Your search keyword '"Van Roy N"' showing total 13 results

1. Anchoring linkage groups of the Rosa genetic map to physical chromosomes with tyramide-FISH and EST-SNP markers.

Author

Kirov I, Van Laere K, De Riek J, De Keyser E, Van Roy N, and Khrustaleva L

Subjects

Expressed Sequence Tags, Genetic Markers, Polymorphism, Single Nucleotide, Chromosome Mapping, Chromosomes, Plant, Genetic Linkage, In Situ Hybridization, Fluorescence methods, Rosa genetics

Abstract

In order to anchor Rosa linkage groups to physical chromosomes, a combination of the Tyramide-FISH technology and the modern molecular marker system based on High Resolution Melting (HRM) is an efficient approach. Although, Tyramide-FISH is a very promising technique for the visualization of short DNA probes, it is very challenging for plant species with small chromosomes such as Rosa. In this study, we successfully applied the Tyramide-FISH technique for Rosa and compared different detection systems. An indirect detection system exploiting biotinylated tyramides was shown to be the most suitable technique for reliable signal detection. Three gene fragments with a size of 1100 pb-1700 bp (Phenylalanine Ammonia Lyase, Pyrroline-5-Carboxylate Synthase and Orcinol O-Methyl Transferase) have been physically mapped on chromosomes 7, 4 and 1, respectively, of Rosa wichurana. The signal frequency was between 25% and 40%. HRM markers of these 3 gene fragments were used to include the gene fragments on the existing genetic linkage map of Rosa wichurana. As a result, three linkage groups could be anchored to their physical chromosomes. The information was used to check for synteny between the Rosa chromosomes and Fragaria.

Published

2014

2. Chromosome 3p microsatellite allelotyping in neuroblastoma: a report on the technical hurdles.

Author

Hoebeeck J, De Wilde B, Michels E, Combaret V, Yigit N, De Smet E, Van Roy N, Stanbridge E, Ru N, Laureys G, De Paepe A, Speleman F, and Vandesompele J

Subjects

Alleles, Cell Line, Gene Expression Regulation, Neoplastic, Gene Transfer Techniques, Genotype, Humans, Neuroblastoma pathology, Reproducibility of Results, Chromosome Mapping methods, Chromosomes, Human, Pair 3, Genes, Tumor Suppressor, Loss of Heterozygosity, Microsatellite Repeats, Neuroblastoma genetics

Abstract

Pinpointing critical regions of recurrent loss may help localize tumor suppressor genes. To determine the regions of loss on chromosome 3p in neuroblastoma, we performed loss of heterozygosity analysis using 16 microsatellite markers in a series of 65 primary tumors and 29 neuroblastoma cell lines. In this study, we report the results and discuss the technical hurdles that we encountered during data generation and interpretation that are of relevance for current studies or tests employing microsatellites. To provide functional support for the implication of 3p tumor suppressor genes in this childhood malignancy, we performed a microcell-mediated chromosome 3 transfer in neuroblastoma cells.

Published

2009

3. Positional and functional mapping of a neuroblastoma differentiation gene on chromosome 11.

Author

De Preter K, Vandesompele J, Menten B, Carr P, Fiegler H, Edsjö A, Carter NP, Yigit N, Waelput W, Van Roy N, Bader S, Påhlman S, and Speleman F

Subjects

Alleles, Cell Differentiation, Cell Line, Chromosome Deletion, Chromosomes, Artificial, Bacterial genetics, Gene Deletion, Heterozygote, Humans, In Situ Hybridization, Fluorescence, Microsatellite Repeats, Neuroblastoma metabolism, Nucleic Acid Hybridization, Oligonucleotide Array Sequence Analysis, Phalloidine pharmacology, Phenotype, RNA, Messenger metabolism, Reverse Transcriptase Polymerase Chain Reaction, Chromosome Mapping methods, Chromosomes, Human, Pair 11 ultrastructure, Genes, Tumor Suppressor, Neuroblastoma genetics, Neuroblastoma pathology

Abstract

Background: Loss of chromosome 11q defines a subset of high-stage aggressive neuroblastomas. Deletions are typically large and mapping efforts have thus far not lead to a well defined consensus region, which hampers the identification of positional candidate tumour suppressor genes. In a previous study, functional evidence for a neuroblastoma suppressor gene on chromosome 11 was obtained through microcell mediated chromosome transfer, indicated by differentiation of neuroblastoma cells with loss of distal 11q upon introduction of chromosome 11. Interestingly, some of these microcell hybrid clones were shown to harbour deletions in the transferred chromosome 11. We decided to further exploit this model system as a means to identify candidate tumour suppressor or differentiation genes located on chromosome 11., Results: In a first step, we performed high-resolution array CGH DNA copy-number analysis in order to evaluate the chromosome 11 status in the hybrids. Several deletions in both parental and transferred chromosomes in the investigated microcell hybrids were observed. Subsequent correlation of these deletion events with the observed morphological changes lead to the delineation of three putative regions on chromosome 11: 11q25, 11p13-->11p15.1 and 11p15.3, that may harbour the responsible differentiation gene., Conclusion: Using an available model system, we were able to put forward some candidate regions that may be involved in neuroblastoma. Additional studies will be required to clarify the putative role of the genes located in these chromosomal segments in the observed differentiation phenotype specifically or in neuroblastoma pathogenesis in general.

