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3. 9B.09: IDENTIFICATION OF MARKERS PREDICTIVE FOR MALIGNANT BEHAVIOR OF PHEOCHROMOCYTOMAS AND PARAGANGLIOMAS

Author

Evenepoel, Lucie, Van Nederveen, F H, Oudijk, L, Papathomas, T G, Restuccia, D F, Belt, E J T, Franssen, G J H, Feelders, R A, Van Eeden, S, Timmers, H, De Herder, W W, Aydin, Selda, Vikkula, Miikka, De Krijger, R R, Dinjens, W N M, Persu, Alexandre, Korpershoek, E, 25th European Meeting on Hypertension and Cardiovascular Protection, UCL - (SLuc) Service d'anatomie pathologique, UCL - SSS/DDUV - Institut de Duve, UCL - SSS/IREC/NEFR - Pôle de Néphrologie, UCL - SSS/IREC/CARD - Pôle de recherche cardiovasculaire, UCL - (SLuc) Centre de génétique médicale UCL, and UCL - (SLuc) Service de pathologie cardiovasculaire

Subjects
Pathology, medicine.medical_specialty, Mutation, Tissue microarray, Physiology, business.industry, SDHB, IL13RA2, Vascular damage Radboud Institute for Molecular Life Sciences [Radboudumc 16], Interleukin-13 receptor, medicine.disease_cause, Genetic marker, Internal Medicine, Medicine, Immunohistochemistry, Cardiology and Cardiovascular Medicine, business, Gene
Abstract

Item does not contain fulltext OBJECTIVE: Pheochromocytomas and paragangliomas (PPGL) are relatively rare and mostly benign tumours. Approximately 10% of PPGL are malignant, as defined by the presence of metastases, i.e chromaffin tissue at a location that usually does not contain chromaffin cells. However, up to 35% of tumours in patients carrying an SDHB mutation appears to be malignant. Nowadays, no reliable marker allows to predict whether a PPGL is, or will become malignant. In addition, there are no curative treatments if metastases occur. The aim of the present study was to dentify genetic markers allowing to distinguish benign from malignant tumours. DESIGN AND METHOD: An mRNA expression array was performed on benign and malignant PPGL. The genes showing a different expression between the benign and malignant tumours were selected to be confirmed and validated by qRT-PCR. Finally, the remaining genes were stained by immunohistochemistry on Tissue MicroArray including a large series of PPGL. RESULTS: Forty benign and 12 malignant PPGL were investigated for differences in mRNA expression with Affymetrix arrays. Expression data were normalized according to Affymetrix recommendations. Then, using Pomelo II (http://pomelo2.bioinfo.cnio.es/), a Limma t-test was performed, to assess which genes were differentially expressed between benign and malignant PPGL. First, a non-clustered analysis was performed and 10 genes with a False Discovery Rate (FDR) below 0.05 and a relative overexpression ratio of at least 4 were found, including Interleukin 13 Receptor alpha 2 (IL13RA2) and Monooxygenase DBH-like 1 (MOXD1). Secondly, a supervised cluster analysis was performed (based on HIF target genes), resulting in 2 groups, which were both investigated for differences in mRNA expression between benign and malignant tumours. Five genes showed an FDR below 0.01 and were overexpressed in malignant tumours with a ratio higher than 4, including Contactin 4 (CNTN4), Iroquois Homeobox 3 (IRX3), and Sulfatase 2 (SULF2). These genes were further investigated using qRT-PCR, and immunohistochemistry on Tissue Micro Array including 91 benign and 12 malignant PPGL. CONCLUSIONS: Significant overexpression of Contactin 4 was shown in malignant compared to benign tumours, and may therefore contribute to distinguish malignant from benign PPGL.

