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2. Genome-wide Association Study of Bladder Cancer Reveals New Biological and Translational Insights

Author

Koutros, S, Kiemeney, LA, Choudhury, PP, Milne, RL, de Maturana, EL, Ye, Y, Joseph, V, Florez-Vargas, O, Dyrskjot, L, Figueroa, J, Dutta, D, Giles, GG, Hildebrandt, MAT, Offit, K, Kogevinas, M, Weiderpass, E, McCullough, ML, Freedman, ND, Albanes, D, Kooperberg, C, Cortessis, VK, Karagas, MR, Johnson, A, Schwenn, MR, Baris, D, Furberg, H, Bajorin, DF, Cussenot, O, Cancel-Tassin, G, Benhamou, S, Kraft, P, Porru, S, Carta, A, Bishop, T, Southey, MC, Matullo, G, Fletcher, T, Kumar, R, Taylor, JA, Lamy, P, Prip, F, Kalisz, M, Weinstein, SJ, Hengstler, JG, Selinski, S, Harland, M, Teo, M, Kiltie, AE, Tardon, A, Serra, C, Carrato, A, Garcia-Closas, R, Lloreta, J, Schned, A, Lenz, P, Riboli, E, Brennan, P, Tjonneland, A, Otto, T, Ovsiannikov, D, Volkert, F, Vermeulen, SH, Aben, KK, Galesloot, TE, Turman, C, De Vivo, I, Giovannucci, E, Hunter, DJ, Hohensee, C, Hunt, R, V. Patel, A, Huang, W-Y, Thorleifsson, G, Gago-Dominguez, M, Amiano, P, Golka, K, Stern, MC, Yan, W, Liu, J, Alfred, S, Katta, S, Hutchinson, A, Hicks, B, Wheeler, WA, Purdue, MP, McGlynn, KA, Kitahara, CM, Haiman, CA, Greene, MH, Rafnar, T, Chatterjee, N, Chanock, SJ, Wu, X, Real, FX, Silverman, DT, Garcia-Closas, M, Stefansson, K, Prokunina-Olsson, L, Malats, N, Rothman, N, Koutros, S, Kiemeney, LA, Choudhury, PP, Milne, RL, de Maturana, EL, Ye, Y, Joseph, V, Florez-Vargas, O, Dyrskjot, L, Figueroa, J, Dutta, D, Giles, GG, Hildebrandt, MAT, Offit, K, Kogevinas, M, Weiderpass, E, McCullough, ML, Freedman, ND, Albanes, D, Kooperberg, C, Cortessis, VK, Karagas, MR, Johnson, A, Schwenn, MR, Baris, D, Furberg, H, Bajorin, DF, Cussenot, O, Cancel-Tassin, G, Benhamou, S, Kraft, P, Porru, S, Carta, A, Bishop, T, Southey, MC, Matullo, G, Fletcher, T, Kumar, R, Taylor, JA, Lamy, P, Prip, F, Kalisz, M, Weinstein, SJ, Hengstler, JG, Selinski, S, Harland, M, Teo, M, Kiltie, AE, Tardon, A, Serra, C, Carrato, A, Garcia-Closas, R, Lloreta, J, Schned, A, Lenz, P, Riboli, E, Brennan, P, Tjonneland, A, Otto, T, Ovsiannikov, D, Volkert, F, Vermeulen, SH, Aben, KK, Galesloot, TE, Turman, C, De Vivo, I, Giovannucci, E, Hunter, DJ, Hohensee, C, Hunt, R, V. Patel, A, Huang, W-Y, Thorleifsson, G, Gago-Dominguez, M, Amiano, P, Golka, K, Stern, MC, Yan, W, Liu, J, Alfred, S, Katta, S, Hutchinson, A, Hicks, B, Wheeler, WA, Purdue, MP, McGlynn, KA, Kitahara, CM, Haiman, CA, Greene, MH, Rafnar, T, Chatterjee, N, Chanock, SJ, Wu, X, Real, FX, Silverman, DT, Garcia-Closas, M, Stefansson, K, Prokunina-Olsson, L, Malats, N, and Rothman, N

Abstract

BACKGROUND: Genomic regions identified by genome-wide association studies (GWAS) for bladder cancer risk provide new insights into etiology. OBJECTIVE: To identify new susceptibility variants for bladder cancer in a meta-analysis of new and existing genome-wide genotype data. DESIGN, SETTING, AND PARTICIPANTS: Data from 32 studies that includes 13,790 bladder cancer cases and 343,502 controls of European ancestry were used for meta-analysis. OUTCOME MEASUREMENTS AND STATISTICAL ANALYSES: Log-additive associations of genetic variants were assessed using logistic regression models. A fixed-effects model was used for meta-analysis of the results. Stratified analyses were conducted to evaluate effect modification by sex and smoking status. A polygenic risk score (PRS) was generated on the basis of known and novel susceptibility variants and tested for interaction with smoking. RESULTS AND LIMITATIONS: Multiple novel bladder cancer susceptibility loci (6p.22.3, 7q36.3, 8q21.13, 9p21.3, 10q22.1, 19q13.33) as well as improved signals in three known regions (4p16.3, 5p15.33, 11p15.5) were identified, bringing the number of independent markers at genome-wide significance (p < 5 × 10-8) to 24. The 4p16.3 (FGFR3/TACC3) locus was associated with a stronger risk for women than for men (p-interaction = 0.002). Bladder cancer risk was increased by interactions between smoking status and genetic variants at 8p22 (NAT2; multiplicative p value for interaction [pM-I] = 0.004), 8q21.13 (PAG1; pM-I = 0.01), and 9p21.3 (LOC107987026/MTAP/CDKN2A; pM-I = 0.02). The PRS based on the 24 independent GWAS markers (odds ratio per standard deviation increase 1.49, 95% confidence interval 1.44-1.53), which also showed comparable results in two prospective cohorts (UK Biobank, PLCO trial), revealed an approximately fourfold difference in the lifetime risk of bladder cancer according to the PRS (e.g., 1st vs 10th decile) for both smokers and nonsmokers. CONCLUSIONS: We report novel loci associated

