Your search keyword '"Van Roy N"' showing total 15 results

1. Improved detection of chromosomal abnormalities in chronic lymphocytic leukemia by conventional cytogenetics using CpG oligonucleotide and interleukin-2 stimulation: A Belgian multicentric study.

Author

Put N, Konings P, Rack K, Jamar M, Van Roy N, Libouton JM, Vannuffel P, Sartenaer D, Ameye G, Speleman F, Herens C, Poirel HA, Moreau Y, Hagemeijer A, Vandenberghe P, and Michaux L

Subjects

Adult, Aged, Aged, 80 and over, Cell Proliferation drug effects, Chromosome Banding, Data Interpretation, Statistical, Female, Humans, In Situ Hybridization, Fluorescence, Karyotyping methods, Leukemia, Lymphocytic, Chronic, B-Cell pathology, Male, Middle Aged, Prospective Studies, Retrospective Studies, Translocation, Genetic, Tumor Cells, Cultured, Chromosome Aberrations, Cytogenetics methods, Interleukin-2 pharmacology, Leukemia, Lymphocytic, Chronic, B-Cell genetics, Oligonucleotides pharmacology

Abstract

We performed a multicentric study to assess the impact of two different culture procedures on the detection of chromosomal abnormalities in 217 consecutive unselected cases with chronic lymphocytic leukemia (CLL) referred for routine analysis either at the time of diagnosis (n = 172) or during disease evolution (n = 45). Parallel cultures of peripheral blood or bone marrow were set up with the addition of either the conventional B-cell mitogen 12-O-tetradecanoyl-phorbol-13-acetate (TPA) or a combination of CpG oligonucleotide (CpG) and interleukin-2 (IL-2). Cytogenetic analyses were performed on both cultures. Clonal abnormalities were identified in 116 cases (53%). In 78 cases (36%), the aberrant clone was detected in both cultures. Among these, the percentages of aberrant metaphases were similar in both conditions in 17 cases, higher in the CpG/IL-2 culture in 43 cases, and higher in the TPA culture in 18 cases. Clonal aberrations were detected in only one culture, either in CpG/IL-2 or TPA in 33 (15%) and 5 (2%) cases, respectively. Taken together, abnormal karyotypes were observed in 51% with CpG/IL-2 and 38% with TPA (P < 0.0001). Application of FISH (n = 201) allowed the detection of abnormalities not visible by conventional cytogenetic analysis in 80 cases: del(13q) (n = 71), del(11q) (n = 5), +12 (n = 2), del(14q) (n = 1), and del(17p) (n = 1). In conclusion, our results confirm that CpG/IL-2 stimulation increases the detection rate of chromosomal abnormalities in CLL compared with TPA and that further improvement can be obtained by FISH. However, neither conventional cytogenetics nor FISH detected all aberrations, demonstrating the complementary nature of these techniques., ((c) 2009 Wiley-Liss, Inc.)

Published

2009

2. ArrayCGH-based classification of neuroblastoma into genomic subgroups.

Author

Michels E, Vandesompele J, De Preter K, Hoebeeck J, Vermeulen J, Schramm A, Molenaar JJ, Menten B, Marques B, Stallings RL, Combaret V, Devalck C, De Paepe A, Versteeg R, Eggert A, Laureys G, Van Roy N, and Speleman F

Subjects

Cell Line, Tumor, Child, Child, Preschool, Gene Amplification, Gene Dosage, Humans, Infant, Infant, Newborn, Neuroblastoma diagnosis, Oligonucleotide Array Sequence Analysis, Reproducibility of Results, Genome, Human, Neuroblastoma classification, Neuroblastoma genetics