Published
2015

4. Immunohistochemical expression of stem cell markers in pheochromocytomas/paragangliomas is associated with SDHx mutations

Author

Oudijk, L., Neuhofer, C. M., Lichtenauer, U. D., Papathomas, T. G., Korpershoek, E., Stoop, H., Oosterhuis, J. W., Smid, M., Restuccia, D. F., Robledo, M., De Cubas, A. A., Mannelli, M., Gimenez-Roqueplo, A. P., Dinjens, W. N M, Beuschlein, F., De Krijger, R. R., Oudijk, L., Neuhofer, C. M., Lichtenauer, U. D., Papathomas, T. G., Korpershoek, E., Stoop, H., Oosterhuis, J. W., Smid, M., Restuccia, D. F., Robledo, M., De Cubas, A. A., Mannelli, M., Gimenez-Roqueplo, A. P., Dinjens, W. N M, Beuschlein, F., and De Krijger, R. R.

Published
2015

5. 9B.09: Identification of markers predictive for malignant behaviour of Pheochromocytomas and paragangliomas

Author

UCL - (SLuc) Service d'anatomie pathologique, UCL - SSS/DDUV - Institut de Duve, UCL - SSS/IREC/NEFR - Pôle de Néphrologie, UCL - SSS/IREC/CARD - Pôle de recherche cardiovasculaire, UCL - (SLuc) Centre de génétique médicale UCL, UCL - (SLuc) Service de pathologie cardiovasculaire, Evenepoel, Lucie, Van Nederveen, F H, Oudijk, L, Papathomas, T G, Restuccia, D F, Belt, E J T, Franssen, G J H, Feelders, R A, Van Eeden, S, Timmers, H, De Herder, W W, Aydin, Selda, Vikkula, Miikka, De Krijger, R R, Dinjens, W N M, Persu, Alexandre, Korpershoek, E, 25th European Meeting on Hypertension and Cardiovascular Protection, UCL - (SLuc) Service d'anatomie pathologique, UCL - SSS/DDUV - Institut de Duve, UCL - SSS/IREC/NEFR - Pôle de Néphrologie, UCL - SSS/IREC/CARD - Pôle de recherche cardiovasculaire, UCL - (SLuc) Centre de génétique médicale UCL, UCL - (SLuc) Service de pathologie cardiovasculaire, Evenepoel, Lucie, Van Nederveen, F H, Oudijk, L, Papathomas, T G, Restuccia, D F, Belt, E J T, Franssen, G J H, Feelders, R A, Van Eeden, S, Timmers, H, De Herder, W W, Aydin, Selda, Vikkula, Miikka, De Krijger, R R, Dinjens, W N M, Persu, Alexandre, Korpershoek, E, and 25th European Meeting on Hypertension and Cardiovascular Protection

Abstract

OBJECTIVE: Pheochromocytomas and paragangliomas (PPGL) are relatively rare and mostly benign tumours. Approximately 10% of PPGL are malignant, as defined by the presence of metastases, i.e chromaffin tissue at a location that usually does not contain chromaffin cells. However, up to 35% of tumours in patients carrying an SDHB mutation appears to be malignant. Nowadays, no reliable marker allows to predict whether a PPGL is, or will become malignant. In addition, there are no curative treatments if metastases occur. The aim of the present study was to dentify genetic markers allowing to distinguish benign from malignant tumours. DESIGN AND METHOD: An mRNA expression array was performed on benign and malignant PPGL. The genes showing a different expression between the benign and malignant tumours were selected to be confirmed and validated by qRT-PCR. Finally, the remaining genes were stained by immunohistochemistry on Tissue MicroArray including a large series of PPGL. RESULTS: Forty benign and 12 malignant PPGL were investigated for differences in mRNA expression with Affymetrix arrays. Expression data were normalized according to Affymetrix recommendations. Then, using Pomelo II (http://pomelo2.bioinfo.cnio.es/), a Limma t-test was performed, to assess which genes were differentially expressed between benign and malignant PPGL. First, a non-clustered analysis was performed and 10 genes with a False Discovery Rate (FDR) below 0.05 and a relative overexpression ratio of at least 4 were found, including Interleukin 13 Receptor alpha 2 (IL13RA2) and Monooxygenase DBH-like 1 (MOXD1). Secondly, a supervised cluster analysis was performed (based on HIF target genes), resulting in 2 groups, which were both investigated for differences in mRNA expression between benign and malignant tumours. Five genes showed an FDR below 0.01 and were overexpressed in malignant tumours with a ratio higher than 4, including Contactin 4 (CNTN4), Iroquois Homeobox 3 (IRX3), and Sulfatase 2 (S