Published

2005

4. Assignment of the cellular retinol-binding protein 1 gene (RBP1) and of the coatomer beta subunit gene (COPB2) to human chromosome band 3q23 by in situ hybridization.

Author

De Baere E, Speleman F, Van Roy N, De Paepe A, and Messiaen L

Subjects

Chromosome Banding, Coatomer Protein, Humans, In Situ Hybridization, Fluorescence, Molecular Sequence Data, Retinol-Binding Proteins, Cellular, Chromosome Mapping, Chromosomes, Human, Pair 3, Membrane Proteins genetics, Retinol-Binding Proteins genetics

Published

1998

5. Assignment of SHOX2 (alias OG12X and SHOT) to human chromosome bands 3q25-->q26.1 by in situ hybridization.

Author

De Baere E, Speleman F, Van Roy N, De Paepe A, and Messiaen L

Subjects

Chromosome Banding, Genes, Homeobox genetics, Humans, In Situ Hybridization, Fluorescence, Molecular Sequence Data, Chromosome Mapping, Chromosomes, Human, Pair 3, Homeodomain Proteins genetics

Published

1998

6. Analysis of 1;17 translocation breakpoints in neuroblastoma: implications for mapping of neuroblastoma genes.

Author

Van Roy N, Laureys G, Van Gele M, Opdenakker G, Miura R, van der Drift P, Chan A, Versteeg R, and Speleman F

Subjects

Genes, Tumor Suppressor genetics, Humans, In Situ Hybridization, Fluorescence, Tumor Cells, Cultured, Chromosome Mapping methods, Chromosomes, Human, Pair 1 genetics, Chromosomes, Human, Pair 17 genetics, Neuroblastoma genetics, Translocation, Genetic genetics

Abstract

Deletions and translocations resulting in loss of distal 1p-material are known to occur frequently in advanced neuroblastomas. Fluorescence in situ hybridisation (FISH) showed that 17q was most frequently involved in chromosome 1p translocations. A review of the literature shows that 10 of 27 cell lines carry 1;17 translocations. Similar translocations were also observed in primary tumours. Together with the occurrence of a constitutional 1;17 translocation in a neuroblastoma patient, these observations suggest a particular role for these chromosome re-arrangements in the development of neuroblastoma. Apart from the loss of distal 1p-material, these translocations invariably lead to extra copies of 17q. This also suggested a possible role for genes on 17q in neuroblastoma tumorigenesis. Further support for this hypothesis comes from the observation that in those cell lines without 1;17 translocations, other chromosome 17q translocations were present. These too lead to extra chromosome 17q material. Molecular analysis of 1;17 translocation breakpoints revealed breakpoint heterogeneity both on 1p and 17q, which suggests the involvement of more than 2 single genes on 1p and 17q. The localisation of the different 1p-breakpoints occurring in 1;17 translocations in neuroblastoma are discussed with respect to the recently identified candidate tumor suppressor regions and genes on 1p. In this study, we focused on the molecular analysis of the 17q breakpoints in 1;17 translocations. Detailed physical mapping of the constitutional 17q breakpoint allowed for the construction of a YAC contig covering the breakpoint. Furthermore, a refined position was determined for a number of 17q breakpoints of 1;17 translocations found in neuroblastoma cell lines. The most distal 17q breakpoint was identified in cell line UHG-NP and mapped telomeric to cosmid cCI17-1049 (17q21). This suggests that genes involved in a dosage-dependent manner in the development of neuroblastoma map in the distal segment 17q22-qter. Future studies aim at the molecular cloning of 1;17 translocation breakpoints and at deciphering the mechanisms leading to 1;17 translocations and possibly to the identification of neuroblastoma genes at or in the vicinity of these breakpoints.

Published

1997

7. Comparative genomic hybridization analysis of human neuroblastomas: detection of distal 1p deletions and further molecular genetic characterization of neuroblastoma cell lines.