Published
2023

4. 1960O Identification of bladder cancer patients that could benefit from early post-cystectomy immunotherapy based on serial circulating tumour DNA (ctDNA) testing: Preliminary results from the TOMBOLA trial

Author

Bjerggaard Jensen, J., Birkenkamp-Demtröder, K., Nordentoft, I., Milling, R.V., Körner, S.K., Brandt, S.B., Knudsen, M., Lam, G.W., Dohn, L.H., Fabrin, K., Carus, A., Petersen, A., Joensen, U.N., Pappot, H., Holt, P.S., Jensen, N.V., Agerbæk, M., and Dyrskjot, L.

Published
2024
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5. Re: An Integrated Multi-Omics Analysis Identifies Prognostic Molecular Subtypes of Non-Muscle Invasive Bladder Cancer : Editorial Comment

Author

Lindskrog, S. , V, Prip, F., Lamy, P., Taber, A., Groeneveld, C. S., Birkenkamp-Demtroder, K., Jensen, J. B., Strandgaard, T., Nordentoft, I, Christensen, E., Sokac, M., Birkbak, N. J., Maretty, L., Hermann, G. G., Petersen, A. C., Weyerer, V, Grimm, M-O, Horstmann, M., Sjodahl, G., Hoglund, M., Steiniche, T., Mogensen, K., de Reynies, A., Nawroth, R., Jordan, B., Lin, X., Dragicevic, D., Ward, D. G., Goel, A., Hurst, C. D., Raman, J. D., Warrick, J. , I, Segersten, Ulrika, Sikic, D., van Kessel, K. E. M., Maurer, T., Meeks, J. J., DeGraff, D. J., Bryan, R. T., Knowles, M. A., Simic, T., Hartmann, A., Zwarthoff, E. C., Malmstrom, P-O, Malats, N., Real, F. X., Dyrskjot, L., Lindskrog, S. , V, Prip, F., Lamy, P., Taber, A., Groeneveld, C. S., Birkenkamp-Demtroder, K., Jensen, J. B., Strandgaard, T., Nordentoft, I, Christensen, E., Sokac, M., Birkbak, N. J., Maretty, L., Hermann, G. G., Petersen, A. C., Weyerer, V, Grimm, M-O, Horstmann, M., Sjodahl, G., Hoglund, M., Steiniche, T., Mogensen, K., de Reynies, A., Nawroth, R., Jordan, B., Lin, X., Dragicevic, D., Ward, D. G., Goel, A., Hurst, C. D., Raman, J. D., Warrick, J. , I, Segersten, Ulrika, Sikic, D., van Kessel, K. E. M., Maurer, T., Meeks, J. J., DeGraff, D. J., Bryan, R. T., Knowles, M. A., Simic, T., Hartmann, A., Zwarthoff, E. C., Malmstrom, P-O, Malats, N., Real, F. X., and Dyrskjot, L.

Published
2022

13. The DNA damage checkpoint precedes activation of ARF in response to escalating oncogenic stress during tumorigenesis

Author

Evangelou, K. Bartkova, J. Kotsinas, A. Pateras, I.S. Liontos, M. Velimezi, G. Kosar, M. Liloglou, T. Trougakos, I.P. Dyrskjot, L. Andersen, C.L. Papaioannou, M. Drosos, Y. Papafotiou, G. Hodny, Z. Sosa-Pineda, B. Wu, X.-R. Klinakis, A. Ørntoft, T. Lukas, J. Bartek, J. Gorgoulis, V.G.

Subjects
body regions
Abstract

Oncogenic stimuli trigger the DNA damage response (DDR) and induction of the alternative reading frame (ARF) tumor suppressor, both of which can activate the p53 pathway and provide intrinsic barriers to tumor progression. However, the respective timeframes and signal thresholds for ARF induction and DDR activation during tumorigenesis remain elusive. Here, these issues were addressed by analyses of mouse models of urinary bladder, colon, pancreatic and skin premalignant and malignant lesions. Consistently, ARF expression occurred at a later stage of tumor progression than activation of the DDR or p16 INK4A, a tumor-suppressor gene overlapping with ARF. Analogous results were obtained in several human clinical settings, including early and progressive lesions of the urinary bladder, head and neck, skin and pancreas. Mechanistic analyses of epithelial and fibroblast cell models exposed to various oncogenes showed that the delayed upregulation of ARF reflected a requirement for a higher, transcriptionally based threshold of oncogenic stress, elicited by at least two oncogenic 'hits', compared with lower activation threshold for DDR. We propose that relative to DDR activation, ARF provides a complementary and delayed barrier to tumor development, responding to more robust stimuli of escalating oncogenic overload. © 2013 Macmillan Publishers Limited. All rights reserved.