Abstract

High-resolution array comparative genomic hybridization (arrayCGH) profiling was performed on 75 primary tumors and 29 cell lines to gain further insight into the genetic heterogeneity of neuroblastoma and to refine genomic subclassification. Using a novel data-mining strategy, three major and two minor genomic subclasses were delineated. Eighty-three percent of tumors could be assigned to the three major genomic subclasses, corresponding to the three known clinically and biologically relevant subsets in neuroblastoma. The remaining subclasses represented (1) tumors with no/few copy number alterations or an atypical pattern of aberrations and (2) tumors with 11q13 amplification. Inspection of individual arrayCGH profiles showed that recurrent genomic imbalances were not exclusively associated with a specific subclass. Of particular notice were tumors with numerical imbalances typically observed in subtype 1 neuroblastoma, in association with genomic features of subtype 2A or 2B. A search for prognostically relevant genomic alterations disclosed 1q gain as a predictive marker for therapy failure within the group of subtype 2A and 2B tumors. In cell lines, a high incidence of 6q loss was observed, with a 3.87-5.32 Mb region of common loss within 6q25.1-6q25.2. Our study clearly illustrates the importance of genomic profiling in relation to tumor behavior in neuroblastoma. We propose that genome-wide assessment of copy number alterations should ideally be included in the genetic workup of neuroblastoma. Further multicentric studies on large tumor series are warranted in order to improve therapeutic stratification in conjunction with other features such as age at diagnosis, tumor stage, and gene expression signatures., ((c) 2007 Wiley-Liss, Inc.)

Published

2007

3. Translocation-excision-deletion-amplification mechanism leading to nonsyntenic coamplification of MYC and ATBF1.

Author

Van Roy N, Vandesompele J, Menten B, Nilsson H, De Smet E, Rocchi M, De Paepe A, Påhlman S, and Speleman F

Subjects

Cell Line, Tumor, Chromosomes, Human, Pair 16, Chromosomes, Human, Pair 8, Humans, In Situ Hybridization, Fluorescence, Proto-Oncogene Mas, Gene Amplification, Gene Deletion, Genes, myc, Homeodomain Proteins genetics, Translocation, Genetic

Abstract

Despite oncogene amplification being a characteristic of many tumor types, the mechanisms leading to amplicon formation have remained largely unresolved. In this study, we used a combinatorial approach of fluorescence in situ hybridization and single-nucleotide polymorphism chip gene copy number analyses to unravel the mechanism leading to nonsyntenic coamplification of MYC and ATBF1 in SJNB-12 cells. To explain our findings, we propose a complex series of events consisting of multiple double-strand breaks, accompanied (or triggered) by the formation of a reciprocal translocation t(8;16), as well as excisions and deletions near the translocation breakpoints. This study provides evidence for a translocation-excision-deletion-amplification sequence of events rather than a breakage-fusion-bridge model, which has been more frequently proposed to explain proto-oncogene amplification. Furthermore, it illustrates the power of presently available tools for detailed analysis of the complex rearrangements that accompany amplicon formation.

Published

2006

4. Localization of the 17q breakpoint of a constitutional 1;17 translocation in a patient with neuroblastoma within a 25-kb segment located between the ACCN1 and TLK2 genes and near the distal breakpoints of two microdeletions in neurofibromatosis type 1 patients.

Author

Van Roy N, Vandesompele J, Berx G, Staes K, Van Gele M, De Smet E, De Paepe A, Laureys G, van der Drift P, Versteeg R, Van Roy F, and Speleman F

Subjects

Chromosome Deletion, Chromosomes, Artificial, Bacterial genetics, Chromosomes, Artificial, P1 Bacteriophage genetics, Cloning, Molecular, Contig Mapping methods, Genes genetics, Genetic Markers genetics, Humans, Proto-Oncogenes genetics, Central Nervous System Neoplasms genetics, Chromosome Breakage genetics, Chromosomes, Human, Pair 1 genetics, Chromosomes, Human, Pair 17 genetics, Neuroblastoma genetics, Neurofibromatosis 1 genetics, Translocation, Genetic genetics

Abstract

We have constructed a 1.4-Mb P1 artificial chromosome/bacterial artificial chromosome (PAC/BAC) contig spanning the 17q breakpoint of a constitutional translocation t(1;17)(p36.2;q11.2) in a patient with neuroblastoma. Three 17q breakpoint-overlapping cosmids were identified and sequenced. No coding sequences were found in the immediate proximity of the 17q breakpoint. The PAC/BAC contig covers the region between the proximally located ACCN1 gene and the distally located TLK2 gene and SCYA chemokine gene cluster. The observation that the 17q breakpoint region could not be detected in any of the screened yeast artificial chromosome libraries and the localization of the 17q breakpoint in the vicinity of the distal breakpoints of two microdeletions in patients with neurofibromatosis type 1 suggest that this chromosomal region is genetically unstable and prone to rearrangements., (Copyright 2002 Wiley-Liss, Inc.)