Published
2015

6. Immunohistochemical expression of stem cell markers in pheochromocytomas/paragangliomas is associated with SDHx mutations

Author

Pathologie patiënten zorg, Oudijk, L., Neuhofer, C. M., Lichtenauer, U. D., Papathomas, T. G., Korpershoek, E., Stoop, H., Oosterhuis, J. W., Smid, M., Restuccia, D. F., Robledo, M., De Cubas, A. A., Mannelli, M., Gimenez-Roqueplo, A. P., Dinjens, W. N M, Beuschlein, F., De Krijger, R. R., Pathologie patiënten zorg, Oudijk, L., Neuhofer, C. M., Lichtenauer, U. D., Papathomas, T. G., Korpershoek, E., Stoop, H., Oosterhuis, J. W., Smid, M., Restuccia, D. F., Robledo, M., De Cubas, A. A., Mannelli, M., Gimenez-Roqueplo, A. P., Dinjens, W. N M, Beuschlein, F., and De Krijger, R. R.

Published
2015

7. O10.05 * FINAL ANALYSIS OF THE BELOB TRIAL (A RANDOMIZED PHASE II STUDY ON BEVACIZUMAB VERSUS BEVACIZUMAB PLUS LOMUSTINE VERSUS LOMUSTINE SINGLE AGENT IN RECURRENT GLIOBLASTOMA) AND FIRST RADIOLOGY REVIEW RESULTS

Author

Taal, W., primary, Oosterkamp, H. M., additional, Walenkamp, A. M. E., additional, Dubbink, H. J., additional, Beerepoot, L. V., additional, Hanse, M., additional, Buter, J., additional, Honkoop, A., additional, Boerman, D., additional, Vos, F. Y. F., additional, Dinjens, W. N. M., additional, Enting, R. H., additional, Taphoorn, M. J. B., additional, van den Berkmortel, F. W. P. J., additional, Jansen, R., additional, Brandsma, D., additional, Bromberg, J. E., additional, van Heuvel, I., additional, Vernhout, R. M., additional, van der Holt, B., additional, and van den Bent, M. J., additional

Published
2014
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8. Molecular parameters associated with insulinoma progression : chromosomal instability versus p53 and CK19 status

Author

Jonkers, Y. M. H., Claessen, S. M. H., Veltman, J. A., Geurts van Kessel, A., Dinjens, W. N. M., Skogseid, Britt, Ramaekers, F. C. S., Speel, E-J. M., Jonkers, Y. M. H., Claessen, S. M. H., Veltman, J. A., Geurts van Kessel, A., Dinjens, W. N. M., Skogseid, Britt, Ramaekers, F. C. S., and Speel, E-J. M.

Abstract

Insulinomas represent the predominant syndromic subtype of endocrine pancreatic tumors (EPTs). Their metastatic potential cannot be predicted reliably using histopathological criteria. In the past few years, several attempts have been made to identify prognostic markers, among them TP53 mutations and immunostaining of p53 and recently cytokeratin 19 (CK19). In a previous study using conventional comparative genomic hybridization (CGH) we have shown that chromosomal instability (CIN) is associated with metastatic disease in insulinomas. It was our aim to evaluate these potential parameters in a single study. For the determination of CIN, we applied CGH to microarrays because it allows a high-resolution detection of DNA copy number changes in comparison with conventional CGH as well as the analysis of chromosomal regions close to the centromeres and telomeres, and at 1pter -> p32, 16p, 19 and 22. These regions are usually excluded from conventional CGH analysis, because they may show DNA gains in negative control hybridizations. Array CGH analysis of 30 insulinomas (15 tumors of benign, eight tumors of uncertain and seven tumors of malignant behavior) revealed that >= 20 chromosomal alterations and >= 6 telomeric losses were the best predictors of malignant progression. A subset of 22 insulinomas was further investigated for TP53 exon 5-8 gene mutations, and p53 and CK19 expression. Only one malignant tumor was shown to harbor an arginine 273 serine mutation and immunopositivity for p53. CK19 immunopositivity was detected in three malignant tumors and one tumor with uncertain behavior. In conclusion, our results indicate that CIN as well as telomeric loss are very powerful indicators for malignant progression in sporadic insulinomas. Our data do not support a critical role for p53 and CK19 as molecular parameters for this purpose.