Published
2013

15. Oncogene-induced senescence is part of the tumorigenesis barrier imposed by DNA damage checkpoints

Author

Bartkova, J., Rezaei, N., Liontos, M., Karakaidos, P., Kletsas, D., Issaeva, N., Vassiliou, L. V. F., Kolettas, E., Niforou, K., Zoumpourlis, Vassilis, Takaoka, M., Nakagawa, H., Tort, F., Fugger, K., Johansson, F., Sehested, M., Andersen, C. L., and Dyrskjot, L

Subjects
InformationSystems_INFORMATIONSTORAGEANDRETRIEVAL, ComputingMethodologies_DOCUMENTANDTEXTPROCESSING, GeneralLiterature_REFERENCE(e.g.,dictionaries,encyclopedias,glossaries)
Abstract

Journal URL: http://www.nature.com/nature/index.html

Published
2008

16. Oncogene-induced senescence is part of the tumorigenesis barrier imposed by DNA damage checkpoints

Author

Bartkova, J. Rezaei, N. Liontos, M. Karakaidos, P. Kletsas, D. Issaeva, N. Vassiliou, L.-V.F. Kolettas, E. Niforou, K. Zoumpourlis, V.C. Takaoka, M. Nakagawa, H. Tort, F. Fugger, K. Johansson, F. Sehested, M. Andersen, C.L. Dyrskjot, L. Ørntoft, T. Lukas, J. Kittas, C. Helleday, T. Halazonetis, T.D. Bartek, J. Gorgoulis, V.G.

Abstract

Recent studies have indicated the existence of tumorigenesis barriers that slow or inhibit the progression of preneoplastic lesions to neoplasia. One such barrier involves DNA replication stress, which leads to activation of the DNA damage checkpoint and thereby to apoptosis or cell cycle arrest, whereas a second barrier is mediated by oncogene-induced senescence. The relationship between these two barriers, if any, has not been elucidated. Here we show that oncogene-induced senescence is associated with signs of DNA replication stress, including prematurely terminated DNA replication forks and DNA double-strand breaks. Inhibiting the DNA double-strand break response kinase ataxia telangiectasia mutated (ATM) suppressed the induction of senescence and in a mouse model led to increased tumour size and invasiveness. Analysis of human precancerous lesions further indicated that DNA damage and senescence markers cosegregate closely. Thus, senescence in human preneoplastic lesions is a manifestation of oncogene-induced DNA replication stress and, together with apoptosis, provides a barrier to malignant progression. ©2006 Nature Publishing Group.

Published
2006

17. Telomerase reverse transcriptase promoter mutations in bladder cancer: High frequency across stages, detection in urine, and lack of association with outcome

Author

Allory, Y. (Yves), Beukers, W. (Willemien), Sagrera, A. (Ana), Flández, M. (Marta), Marqués, M. (Miriam), Márquez, M. (Mirari), Keur, K.A. (Kirstin) van der, Dyrskjot, L. (Lars), Lurkin, I. (Irene), Vermeij, M. (Marcel), Carrato, A. (Alfredo), Lloreta, J. (Josep), Lorente, J.A. (José), Carrillo-de Santa Pau, E. (Enrique), Masius, R.G. (Roy), Kogevinas, M. (Manolis), Steyerberg, E.W. (Ewout), Tilborg, A.A.G. (Angela) van, Abas, C.S. (Cheno), Orntoft, T.F. (Torben), Zuiverloon, T.C.M. (Tahlita), Malats, N. (Núria), Zwarthoff, E.C. (Ellen), Real, F.X. (Francisco), Allory, Y. (Yves), Beukers, W. (Willemien), Sagrera, A. (Ana), Flández, M. (Marta), Marqués, M. (Miriam), Márquez, M. (Mirari), Keur, K.A. (Kirstin) van der, Dyrskjot, L. (Lars), Lurkin, I. (Irene), Vermeij, M. (Marcel), Carrato, A. (Alfredo), Lloreta, J. (Josep), Lorente, J.A. (José), Carrillo-de Santa Pau, E. (Enrique), Masius, R.G. (Roy), Kogevinas, M. (Manolis), Steyerberg, E.W. (Ewout), Tilborg, A.A.G. (Angela) van, Abas, C.S. (Cheno), Orntoft, T.F. (Torben), Zuiverloon, T.C.M. (Tahlita), Malats, N. (Núria), Zwarthoff, E.C. (Ellen), and Real, F.X. (Francisco)

Abstract

Background Hotspot mutations in the promoter of the gene coding for telomerase reverse transcriptase (TERT) have been described and proposed to activate gene expression. Objectives To investigate TERT mutation frequency, spectrum, association with expression and clinical outcome, and potential for detection of recurrences in urine in patients with urothelial bladder cancer (UBC). De

Published
2014
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18. External validation of a multiplex urinary protein panel for the detection of bladder cancer in a multicenter cohort

Author

Chen, L.-M. (Li-Mei), Chang, M. (Myron), Dai, Y. (Yunfeng), Chai, K.X. (Karl X.), Dyrskjot, L. (Lars), Sanchez-Carbayo, M. (Marta), Szarvas, T. (Tibor), Zwarthoff, E.C. (Ellen), Lokeshwar, V. (Vinata), Jeronimo, C. (Carmen), Parker, A.S. (Alexander S.), Ross, S. (Shanti), Borre, M. (M.), Orntoft, T.F. (Torben), Jaeger, T. (Tobias), Beukers, W. (Willemien), Lopez, L.E. (Luis E.), Henrique, R. (Rui), Young, P.R. (Paul R.), Urquidi, V. (Virginia), Goodison, S. (Steve), Rosser, C.J. (Charles J.), Chen, L.-M. (Li-Mei), Chang, M. (Myron), Dai, Y. (Yunfeng), Chai, K.X. (Karl X.), Dyrskjot, L. (Lars), Sanchez-Carbayo, M. (Marta), Szarvas, T. (Tibor), Zwarthoff, E.C. (Ellen), Lokeshwar, V. (Vinata), Jeronimo, C. (Carmen), Parker, A.S. (Alexander S.), Ross, S. (Shanti), Borre, M. (M.), Orntoft, T.F. (Torben), Jaeger, T. (Tobias), Beukers, W. (Willemien), Lopez, L.E. (Luis E.), Henrique, R. (Rui), Young, P.R. (Paul R.), Urquidi, V. (Virginia), Goodison, S. (Steve), and Rosser, C.J. (Charles J.)