Published

2002

5. Combined M-FISH and CGH analysis allows comprehensive description of genetic alterations in neuroblastoma cell lines.

Author

Van Roy N, Van Limbergen H, Vandesompele J, Van Gele M, Poppe B, Salwen H, Laureys G, Manoel N, De Paepe A, and Speleman F

Subjects

Female, Humans, Karyotyping, Male, Tumor Cells, Cultured, Chromosome Painting methods, In Situ Hybridization, Fluorescence methods, Neuroblastoma genetics, Nucleic Acid Hybridization methods

Abstract

Cancer cell lines are essential gene discovery tools and have often served as models in genetic and functional studies of particular tumor types. One of the future challenges is comparison and interpretation of gene expression data with the available knowledge on the genomic abnormalities in these cell lines. In this context, accurate description of these genomic abnormalities is required. Here, we show that a combination of M-FISH with banding analysis, standard FISH, and CGH allowed a detailed description of the genetic alterations in 16 neuroblastoma cell lines. In total, 14 cryptic chromosome rearrangements were detected, including a balanced t(2;4)(p24.3;q34.3) translocation in cell line NBL-S, with the 2p24 breakpoint located at about 40 kb from MYCN. The chromosomal origin of 22 marker chromosomes and 41 cytogenetically undefined translocated segments was determined. Chromosome arm 2 short arm translocations were observed in six cell lines (38%) with and five (31%) without MYCN amplification, leading to partial chromosome arm 2p gain in all but one cell line and loss of material in the various partner chromosomes, including 1p and 11q. These 2p gains were often masked in the GGH profiles due to MYCN amplification. The commonly overrepresented region was chromosome segment 2pter-2p22, which contains the MYCN gene, and five out of eleven 2p breakpoints clustered to the interface of chromosome bands 2p16 and 2p21. In neuroblastoma cell line SJNB-12, with double minutes (dmins) but no MYCN amplification, the dmins were shown to be derived from 16q22-q23 sequences. The ATBF1 gene, an AT-binding transcription factor involved in normal neurogenesis and located at 16q22.2, was shown to be present in the amplicon. This is the first report describing the possible implication of ATBF1 in neuroblastoma cells. We conclude that a combined approach of M-FISH, cytogenetics, and CGH allowed a more complete and accurate description of the genetic alterations occurring in the investigated cell lines., (Copyright 2001 Wiley-Liss, Inc.)

Published

2001

6. Molecular cytogenetic and clinical findings in ETV6/ABL1-positive leukemia.

Author

Van Limbergen H, Beverloo HB, van Drunen E, Janssens A, Hählen K, Poppe B, Van Roy N, Marynen P, De Paepe A, Slater R, and Speleman F

Subjects

Child, Preschool, Chromosome Deletion, Humans, In Situ Hybridization, Fluorescence, Leukemia, Myelogenous, Chronic, BCR-ABL Positive blood, Leukemia-Lymphoma, Adult T-Cell blood, Male, Middle Aged, Proto-Oncogene Proteins c-ets, Reverse Transcriptase Polymerase Chain Reaction, Translocation, Genetic genetics, ETS Translocation Variant 6 Protein, DNA-Binding Proteins genetics, Genes, abl genetics, Karyotyping, Leukemia, Myelogenous, Chronic, BCR-ABL Positive genetics, Leukemia-Lymphoma, Adult T-Cell genetics, Oncogene Proteins, Fusion genetics, Repressor Proteins, Transcription Factors genetics

Abstract

Rearrangements of 12p, resulting from deletions or translocations, are common findings in hematologic malignancies. In many cases, these rearrangements target the ETV6 gene (previously called TEL) located at 12p13. Various partner genes have been implicated in the formation of fusion genes with ETV6. These include PDGFRB, JAK2, NTRK3, ABL2, and ABL1, each of which encodes for proteins with tyrosine kinase activity. To date, ETV6/ABL1 transcripts have been detected in only four patients with a leukemic disorder. Here, we describe one adult with chronic myeloid leukemia and a child with T-cell acute lymphocytic leukemia with ETV6/ABL1. Molecular cytogenetic analysis confirmed that formation of an ETV6/ABL1 fusion in these patients required at least three chromosomal breaks and showed that each of these translocations is the result of a complex chromosomal rearrangement. Molecular analysis showed the presence of two fusion transcripts in both patients as the result of alternative splicing, questioning the suggested role of these transcripts in the lineage specificity. Clinical findings of these patients were compared to those of previously reported cases, and the possible clinical and biological similarities between ETV6/ABL1 and other fusion genes leading to increased tyrosine kinase activity are discussed., (Copyright 2001 Wiley-Liss, Inc.)