Author

Van Roy N, Jauch A, Van Gele M, Laureys G, Versteeg R, De Paepe A, Cremer T, and Speleman F

Subjects

Child, Preschool, Chromosome Aberrations pathology, Chromosome Banding, Chromosome Disorders, Chromosomes, Human, Pair 17, Gene Amplification, Genes, myc, Humans, In Situ Hybridization, Fluorescence, Male, Sequence Deletion, Chromosome Deletion, Chromosome Mapping methods, Neuroblastoma genetics, Nucleic Acid Hybridization methods

Abstract

Deletions of the short arm of chromosome 1 and MYCN amplification are the most frequently encountered genetic changes in disseminated neuroblastomas and neuroblastoma cell lines. Different strategies have been followed for detection of these and other genomic changes in neuroblastoma including karyotyping, FISH, and LOH, each with its own limitations. Here we report upon the evaluation of comparative genomic hybridization (CGH) in the analysis of neuroblastoma cell lines, with the emphasis on the assessment of the reliability of CGH for the detection of distal 1p deletions. We have analyzed seven neuroblastoma cell lines for which the 1p status was previously studied in detail using FISH and LOH. Our results show that CGH allows reliable detection of distal 1p deletions, including a small interstitial deletion in cell line SK-N-AS. Furthermore, CGH also allows the detection of chromosomal imbalance which would otherwise remain undetected, and provides useful information for further molecular characterization of chromosomal imbalances.

Published

1997

8. Report and abstracts of the third international workshop on human chromosome 1 mapping 1997.

Author

Vance JM, Matise TC, Wooster R, Schutte BC, Bruns GA, van Roy N, Brodeur GM, Tao YX, Gregory S, Weith A, Vaudin M, and White P

Subjects

Computer Communication Networks, Databases, Factual, Humans, Radiation Chimera, Sequence Analysis, DNA, Chromosome Aberrations, Chromosome Disorders, Chromosome Mapping, Chromosomes, Human, Pair 1

Published

1997

9. Report of the second international workshop on human chromosome 1 mapping 1995.

Author

Weith A, Brodeur GM, Bruns GA, Matise TC, Mischke D, Nizetic D, Seldin MF, van Roy N, and Vance J

Subjects

Humans, Chromosome Mapping, Chromosomes, Human, Pair 1 genetics

Published

1996

10. Identification and characterization of a novel member of the EXT gene family, EXTL2

Author

Wuyts W, Wim Van Hul, Hendrickx J, Speleman F, Wauters J, De Boulle K, Van Roy N, Van Agtmael T, Bossuyt P, Pj, Willems, and Other departments

Subjects

musculoskeletal diseases, Base Sequence, Molecular Sequence Data, Chromosome Mapping, Membrane Proteins, Proteins, Sequence Analysis, DNA, Blotting, Northern, N-Acetylglucosaminyltransferases, Polymerase Chain Reaction, Chromosomes, Human, Pair 2, Genetics, Humans, Genes, Tumor Suppressor, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, human activities, Sequence Alignment, Genetics (clinical), Exostoses, Multiple Hereditary, In Situ Hybridization, Fluorescence, Pseudogenes, DNA Primers

Abstract

Recently, two homologous genes, EXT1 and EXT2, with a putative tumor suppressor function have been described. Mutations in both genes are responsible for multiple exostosis syndrome (EXT), an autosomal dominant condition characterized by the presence of multiple osteochondromas, bony excrescences that sometimes undergo malignant transformation to chondrosarcoma. This family of EXT genes has been extended by the identification of an EXT-like (EXTL) gene showing a high degree of homology with the EXT genes. We report here a second EXT-like gene (EXTL2) which is homologous to the EXT and EXTL genes. EXTL2 consists of 5 exons encoding an ubiquitously expressed protein of 330 amino acids. In addition, a putative pseudogene, EXTL2P was also identified. The EXTL2 gene was assigned to chromosome 1p11-p12, whereas EXTL2P was mapped on chromosome 2q24-q31.

Published

1998

11. Deletion mapping in neuroblastoma cell lines suggests two distinct tumor suppressor genes in the 1p35-36 region, only one of which is associated with N-myc amplification

Author

Nc, Cheng, Van Roy N, Chan A, Beitsma M, Westerveld A, Speleman F, Rogier Versteeg, and Other departments

Subjects

Blotting, Southern, Neuroblastoma, Chromosomes, Human, Pair 1, Gene Amplification, Genes, myc, Tumor Cells, Cultured, Chromosome Mapping, Humans, Genes, Tumor Suppressor, Chromosome Deletion, Hybrid Cells, Blotting, Northern