Abstract

Background: Because of the faltering sensitivity and/or specificity, urine-based assays currently have a limited role in the management of patients with bladder cancer. The aim of this study was to externally validate our previously reported protein biomarker panel from multiple sites in the United States and Europe.Methods: This multicenter external validation study included a total of 320 subjects (bladder cancer = 183). The 10 biomarkers (IL8, MMP9, MMP10, SERPINA1, VEGFA, ANG, CA9, APOE, SDC1, and SERPINE1) were measured using commercial ELISA assays in an external laboratory. The diagnostic performance of the biomarker panel was assessed using receiver operator curves (ROC) and descriptive statistical values.Results: Utilizing the combination of all 10 biomarkers, the area under the ROC for the diagnostic panel was noted to be 0.847 (95% confidence interval, 0.796-0.899), outperforming any single biomarker. The multiplex assay at optimal cutoff value achieved an overall sensitivity of 0.79, specificity of 0.79, positive prediction value of 0.73, and negative prediction value of 0.84 for bladder cancer classification. Sensitivity values of the diagnostic panel for high-grade bladder cancer, low-grade bladder cancer, muscle invasive bladder cancer, and non-muscle invasive bladder cancer were 0.81, 0.90, 0.95, and 0.77, respectively.Conclusions: Urinary levels of the biomarker panel enabled discrimination of patients with bladder cancer and controls, and the levels of biomarker subsets were associated with advancing tumor grade and stage.Impact: If proven to be reliable, urinary diagnostic biomarker assays can detect bladder cancer in a timely manner such that the patient can expect improvements in overall survival and quality of life.

Published
2014
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19. Risk prediction scores for recurrence and progression of non-muscle invasive bladder cancer

Author

Vedder, M.M. (Moniek), Márquez, M. (Mirari), Bekker-Grob, E.W. (Esther) de, Calle, M.L. (Malu), Dyrskjot, L. (Lars), Kogevinas, M. (Manolis), Segersten, U. (Ulrika), Malmström, P.-U. (Per-Uno), Algaba, F. (Ferran), Beukers, W. (Willemien), Orntoft, T.F. (Torben), Zwarthoff, E.C. (Ellen), Real, F.X. (Francisco), Malats, N. (Núria), Steyerberg, E.W. (Ewout), Vedder, M.M. (Moniek), Márquez, M. (Mirari), Bekker-Grob, E.W. (Esther) de, Calle, M.L. (Malu), Dyrskjot, L. (Lars), Kogevinas, M. (Manolis), Segersten, U. (Ulrika), Malmström, P.-U. (Per-Uno), Algaba, F. (Ferran), Beukers, W. (Willemien), Orntoft, T.F. (Torben), Zwarthoff, E.C. (Ellen), Real, F.X. (Francisco), Malats, N. (Núria), and Steyerberg, E.W. (Ewout)

Abstract

Objective: We aimed to determine the validity of two risk scores for patients with non-muscle invasive bladder cancer in different European settings, in patients with primary tumours. Methods: We included 1,892 patients with primary stage Ta or T1 non-muscle invasive bladder cancer who underwent a transurethral resection in Spain (n = 973), the Netherlands (n = 639), or Denmark (n = 280). We evaluated recurrence-free survival and progression-free survival according to the European Organisation for Research a

Published
2014
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20. Next-generation sequencing identifies germline MRE11A variants as markers of radiotherapy outcomes in muscle-invasive bladder cancer

Author

Teo, MTW, Dyrskjot, L, Nsengimana, J, Buchwald, C, Snowden, H, Morgan, J, Jensen, JB, Knowles, MA, Taylor, G, Barrett, JH, Borre, M, Orntoft, TF, Bishop, DT, Kiltie, AE, Teo, MTW, Dyrskjot, L, Nsengimana, J, Buchwald, C, Snowden, H, Morgan, J, Jensen, JB, Knowles, MA, Taylor, G, Barrett, JH, Borre, M, Orntoft, TF, Bishop, DT, and Kiltie, AE

Abstract

BACKGROUND: Muscle-invasive bladder cancer (MIBC) can be cured by radical radiotherapy (RT). We previously found tumour MRE11 expression to be predictive of survival following RT in MIBC, and this was independently validated in a separate institute. Here, we investigated germline MRE11A variants as possible predictors of RT outcomes in MIBC, using next-generation sequencing (NGS). PATIENTS AND METHODS: The MRE11A gene was amplified in germline DNA from 186 prospectively recruited MIBC patients treated with RT and sequenced using bar-coded multiplexed NGS. Germline variants were analysed for associations with cancer-specific survival (CSS). For validation as a prognostic or predictive marker, rs1805363 was then genotyped in a cystectomy-treated MIBC cohort of 256 individuals. MRE11A mRNA isoform expression was measured in bladder cancer cell lines and primary tumour samples. RESULTS: Carriage of at least one of six (five novel) rare variants was associated with the worse RT outcome (hazard ratio [HR] 4.04, 95% confidence interval [95% CI] 1.42-11.51, P = 0.009). The single-nucleotide polymorphism (SNP), rs1805363 (minor allele frequency 11%), was also associated with worse CSS (per-allele HR 2.10, 95% CI 1.34-3.28, Ptrend = 0.001) following RT in MIBC, with a gene-dosage effect observed, but no effect seen on CSS in the cystectomy cohort (Ptrend = 0.89). Furthermore, rs1805363 influenced relative MRE11A isoform expression, with increased isoform 2 expression with carriage of the rs1805363 minor A allele. CONCLUSIONS: Germline MRE11A SNP rs1805363 was predictive of RT, but not of cystectomy outcome in MIBC. If successfully validated in an independent RT-treated cohort, this SNP could be a useful clinical tool for selecting patients for bladder-conserving treatment.