Published
2006
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9. Tumours with loss of MSH6 expression are MSI-H when screened with a pentaplex of five mononucleotide repeats

Author

You, J-F, primary, Buhard, O, additional, Ligtenberg, M J L, additional, Kets, C M, additional, Niessen, R C, additional, Hofstra, R M W, additional, Wagner, A, additional, Dinjens, W N M, additional, Colas, C, additional, Lascols, O, additional, Collura, A, additional, Flejou, J-F, additional, Duval, A, additional, and Hamelin, R, additional

Published
2010
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16. Frequent loss of the AXIN1 locus but absence of AXIN1 gene mutations in adenocarcinomas of the gastro-oesophageal junction with nuclear ß-catenin expression.

Author

Koppert, L. B., van der Velden, A. W., van de Wetering, M., Abbou, M., van den Ouweland, A. M. W., Tilanus, H. W., Wijnhoven, B. P. L., and Dinjens, W. N. M.

Subjects
GENETIC transcription, ESOPHAGEAL cancer, ESOPHAGOGASTRIC junction, GENE expression, ADENOCARCINOMA, GENETIC mutation
Abstract

Up to 60% of gastro-oesophageal junction (GEJ) adenocarcinomas show nuclear ß-catenin expression, pointing to activated T-cell factor (TCF)/ß-catenin-driven gene transcription. We demonstrate in five human GEJ adenocarcinoma cell lines that nuclear ß-catenin expression indeed correlates with enhanced TCF-mediated transcription of a reporter gene. In several tumour types, TCF/ß-catenin activation is caused by mutations in either adenomatous polyposis coli (APC), ß-catenin exon 3, AXIN1, AXIN2 or ß-transducin repeat-containing protein (ß-TrCP). In GEJ adenocarcinomas, very few APC and ß-catenin mutations have been found. Therefore, the mechanism of Wnt pathway activation remains unclear. In the present study, we did not find AXIN1 gene mutations in 17 GEJ tumours with nuclear ß-catenin expression (without ß-catenin exon 3 mutations). Six intragenic single nucleotide polymorphisms (SNPs) were identified. One of these, the AXIN1 gene T1942C SNP, has a frequency of 21% but is only very recently described despite numerous AXIN1 gene mutational studies. We provide evidence why this SNP was missed in single strand conformation polymorphism analyses. The AXIN1 gene G2063A variation was previously described as a gene mutation but we demonstrate that this is a polymorphism. With these six SNPs loss of heterozygosity (LOH) was found in 11 of 15 (73%) informative tumours. To investigate a possible AXIN1 gene dosage effect in GEJ tumours expressing nuclear ß-catenin, AXIN1 locus LOH was determined in 20 tumours expressing membranous and no nuclear ß-catenin. LOH was found in 10 of 13 (77%) informative cases. AXIN1 protein immunohistochemistry revealed cytoplasmic expression in all tumours irrespective of the presence of AXIN1 locus LOH. These data indicate that nuclear ß-catenin expression is indicative for activated Wnt signalling and that neither AXIN1 gene mutations nor AXIN1 locus LOH are involved in Wnt pathway activation in GEJ adenocarcinomas.British Journal of Cancer (2004) 90, 892-899. doi:10.1038/sj.bjc.6601589 www.bjcancer.com [ABSTRACT FROM AUTHOR]

Published
2004
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17. The CHEK2*1100delC mutation has no major contribution in oesophageal carcinogenesis.

Author

Koppert, L. B., Schutte, M., Abbou, M., Tilanus, H. W., and Dinjens, W. N. M.