Published

2001

7. Genetic heterogeneity of neuroblastoma studied by comparative genomic hybridization.

Author

Vandesompele J, Van Roy N, Van Gele M, Laureys G, Ambros P, Heimann P, Devalck C, Schuuring E, Brock P, Otten J, Gyselinck J, De Paepe A, and Speleman F

Subjects

Adolescent, Child, Child, Preschool, Chromosome Aberrations genetics, Chromosome Disorders, DNA, Neoplasm analysis, Gene Amplification, Humans, Infant, Infant, Newborn, Loss of Heterozygosity, Male, Genetic Heterogeneity, Neuroblastoma genetics, Nucleic Acid Hybridization methods

Abstract

Comparative genomic hybridization (CGH) analysis was performed on 36 neuroblastomas of both low and high stage of disease. This study significantly increases the number of neuroblastoma tumors studied by CGH. Analysis of larger series of tumors is particularly important in view of the different clinical subgroups that are recognized for this tumor. The present data and a comparison with all published CGH data on neuroblastoma provide further insights into the genetic heterogeneity of neuroblastoma. Stage 1, 2, and 4S tumors showed predominantly whole chromosome gains and losses. A similar pattern of whole chromosome imbalances, although less frequent, was observed in stage 3 and 4 tumors, in addition to partial chromosome gains and losses. An increase in chromosome 17 or 17q copy number was observed in 81% of tumors. The most frequent losses, either through partial or whole chromosome underrepresentation, were observed for 1p (25%), 3p (25%), 4p (14%), 9p (19%), 11q (28%), and 14q (31%). The presence of 3p, 11q or 14q deletions defines a genetic subset of neuroblastomas and contributes to the further genetic characterization of stage 3 and 4 tumors without MYCN amplification (MNA) and 1p deletion. The present study also provides additional evidence for a possible role of genes at 11q13 in neuroblastoma. In a few cases, 1p deletion or MNA detected by FISH or Southern blotting was not found by CGH, indicating that the use of a second, independent technique for evaluation of these genetic parameters is recommended.

Published

1998

8. Molecular cytogenetic delineation of 17q translocation breakpoints in neuroblastoma cell lines.

Author

Lastowska M, Van Roy N, Bown N, Speleman F, Lunec J, Strachan T, Pearson AD, and Jackson MS

Subjects

Genetic Markers, Humans, In Situ Hybridization, Fluorescence, Metaphase, Neuroblastoma pathology, Tumor Cells, Cultured, Chromosome Breakage genetics, Chromosomes, Human, Pair 17 genetics, Neuroblastoma genetics, Translocation, Genetic genetics

Abstract

It has recently been recognized that unbalanced translocations resulting in the gain of material from 17q are the most common chromosomal changes in neuroblastoma. These rearrangements are associated with established indicators of bad prognosis and poor patient survival. We have used 13 fluorescence in situ hybridization (FISH) probes to map 12 translocation breakpoints on 17q in 10 neuroblastoma cell lines, identifying at least seven different breakpoints, all localized within the proximal half of 17q (268-369 cR, 53-68 cM). These results suggest that the dosage of a gene, or genes, in 17q22-qter is responsible for the clinical effects of 17q gain, rather than the disruption of a specific gene. This region contains two genes, nm23-H1 and NGFR, already implicated in neuroblastoma biology.

Published

1998

9. Molecular analysis of 1p36 breakpoints in two Merkel cell carcinomas.

Author

Van Gele M, Van Roy N, Ronan SG, Messiaen L, Vandesompele J, Geerts ML, Naeyaert JM, Blennow E, Bar-Am I, Das Gupta TK, van der Drift P, Versteeg R, Leonard JH, and Speleman F

Subjects

Aged, Aged, 80 and over, Chromosome Aberrations, Chromosome Banding, Chromosome Disorders, Chromosome Fragility, Female, Humans, In Situ Hybridization, Fluorescence, Karyotyping, Loss of Heterozygosity, Microsatellite Repeats genetics, Tumor Cells, Cultured, Carcinoma, Merkel Cell genetics, Chromosomes, Human, Pair 1 genetics, Skin Neoplasms genetics