Published
2014

21. Telomerase Reverse Transcriptase Promoter Mutations in Bladder Cancer: High Frequency Across Stages, Detection in Urine, and Lack of Association with Outcome

Author

Allory, Y, Beukers, Willemien, Sagrera, A, Flandez, M, Marques, M, Marquez, M, Keur, Kirstin, Dyrskjot, L, Lurkin, Irene, Vermeij, Marcel, Carrato, A, Lloreta, J, Lorente, JA, Pau, ECD, Masius, Roy, Kogevinas, M, Steyerberg, Ewout, van Tilborg, AAG, Abas, C, Orntoft, TF, Zuiverloon, Tahlita, Malats, N, Zwarthoff, Ellen, Real, FX, Allory, Y, Beukers, Willemien, Sagrera, A, Flandez, M, Marques, M, Marquez, M, Keur, Kirstin, Dyrskjot, L, Lurkin, Irene, Vermeij, Marcel, Carrato, A, Lloreta, J, Lorente, JA, Pau, ECD, Masius, Roy, Kogevinas, M, Steyerberg, Ewout, van Tilborg, AAG, Abas, C, Orntoft, TF, Zuiverloon, Tahlita, Malats, N, Zwarthoff, Ellen, and Real, FX

Abstract

Background: Hotspot mutations in the promoter of the gene coding for telomerase reverse transcriptase (TERT) have been described and proposed to activate gene expression. Objectives: To investigate TERT mutation frequency, spectrum, association with expression and clinical outcome, and potential for detection of recurrences in urine in patients with urothelial bladder cancer (UBC). Design, setting, and participants: A set of 111 UBCs of different stages was used to assess TERT promoter mutations by Sanger sequencing and TERT messenger RNA (mRNA) expression by reverse transcription-quantitative polymerase chain reaction. The two most frequent mutations were investigated, using a SNaPshot assay, in an independent set of 184 non-muscle-invasive and 173 muscle-invasive UBC (median follow-up: 53 mo and 21 mo, respectively). Voided urine from patients with suspicion of incident UBC (n = 174), or under surveillance after diagnosis of non-muscle-invasive UBC (n = 194), was tested using a SNaPshot assay. Outcome measurements and statistical analysis: Association of mutation status with age, sex, tobacco, stage, grade, fibroblast growth factor receptor 3 (FGFR3) mutation, progression-free survival, disease-specific survival, and overall survival. Results and limitations: In the two series, 78 of 111 (70%) and 283 of 357 (79%) tumors harbored TERT mutations, C228T being the most frequent substitution (83% for both series). TERT mutations were not associated with clinical or pathologic parameters, but were more frequent among FGFR3 mutant tumors (p = 0.0002). There was no association between TERT mutations and mRNA expression (p = 0.3). Mutations were not associated with clinical outcome. In urine, TERT mutations had 90% specificity in subjects with hematuria but no bladder tumor, and 73% in recurrence-free UBC patients. The sensitivity was 62% in incident and 42% in recurrent UBC. A limitation of the study is its retrospective nature. Conclusions: Somatic TERT promoter mutatio

Published
2014

22. Risk Prediction Scores for Recurrence and Progression of Non-Muscle Invasive Bladder Cancer: An International Validation in Primary Tumours

Author

Vedder, Moniek, Marquez, M, de Bekker - Grob, Esther, Calle, ML, Dyrskjot, L, Kogevinas, M, Segersten, U, Malmstrom, PU, Algaba, F, Beukers, Willemien, Orntoft, TF, Zwarthoff, Ellen, Real, FX, Malats, N, Steyerberg, Ewout, Vedder, Moniek, Marquez, M, de Bekker - Grob, Esther, Calle, ML, Dyrskjot, L, Kogevinas, M, Segersten, U, Malmstrom, PU, Algaba, F, Beukers, Willemien, Orntoft, TF, Zwarthoff, Ellen, Real, FX, Malats, N, and Steyerberg, Ewout

Abstract

Objective: We aimed to determine the validity of two risk scores for patients with non-muscle invasive bladder cancer in different European settings, in patients with primary tumours. Methods: We included 1,892 patients with primary stage Ta or T1 non-muscle invasive bladder cancer who underwent a transurethral resection in Spain (n = 973), the Netherlands (n = 639), or Denmark (n = 280). We evaluated recurrence-free survival and progression-free survival according to the European Organisation for Research and Treatment of Cancer (EORTC) and the Spanish Urological Club for Oncological Treatment (CUETO) risk scores for each patient and used the concordance index (c-index) to indicate discriminative ability. Results: The 3 cohorts were comparable according to age and sex, but patients from Denmark had a larger proportion of patients with the high stage and grade at diagnosis (p < 0.01). At least one recurrence occurred in 839 (44%) patients and 258 (14%) patients had a progression during a median follow-up of 74 months. Patients from Denmark had the highest 10-year recurrence and progression rates (75% and 24%, respectively), whereas patients from Spain had the lowest rates (34% and 10%, respectively). The EORTC and CUETO risk scores both predicted progression better than recurrence with c-indices ranging from 0.72 to 0.82 while for recurrence, those ranged from 0.55 to 0.61. Conclusion: The EORTC and CUETO risk scores can reasonably predict progression, while prediction of recurrence is more difficult. New prognostic markers are needed to better predict recurrence of tumours in primary non-muscle invasive bladder cancer patients.