Subjects
GENETIC mutation, CARCINOGENESIS, ESOPHAGEAL cancer, ADENOCARCINOMA, SQUAMOUS cell carcinoma, DNA damage, CELL cycle
Abstract

In response to DNA damage, the cell cycle checkpoint kinase 2 (CHEK2) may phosphorylate p53, Cdc25A and Cdc25C, and regulate BRCA1 function, leading to cell cycle arrest and DNA repair. The truncating germline mutation CHEK2*1100delC abrogates kinase activity and confers low-penetrance susceptibility to breast cancer. We found CHEK2*1100delC in 0.5% of 190 oesophageal squamous cell carcinomas and in 1.5% of 196 oesophageal adenocarcinomas. In addition, we observed the mutation in 3.0% of 99 Barrett's metaplasias and 1.5% of 66 dysplastic Barrett's epithelia, both known precursor lesions of oesophageal adenocarcinoma. Since CHEK2*1100delC mutation frequencies did not significantly differ among oesophageal squamous cell carcinomas, adenocarcinomas and (dysplastic) Barrett's epithelia, as compared to healthy individuals, we conclude that the CHEK2*1100delC mutation has no major contribution in oesophageal carcinogenesis.British Journal of Cancer (2004) 90, 888-891. doi:10.1038/sj.bjc.6601551 www.bjcancer.com [ABSTRACT FROM AUTHOR]

Published
2004
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18. Human oesophageal adenocarcinoma cell lines JROECL 47 and JROECL 50 are admixtures of the human colon carcinoma cell line HCT 116.

Author

Wijnhoven, B P L, Tilanus, M G J, Morris, A G, Darnton, S J, Tilanus, H W, and Dinjens, W N M

Subjects
ADENOCARCINOMA, ESOPHAGUS, COLON (Anatomy), CELL lines
Abstract

In two recently described human oesophageal adenocarcinoma cell lines JROECL 47 and JROECL 50, derived from one tumour, we detected identical E-cadherin and β-catenin gene mutations as in colon carcinoma cell line HCT 116. We demonstrate by HLA-typing, mutation analysis and microsatellite analysis that cell lines JROECL 47 and JROECL 50 are admixtures of the human colon adenocarcinoma cell line HCT 116. [ABSTRACT FROM AUTHOR]

Published
2000

19. PTEN in colorectal cancer: a report on two Cowden syndrome patients.

Author

Kersseboom R, Dubbink HJ, Corver WE, van Tilburg AJ, Poley JW, van Leerdam ME, Atmodimedjo PN, van de Laar IM, Collée JM, Dinjens WN, Morreau H, and Wagner A

Subjects
Adult, Colorectal Neoplasms genetics, Colorectal Neoplasms pathology, Female, Follow-Up Studies, Germ-Line Mutation, Hamartoma Syndrome, Multiple pathology, Heterozygote, Humans, Loss of Heterozygosity, Male, Prospective Studies, Hamartoma Syndrome, Multiple genetics, PTEN Phosphohydrolase genetics
Abstract

Heterozygous germline PTEN mutations cause Cowden syndrome. The risk of colorectal cancer in Cowden patients, however, remains a matter of debate. We describe two patients presenting with colorectal cancer at a young age (28 and 39 years) and dysmorphisms fitting the Cowden spectrum. Heterozygous germline mutations in PTEN were found in both patients. Moreover, analysis of the resected colorectal cancer specimens revealed loss of heterozygosity at the PTEN locus with retention of the mutated alleles, and greatly reduced or absent PTEN expression. Histologically and molecularly, the tumours showed resemblance with sporadic colorectal cancers, although they had prominent fibrotic stroma. Our data indicate that PTEN loss was involved in carcinogenesis in the two patients, supporting that colorectal cancer is part of the Cowden syndrome-spectrum. This is in line with data on sporadic colorectal cancer, mice studies and emerging epidemiological data on Cowden syndrome. Although the exact role of germline PTEN mutations in the carcinogenesis of colorectal cancer remains unclear, we think that Cowden syndrome should be in the differential diagnosis of colorectal cancer certainly in view of the possible prognostic and therapeutic consequences. Prospective follow-up and surveillance of PTEN mutation carriers from the age of 25 to 30 years in a study setting should clarify this issue., (© 2011 John Wiley & Sons A/S.)