Abstract

Merkel cell carcinoma (MCC) is a rare aggressive neuroendocrine tumor of the skin. Only little information is available on the genetic alterations occurring in this tumor. Cytogenetic studies thus far have not shown recurrent chromosomal changes, although various structural chromosome 1 rearrangements, including deletions, often leading to loss of distal 1p material appear to be frequent. We report on fluorescence in situ hybridization and loss of heterozygosity analyses of an MCC tumor and MCC cell line UISO. The present study has shown that two distinct regions in the most distal band 1p36 on the short arm of chromosome 1 can be implicated in MCC. One region at 1p36.3 was delineated by a distal deletion in the MCC tumor as a result of an unbalanced translocation, resulting in loss of all markers distal to ENO1. This region was previously shown to be deleted in different tumor types including neuroblastoma. In cell line UISO an insertion in 1p36.2 was identified. The insertion breakpoint indicates a second, more proximal, region on 1p involved in MCC. The insertion breakpoint was mapped within a cluster of repetitive tRNA and snRNA genes and thus could coincide with the constitutional 1p36 breakpoint previously reported in a patient with neuroblastoma.

Published

1998

10. Cytogenetic and molecular analysis of cellular atypical mesoblastic nephroma.

Author

Speleman F, van den Berg E, Dhooge C, Oosterhuis W, Redeker B, De Potter CR, Tamminga RY, Van Roy N, and Mannens M

Subjects

Chromosome Banding, Female, Humans, Infant, Karyotyping, Loss of Heterozygosity, Male, Trisomy, Chromosomes, Human genetics, Kidney Neoplasms genetics, Nephroma, Mesoblastic genetics

Abstract

Cytogenetic and molecular analyses were performed on three cellular (atypical) congenital mesoblastic nephromas (CMNs). Two cases had trisomy 11; in one, it was the sole karyotypic abnormality, and the other had additional numerical changes as well as an isochromosome for the long arm of chromosome 1. Markers for the 11p13 and 11p15 loci were present in three copies in these two CMNs. In the third CMN, two apparently normal copies of chromosome 11 were present together with additional numerical and structural chromosome changes. Because loss of heterozygosity was observed for both 11p13 and 11p15 markers, we assume that mitotic recombination occurred. Duplication and loss of imprinting of genes at 11p15 has also been observed frequently in Wilms' tumor. We therefore propose that CMN and Wilms' tumor might share common genetic pathways.

Published

1998

11. Monosomy 22 in a mixed germ cell-sex cord-stromal tumor of the ovary.

Author

Speleman F, Dermaut B, De Potter CR, Van Gele M, Van Roy N, De Paepe A, and Laureys G

Subjects

Female, Germinoma pathology, Humans, Infant, Karyotyping, Monosomy, Ovarian Neoplasms pathology, Sex Cord-Gonadal Stromal Tumors pathology, Chromosomes, Human, Pair 22 genetics, Germinoma genetics, Ovarian Neoplasms genetics, Sex Cord-Gonadal Stromal Tumors genetics

Abstract

We report the cytogenetic findings in a case of mixed germ cell-sex cord-stromal tumor of the ovary in a 5-month-old girl. Monosomy 22 was observed as the sole karyotypic abnormality. This result was confirmed by comparative genomic hybridization, which revealed no additional chromosomal imbalances. This is the first observation of a chromosomal aberration in a mixed germ cell-sex cord-stromal tumor of the ovary. Monosomy 22 has been previously observed in granulosa cell tumors of the ovary. This could suggest a common pathogenetic pathway for both types of tumors.

Published

1997

12. Balanced translocation in a neuroblastoma patient disrupts a cluster of small nuclear RNA U1 and tRNA genes in chromosomal band 1p36.

Author

van der Drift P, Chan A, Laureys G, van Roy N, Sickmann G, den Dunnen J, Westerveld A, Speleman F, and Versteeg R

Subjects

Animals, Base Sequence, Chromosome Banding, Chromosomes, Human, Pair 17, Cricetinae, DNA Primers, Humans, Molecular Sequence Data, Chromosomes, Human, Pair 1, Multigene Family, Neuroblastoma genetics, RNA, Small Nuclear genetics, RNA, Transfer genetics, Translocation, Genetic