Published
2014

23. 380 - Prognostic impact of a 12-gene progression score in non-muscle invasive bladder cancer: A prospective multicenter validation study

Author

Dyrskjøt, L., Reinert, T., Algaba, F., Christensen, E., Nieboer, D., Hermann, G., Morgensen, K., Marquez, M., Segersten, U., Hoyer, S., Ulhøj, B., Hartmann, A., Stöhr, R., Wach, S., Nawroth, R., Beukers, W., Schwamborn, K., Tulic, C., Simic, T., Junker, K., Harving, N., Petersen, A.C., Jensen, J.B., Keck, B., Horstmann, M., Maurer, T., Steyerberg, E., Zwarthoff, E., Real, F., Malats, N., Malmström, P.-U., and Ørntoft, T.F.

Published
2017
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24. The Use of Molecular Analyses in Voided Urine for the Assessment of Patients with Hematuria

Author

Beukers, W. (Willemien), Kandimalla, R. (Raju), Houwelingen, D. (Diandra) van, Kovacic, H. (Hrvoje), Chin, J.-F.D. (Jie-Fen), Lingsma, H.F. (Hester), Dyrskjot, L. (Lars), Zwarthoff, E.C. (Ellen), Beukers, W. (Willemien), Kandimalla, R. (Raju), Houwelingen, D. (Diandra) van, Kovacic, H. (Hrvoje), Chin, J.-F.D. (Jie-Fen), Lingsma, H.F. (Hester), Dyrskjot, L. (Lars), and Zwarthoff, E.C. (Ellen)

Abstract

Introduction:Patients presenting with painless hematuria form a large part of the urological patient population. In many cases, especially in younger patients, the cause of hematuria is harmless. Nonetheless, hematuria could be a symptom of malignant disease and hence most patients will be subject to cystoscopy. In this study, we aimed to develop a prediction model based on methylation markers in combination with clinical variables, in order to stratify patients with high risk for bladder cancer.Material and Methods:Patients (n=169) presenting with painless hematuria were included. 54 patients were diagnosed with bladder cancer. In the remaining 115 patients, the cause of hematuria was non-malignant. Urine samples were collected prior to cystoscopy. Urine DNA was analyzed for methylation of OSR1, SIM2, OTX1, MEIS1 and ONECUT2. Methylation percentages were calculated and were combined with clinical variables into a logistic regression model.Results:Logistic regression analysis based on the five methylation markers, age, gender and type of hematuria resulted in an area under the curve (AUC) of 0.88 and an optimism corrected AUC of 0.84 after internal validation by bootstrapping. Using a cut-off value of 0.307 allowed stratification of patients in a low-risk and high-risk group, resulting in a sensitivity of 82% (44/54) and a specificity of 82% (94/115). Most aggressive tumors were found in patients in the high-risk group. The addition of cytology to the prediction model, improved the AUC from 0.88 to 0.89, with a sensitivity and specificity of 85% (39/46) and 87% (80/92), retrospectively.Conclusions:This newly developed prediction model could be a helpful tool in risk stratification of patients presenting with painless hematuria. Accurate risk prediction might result in less extensive examination of low risk patients and thereby, reducing patient burden and costs. Further validation in a large prospective patient cohort is necessary to prove the true clinical value of

Published
2013
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25. The DNA damage checkpoint precedes activation of ARF in response to escalating oncogenic stress during tumorigenesis

Author

Evangelou, K., Bartkova, J., Kotsinas, A., Pateras, I.S., Liontos, M., Velimezi, G., Kosar, M., Liloglou, T., Trougakos, I.P., Dyrskjot, L., Andersen, C.L., Papaioannou, M., Drosos, Y., Papafotiou, G., Hodny, Z., Sosa-Pineda, B., Wu, X.-R., Klinakis, A., Ørntoft, Torben Falck, Lukas, J., Bartek, J., Gorgoulis, V.G., Evangelou, K., Bartkova, J., Kotsinas, A., Pateras, I.S., Liontos, M., Velimezi, G., Kosar, M., Liloglou, T., Trougakos, I.P., Dyrskjot, L., Andersen, C.L., Papaioannou, M., Drosos, Y., Papafotiou, G., Hodny, Z., Sosa-Pineda, B., Wu, X.-R., Klinakis, A., Ørntoft, Torben Falck, Lukas, J., Bartek, J., and Gorgoulis, V.G.

Abstract

Oncogenic stimuli trigger the DNA damage response (DDR) and induction of the alternative reading frame (ARF) tumor suppressor, both of which can activate the p53 pathway and provide intrinsic barriers to tumor progression. However, the respective timeframes and signal thresholds for ARF induction and DDR activation during tumorigenesis remain elusive. Here, these issues were addressed by analyses of mouse models of urinary bladder, colon, pancreatic and skin premalignant and malignant lesions. Consistently, ARF expression occurred at a later stage of tumor progression than activation of the DDR or p16 , a tumor-suppressor gene overlapping with ARF. Analogous results were obtained in several human clinical settings, including early and progressive lesions of the urinary bladder, head and neck, skin and pancreas. Mechanistic analyses of epithelial and fibroblast cell models exposed to various oncogenes showed that the delayed upregulation of ARF reflected a requirement for a higher, transcriptionally based threshold of oncogenic stress, elicited by at least two oncogenic 'hits', compared with lower activation threshold for DDR. We propose that relative to DDR activation, ARF provides a complementary and delayed barrier to tumor development, responding to more robust stimuli of escalating oncogenic overload.