Published
2012
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20. Pitfalls in molecular analysis for mismatch repair deficiency in a family with biallelic pms2 germline mutations.

Author

Leenen CH, Geurts-Giele WR, Dubbink HJ, Reddingius R, van den Ouweland AM, Tops CM, van de Klift HM, Kuipers EJ, van Leerdam ME, Dinjens WN, and Wagner A

Subjects
Adult, Aged, 80 and over, Brain Neoplasms diagnosis, Brain Neoplasms genetics, Brain Neoplasms pathology, Child, DNA Mismatch Repair, DNA Repair-Deficiency Disorders genetics, Female, Genetic Testing, Heterozygote, Humans, Immunohistochemistry, Male, Microsatellite Instability, Middle Aged, Mismatch Repair Endonuclease PMS2, MutS Homolog 2 Protein genetics, Neoplastic Syndromes, Hereditary diagnosis, Neoplastic Syndromes, Hereditary genetics, Pedigree, Adenosine Triphosphatases genetics, DNA Repair Enzymes genetics, DNA-Binding Proteins genetics, Gene Expression Regulation, Neoplastic, Germ-Line Mutation
Abstract

Heterozygous germline mutations in the mismatch repair (MMR) genes MLH1, MSH2, MSH6 and PMS2 cause Lynch syndrome. Biallelic mutations in the MMR genes are associated with a childhood cancer syndrome [constitutional mismatch repair deficiency (CMMR-D)]. This is predominantly characterized by hematological malignancies and tumors of the bowel and brain, often associated with signs of neurofibromatosis type 1 (NF1). Diagnostic strategies for selection of patients for MMR gene analysis include analysis of microsatellite instability (MSI) and immunohistochemical (IHC) analysis of MMR proteins in tumor tissue. We report the clinical characterization and molecular analyses of tumor specimens from a family with biallelic PMS2 germline mutations. This illustrates the pitfalls of present molecular screening strategies. Tumor tissues of five family members were analyzed for MSI and IHC. MSI was observed in only one of the analyzed tissues. However, IHC analysis of brain tumor tissue of the index patient and his sister showed absence of PMS2 expression, and germline mutation analyses showed biallelic mutations in PMS2: p.Ser46IIe and p.Pro246fs. The same heterozygous mutations were confirmed in the father and mother, respectively. These data support the conclusion that in case of a clinical phenotype of CMMR-D, it is advisable to routinely combine MSI analysis with IHC analysis for the expression of MMR proteins. With inconclusive or conflicting results, germline mutation analysis of the MMR genes should be considered after thorough counselling of the patients and/or their relatives., (© 2011 John Wiley & Sons A/S.)

Published
2011
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21. Biochemical analysis and subcellular distribution of E-cadherin-catenin in adenocarcinomas of the gastro-oesophageal junction.

Author

Wijnhoven BP, Tucker ET, Dinjens WN, Tilanus HW, and Pignatelli M

Subjects
Adult, Aged, Blotting, Western, Cadherins biosynthesis, Cardia, Cytoskeletal Proteins biosynthesis, Female, Humans, Immunohistochemistry, Male, Middle Aged, Subcellular Fractions metabolism, Trans-Activators biosynthesis, alpha Catenin, beta Catenin, Adenocarcinoma metabolism, Cadherins metabolism, Cytoskeletal Proteins metabolism, Esophageal Neoplasms metabolism, Esophagogastric Junction, Stomach Neoplasms metabolism, Trans-Activators metabolism
Abstract