Abstract

Chromosomal band 1p36 probably harbours several neuroblastoma suppressor genes. A neuroblastoma patient has been described with a constitutional balanced translocation, t(1;17)(p36;q12-21). Cytogenetically, no loss of chromosomal material was visible. The 1p36 translocation breakpoint could therefore have inactivated one allele of a tumour suppressor gene, thus predisposing the patient to develop neuroblastoma. We localized this breakpoint by pulsed field gel electrophoresis, analysis of yeast artificial chromosomes, and fluorescence in situ hybridization. Here we report that the breakpoint is within a large cluster of small nuclear RNA U1 (RNU1) and some tRNA genes (TRE, TRN) on chromosomal band 1p36. The size of this cluster is over two megabases and it contains many other locally repeated sequences. Polyadenylated transcripts were identified for some of these sequences. In addition, the cluster is the target for integration of an adenovirus 5/SV40 hybrid virus. The translocation breakpoint maps distal of this viral integration site and proximal of marker PND.

Published

1995

13. 1;17 translocations and other chromosome 17 rearrangements in human primary neuroblastoma tumors and cell lines.

Author

Van Roy N, Laureys G, Cheng NC, Willem P, Opdenakker G, Versteeg R, and Speleman F

Subjects

Adrenal Gland Neoplasms genetics, Adrenal Gland Neoplasms pathology, Adrenal Gland Neoplasms secondary, Bone Marrow pathology, Bone Neoplasms genetics, Bone Neoplasms pathology, Bone Neoplasms secondary, Brain Neoplasms pathology, Cell Line, Child, Preschool, Chromosome Banding, Humans, In Situ Hybridization, Fluorescence, Karyotyping, Male, Neuroblastoma pathology, Neuroblastoma secondary, Tumor Cells, Cultured, Brain Neoplasms genetics, Chromosome Aberrations, Chromosome Disorders, Chromosomes, Human, Pair 1, Chromosomes, Human, Pair 17, Neuroblastoma genetics, Translocation, Genetic

Abstract

We report on the finding of a t(1;17) in two primary neuroblastomas. Subsequent fluorescence in situ hybridization (FISH) analysis revealed the presence of 1;17 translocations in four out of nine neuroblastoma cell lines. The chromosome 1 short arm breakpoints were determined using region-specific probes. FISH screening also demonstrated or confirmed the presence of 11;17 translocations in three cell lines and other chromosome 17 rearrangements in those cell lines that did not carry a t(1;17) or t(11;17). Our data extend previous cytogenetic findings and suggest that, in addition to the known involvement of chromosome 1, one or more genes on chromosome 17 also play a role in neuroblastoma development.

Published

1994

14. Molecular cytogenetic analysis of a complex t(10;22;11) translocation in Ewing's sarcoma.

Author

Speleman F, Van Roy N, Wiegant J, Dierick AM, Uyttendaele D, and Leroy JG

Subjects

Adult, Chromosomes, Human, Pair 10, Chromosomes, Human, Pair 11, Chromosomes, Human, Pair 22, Chromosomes, Human, Pair 8, Female, Humans, Karyotyping, Microscopy, Fluorescence, Nucleic Acid Hybridization, Tibia pathology, Tumor Cells, Cultured, Bone Neoplasms genetics, Sarcoma, Ewing genetics, Translocation, Genetic

Abstract

Fluorescence in situ hybridization (FISH) using chromosome-specific plasmid libraries and chromosome region-specific DNA markers allowed the characterization of a t(10;22;11) (p11.2;q12;q24) in a Ewing's sarcoma (ES). This study illustrates the usefulness of molecular cytogenetic analysis of ES, especially for determining the localization of the translocated 11q24-25 segment in complex or variant translocations.

Published

1992

15. Is t(6;20)(p21;q13) a characteristic chromosome change in endometrial polyps?

Author

Speleman F, Dal Cin P, Van Roy N, Van Marck E, Buytaert P, Van den Berghe H, and Leroy JG

Subjects

Breast Neoplasms, Female, Gene Rearrangement, Humans, Middle Aged, Neoplasms, Multiple Primary, Biomarkers, Tumor genetics, Chromosomes, Human, Pair 20 ultrastructure, Chromosomes, Human, Pair 6 ultrastructure, Genetic Markers, Polyps genetics, Translocation, Genetic, Uterine Neoplasms genetics

Abstract

Cytogenetic analysis of an endometrial polyp showed the presence of a t(6;20)(p21;q13) together with an ins(16;1)(q22;q32q42). Since a 6;20-translocation has been previously found in another endometrial polyp, we think that t(6;20)(p21;q13) may be a characteristic chromosomal change in endometrial polyps.

Published

1991