Abstract

Neuroblastoma is characterized by deletions of the short arm of chromosome 1 (1p) and amplification of the N-myc oncogene. We have made somatic cell hybrids of two human neuroblastoma cell lines, one with and one without N-myc expression and amplification. The expression of the amplified N-myc gene is completely switched off in the hybrids. This suggests that N-myc expression results from loss of a repressor function. As N-myc amplification is associated with loss of heterozygosity (LOH) of 1p36, we analysed 1p deletions in 16 neuroblastoma cell lines. The seven cell lines without N-myc amplification have no deletions or relatively small deletions, with an SRO on 1p36.23-33. This suggests that a tumor suppressor gene maps in this region. All nine cell lines with N-myc amplification have larger deletions, with an SRO from 1p35-36.1 to the telomere. This suggests that a second tumor suppressor gene which is associated with N-myc amplification maps more proximally. Fine mapping of 1p36 deletions in the two cell lines of the fusion experiment suggests that the distal locus is not a repressor of N-myc expression, but the more proximal locus could be a candidate for this function.

Published

1995

12. Constitutional translocation t(1;17)(p36.31-p36.13;q11.2-q12.1) in a neuroblastoma patient. Establishment of somatic cell hybrids and identification of PND/A12M2 on chromosome 1 and NF1/SCYA7 on chromosome 17 as breakpoint flanking single copy markers

Author

Laureys G, Speleman F, Rogier Versteeg, van der Drift P, Chan A, Leroy J, Francke U, Opdenakker G, Van Roy N, and Other departments

Subjects

Genetic Markers, Neurofibromin 1, Chromosome Mapping, Proteins, Hybrid Cells, Translocation, Genetic, Blotting, Southern, Neuroblastoma, Cricetulus, Chromosomes, Human, Pair 1, Cricetinae, Animals, Humans, Genes, Tumor Suppressor, Chromosomes, Human, Pair 17

Abstract

Cytogenetic and molecular studies in neuroblastoma suggest the presence of a tumor suppressor gene at the distal band p36 of human chromosome 1. We described a constitutional translocation t(1;17)(p36;q12-q21), involving the critical region 1p36, in a patient with neuroblastoma, and hypothesized that the translocation predisposed the patient to tumor development. Here we report the molecular delineation of the translocation breakpoints. Somatic cell hybrids were generated by fusion of the patient's fibroblasts with the thymidine kinase deficient hamster cell line, a3. In hybrid cell lines which retained the human derivative chromosomes, the position of chromosome 1p and 17q DNA probes respective to the translocation breakpoints was determined by fluorescence in situ hybridization and Southern blot analysis. The chromosome 1p breakpoint was localized within a repetitive region encoding t-RNA genes, with 12A-2 (PND) as most distal and pHE2.6 (A12M2) as most proximal single-copy breakpoint flanking markers. For the chromosome 17 breakpoint, the proximal and distal flanking markers were identified as 7G4 (NF1) and cMCP-3 (SCYA7), respectively. In this study, cMCP-3 (SCYA7), encoding the human monocyte chemotactic protein-3, was mapped between NF1 and ERBB2. As a pivotal step towards breakpoint cloning, at present these flanking markers optimally delineate the breakpoint regions of both chromosomes 1 and 17 at the molecular level.

13. Mapping of novel regions of DNA gain and loss by comparative genomic hybridization in esophageal carcinoma in the black and colored populations of South Africa

Author

Du Plessis L, Dietzsch E, Van Gele M, Van Roy N, Van Helden P, Mi, Parker, Dk, Mugwanya, De Groot M, Mp, Marx, Martha Kotze, and Speleman F

Subjects

Male, South Africa, Esophageal Neoplasms, Gene Dosage, Black People, Chromosome Mapping, Humans, Nucleic Acid Hybridization, Female, DNA, Neoplasm, Chromosome Deletion

Abstract

Esophageal cancer (EC) is the leading cause of cancer death in the Black male population in South Africa. Although several oncogenes and tumor suppressor genes have previously been found altered in this cancer, many novel genes remain to be identified. To identify the chromosomal location of these unknown genes, we have analyzed DNA of 29 South African EC patients by comparative genomic hybridization. Frequent loss occurred at chromosome 1p (52%), 4p (52%), 18q (48%), 19p (52%), 19q (55%), and 22q (41%). The most common gains were detected at 1q (41%), 2q (52%), 3q (72%), 5p (31%), 7p (48%), 7q (45%), 8q (55%), and Xq (69%). High level amplification was detected at 2q24-33, 6p21.1-q14, 7p12-q21, 7q11.2-31, 8q22-24, 8q13-qter, 13q21-34, and at 13q32-34. The present comparative genomic hybridization study opens the way for additional targeted studies on these particular chromosomal regions to identify the specific genes involved in the higher susceptibility to specific subtypes of esophageal carcinoma in different geographical regions. The loss of 8p (28%) and Xp (17%) in tumors of male individuals may provide clues to the basis of the sex-biased frequency of occurrence of EC favoring men.