Background: Disturbances in the expression or structure of E-cadherin-catenin, a cell-cell adhesion complex, perturb its cell adhesive function., Materials and Methods: We studied the expression and distribution of the E-cadherin-catenin complex in 24 adenocarcinomas of the gastro-oesophageal junction (GOJ) by immunohistochemistry and Western blotting of the Triton X-100-soluble (membrane bound) and insoluble fractions (cytoskeleton bound)., Results: Immunohistochemistry demonstrated redistribution of E-cadherin, alpha-, beta- and gamma-catenin from the membrane to the cytoplasm in 13/24 (54%), 18/24 (75%), 16/24 (67%) and 15/24 (63%) tumours, respectively. Five tumours showed nuclear localisation of beta-catenin. Western blotting showed redistribution between the TX-100 soluble and insoluble fraction of E-cadherin and the catenins in 5/11 (45%), 4/10 (40%), 5/11 (45%) and 5/11 (45%) tumours, respectively., Conclusion: Loss of membrane bound E-cadherin-catenin is frequently observed in adenocarcinomas of the GOJ and this may reflect loss of function of the E-cadherin-catenin complex in these cancers.

Published
2004

22. Frequent loss of the AXIN1 locus but absence of AXIN1 gene mutations in adenocarcinomas of the gastro-oesophageal junction with nuclear beta-catenin expression.

Author

Koppert LB, van der Velden AW, van de Wetering M, Abbou M, van den Ouweland AM, Tilanus HW, Wijnhoven BP, and Dinjens WN

Subjects
Adenocarcinoma physiopathology, Axin Protein, Cadherins, DNA Mutational Analysis, Esophageal Neoplasms physiopathology, Humans, Immunohistochemistry, Loss of Heterozygosity, Protein-Tyrosine Kinases pharmacology, Proto-Oncogene Proteins pharmacology, Repressor Proteins biosynthesis, Signal Transduction, Stomach Neoplasms physiopathology, Tumor Cells, Cultured, Wnt Proteins, beta Catenin, Adenocarcinoma genetics, Cytoskeletal Proteins biosynthesis, Esophageal Neoplasms genetics, Gene Dosage, Repressor Proteins genetics, Stomach Neoplasms genetics, Trans-Activators biosynthesis, Zebrafish Proteins
Abstract

Up to 60% of gastro-oesophageal junction (GEJ) adenocarcinomas show nuclear beta-catenin expression, pointing to activated T-cell factor (TCF)/beta-catenin-driven gene transcription. We demonstrate in five human GEJ adenocarcinoma cell lines that nuclear beta-catenin expression indeed correlates with enhanced TCF-mediated transcription of a reporter gene. In several tumour types, TCF/beta-catenin activation is caused by mutations in either adenomatous polyposis coli (APC), beta-catenin exon 3, AXIN1, AXIN2 or beta-transducin repeat-containing protein (beta-TrCP). In GEJ adenocarcinomas, very few APC and beta-catenin mutations have been found. Therefore, the mechanism of Wnt pathway activation remains unclear. In the present study, we did not find AXIN1 gene mutations in 17 GEJ tumours with nuclear beta-catenin expression (without beta-catenin exon 3 mutations). Six intragenic single nucleotide polymorphisms (SNPs) were identified. One of these, the AXIN1 gene T1942C SNP, has a frequency of 21% but is only very recently described despite numerous AXIN1 gene mutational studies. We provide evidence why this SNP was missed in single strand conformation polymorphism analyses. The AXIN1 gene G2063A variation was previously described as a gene mutation but we demonstrate that this is a polymorphism. With these six SNPs loss of heterozygosity (LOH) was found in 11 of 15 (73%) informative tumours. To investigate a possible AXIN1 gene dosage effect in GEJ tumours expressing nuclear beta-catenin, AXIN1 locus LOH was determined in 20 tumours expressing membranous and no nuclear beta-catenin. LOH was found in 10 of 13 (77%) informative cases. AXIN1 protein immunohistochemistry revealed cytoplasmic expression in all tumours irrespective of the presence of AXIN1 locus LOH. These data indicate that nuclear beta-catenin expression is indicative for activated Wnt signalling and that neither AXIN1 gene mutations nor AXIN1 locus LOH are involved in Wnt pathway activation in GEJ adenocarcinomas.

Published
2004
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