is located in the upstream AFP promoter domain. Receptor-binding assays indicate that this element is the glucocorticoid receptor recognition sequence which overlaps withmore » promoter-activating element DE.« less

Published
1988

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