Published
2013

26. The Use of Molecular Analyses in Voided Urine for the Assessment of Patients with Hematuria

Author

Beukers, Willemien, Kandimalla, Raju, van Houwelingen, D, Kovacic, H, Chin, JF (Jie-Fen), Lingsma, Hester, Dyrskjot, L, Zwarthoff, Ellen, Beukers, Willemien, Kandimalla, Raju, van Houwelingen, D, Kovacic, H, Chin, JF (Jie-Fen), Lingsma, Hester, Dyrskjot, L, and Zwarthoff, Ellen

Abstract

Introduction: Patients presenting with painless hematuria form a large part of the urological patient population. In many cases, especially in younger patients, the cause of hematuria is harmless. Nonetheless, hematuria could be a symptom of malignant disease and hence most patients will be subject to cystoscopy. In this study, we aimed to develop a prediction model based on methylation markers in combination with clinical variables, in order to stratify patients with high risk for bladder cancer. Material and Methods: Patients (n=169) presenting with painless hematuria were included. 54 patients were diagnosed with bladder cancer. In the remaining 115 patients, the cause of hematuria was non-malignant. Urine samples were collected prior to cystoscopy. Urine DNA was analyzed for methylation of OSR1, SIM2, OTX1, MEIS1 and ONECUT2. Methylation percentages were calculated and were combined with clinical variables into a logistic regression model. Results: Logistic regression analysis based on the five methylation markers, age, gender and type of hematuria resulted in an area under the curve (AUC) of 0.88 and an optimism corrected AUC of 0.84 after internal validation by bootstrapping. Using a cut-off value of 0.307 allowed stratification of patients in a low-risk and high-risk group, resulting in a sensitivity of 82% (44/54) and a specificity of 82% (94/115). Most aggressive tumors were found in patients in the high-risk group. The addit Conclusions: This newly developed prediction model could be a helpful tool in risk stratification of patients presenting with painless hematuria. Accurate risk prediction might result in less extensive examination of low risk patients and thereby, reducing patient burden and costs. Further validation in a large prospective patient cohort is necessary to prove the true clinical value of this model.

Published
2013

27. Analysis of molecular intra-patient variation and delineation of a prognostic 12-gene signature in non-muscle invasive bladder cancer; technology transfer from microarrays to PCR

Author

Dyrskjot, L., Reinert, T., Novoradovsky, A., Zuiverloon, T. C. M., Beukers, W., Zwarthoff, E., Malats, N., Real, F. X., Segersten, Ulrika, Malmström, Per-Uno, Knowles, M., Hurst, C., Sorge, J., Borre, M., Orntoft, T. F., Dyrskjot, L., Reinert, T., Novoradovsky, A., Zuiverloon, T. C. M., Beukers, W., Zwarthoff, E., Malats, N., Real, F. X., Segersten, Ulrika, Malmström, Per-Uno, Knowles, M., Hurst, C., Sorge, J., Borre, M., and Orntoft, T. F.

Abstract

BACKGROUND: Multiple clinical risk factors and genetic profiles have been demonstrated to predict progression of non-muscle invasive bladder cancer; however, no easily clinical applicable gene signature has been developed to predict disease progression independent of disease stage and grade. METHODS: We measured the intra-patient variation of an 88-gene progression signature using 39 metachronous tumours from 17 patients. For delineation of the optimal quantitative reverse transcriptase PCR panel of markers, we used 115 tumour samples from patients in Denmark, Sweden, UK and Spain. RESULTS: Analysis of intra-patient variation of the molecular markers showed 71% similar classification results. A final panel of 12 genes was selected, showing significant correlation with outcome. In multivariate Cox regression analysis, we found that the 12-gene signature was an independent prognostic factor (hazard ratio = 7.4 (95% confidence interval: 3.4-15.9), P < 0.001) when adjusting for stage, grade and treatment. Independent validation of the 12-gene panel and the determined cut-off values is needed and ongoing. CONCLUSION: Intra-patient marker variation in metachronous tumours is present. Therefore, to increase test sensitivity, it may be necessary to test several metachronous tumours from a patient's disease course. A PCR-based 12-gene signature significantly predicts disease progression in patients with non-muscle invasive bladder cancer.

Published
2012
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28. Selection of microsatellite markers for bladder cancer diagnosis without the need for corresponding blood

Author

Tilborg, A.A.G. (Angela) van, Kompier, L.C. (Lucie), Lurkin, I. (Irene), Poort, R. (Ricardo), Bouazzaoui, S. (Samira) El, Keur, K.A. (Kirstin) van der, Zuiverloon, T.C.M. (Tahlita), Dyrskjot, L. (Lars), Orntoft, T.F. (Torben), Roobol-Bouts, M.J. (Monique), Zwarthoff, E.C. (Ellen), Tilborg, A.A.G. (Angela) van, Kompier, L.C. (Lucie), Lurkin, I. (Irene), Poort, R. (Ricardo), Bouazzaoui, S. (Samira) El, Keur, K.A. (Kirstin) van der, Zuiverloon, T.C.M. (Tahlita), Dyrskjot, L. (Lars), Orntoft, T.F. (Torben), Roobol-Bouts, M.J. (Monique), and Zwarthoff, E.C. (Ellen)

Abstract

Microsatellite markers are used for loss-of-heterozygosity, allelic imbalance and clonality analyses in cancers. Usually, tumor DNA is compared to corresponding normal DNA. However, normal DNA is not always available and can display aberrant allele ratios due to copy number variations in the genome. Moreover, stutter peaks may complicate the analysis. To use microsatellite markers for diagnosis of recurrent bladder cancer, we aimed to select markers without stutter peaks and a constant ratio between alleles, thereby avoiding the need for a control DNA sample. We investigated 49 microsatellite markers with tri- and tetranucleotide repeats in regions commonly lost in bladder cancer. Based on analysis of 50 blood DNAs the 12 best performing markers were selected with few stutter peaks and a constant ratio between peaks heights. Per marker upper and lower cut off values for allele ratios were determined. LOH of the markers was observed in 59/104 tumor DNAs. We then determined the sensitivity of the marker panel for detection of recurrent bladder cancer by assaying 102 urine samples of these patients. Sensitivity was 63% when patients were stratified for LOH in their primary tumors. We demonstrate that up-front selection of microsatellite markers obliterates the need for a corresponding blood sample. For diagnosis of bladder cancer recurrences in urine this significantly reduces costs. Moreover, this approach facilitates retrospective analysis of archival tumor samples for allelic imbalance.

Published
2012
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29. Selection of microsatellite markers for bladder cancer diagnosis without the need for corresponding blood

Author

Tilborg, A.G. van, Kompier, L., Lurkin, I., Poort, R., El Bouazzaoui, S., van der Keur, K., Zuiverloon, T., Dyrskjot, L., Orntoft, T., Roobol, M., Zwarthoff, E., Tilborg, A.G. van, Kompier, L., Lurkin, I., Poort, R., El Bouazzaoui, S., van der Keur, K., Zuiverloon, T., Dyrskjot, L., Orntoft, T., Roobol, M., and Zwarthoff, E.

Abstract

Contains fulltext : 109466.pdf (publisher's version ) (Open Access)

Published
2012

30. Analysis of molecular intra-patient variation and delineation of a prognostic 12-gene signature in non-muscle invasive bladder cancer; technology transfer from microarrays to PCR

Author

Dyrskjot, L, Reinert, T, Novoradovsky, A, Zuiverloon, Tahlita, Beukers, Willemien, Zwarthoff, Ellen, Malats, N, Real, FX, Segersten, U, Malmstrom, PU, Knowles, M, Hurst, C, Sorge, J, Borre, M, Orntoft, TF, Dyrskjot, L, Reinert, T, Novoradovsky, A, Zuiverloon, Tahlita, Beukers, Willemien, Zwarthoff, Ellen, Malats, N, Real, FX, Segersten, U, Malmstrom, PU, Knowles, M, Hurst, C, Sorge, J, Borre, M, and Orntoft, TF

Abstract

BACKGROUND: Multiple clinical risk factors and genetic profiles have been demonstrated to predict progression of non-muscle invasive bladder cancer; however, no easily clinical applicable gene signature has been developed to predict disease progression independent of disease stage and grade. METHODS: We measured the intra-patient variation of an 88-gene progression signature using 39 metachronous tumours from 17 patients. For delineation of the optimal quantitative reverse transcriptase PCR panel of markers, we used 115 tumour samples from patients in Denmark, Sweden, UK and Spain. RESULTS: Analysis of intra-patient variation of the molecular markers showed 71% similar classification results. A final panel of 12 genes was selected, showing significant correlation with outcome. In multivariate Cox regression analysis, we found that the 12-gene signature was an independent prognostic factor (hazard ratio = 7.4 (95% confidence interval: 3.4-15.9), P < 0.001) when adjusting for stage, grade and treatment. Independent validation of the 12-gene panel and the determined cut-off v CONCLUSION: Intra-patient marker variation in metachronous tumours is present. Therefore, to increase test sensitivity, it may be necessary to test several metachronous tumours from a patient's disease course. A PCR-based 12-gene signature significantly predicts disease progression in patients with non-muscle invasive bladder cancer. British Journal of Cancer (2012) 107, 1392-1398. doi:10.1038/bjc.2012.412 www.bjcancer.com Published online 13 September 2012 (C) 2012 Cancer Research UK

Published
2012

31. Selection of Microsatellite Markers for Bladder Cancer Diagnosis without the Need for Corresponding Blood

Author

Tilborg, Angela, Kompier, Lucie, Lurkin, Irene, Poort, R, el Bouazzaoui, S, Keur, Kirstin, Zuiverloon, Tahlita, Dyrskjot, L, Orntoft, TF, Roobol - Bouts, Monique, Zwarthoff, Ellen, Tilborg, Angela, Kompier, Lucie, Lurkin, Irene, Poort, R, el Bouazzaoui, S, Keur, Kirstin, Zuiverloon, Tahlita, Dyrskjot, L, Orntoft, TF, Roobol - Bouts, Monique, and Zwarthoff, Ellen

Abstract

Microsatellite markers are used for loss-of-heterozygosity, allelic imbalance and clonality analyses in cancers. Usually, tumor DNA is compared to corresponding normal DNA. However, normal DNA is not always available and can display aberrant allele ratios due to copy number variations in the genome. Moreover, stutter peaks may complicate the analysis. To use microsatellite markers for diagnosis of recurrent bladder cancer, we aimed to select markers without stutter peaks and a constant ratio between alleles, thereby avoiding the need for a control DNA sample. We investigated 49 microsatellite markers with tri- and tetranucleotide repeats in regions commonly lost in bladder cancer. Based on analysis of 50 blood DNAs the 12 best performing markers were selected with few stutter peaks and a constant ratio between peaks heights. Per marker upper and lower cut off values for allele ratios were determined. LOH of the markers was observed in 59/104 tumor DNAs. We then determined the sensitivity of the marker panel for detection of recurrent bladder cancer by assaying 102 urine samples of these patients. Sensitivity was 63% when patients were stratified for LOH in their primary tumors. We demonstrate that up-front selection of microsatellite markers obliterates the need for a corresponding blood sample. For diagnosis of bladder cancer recurrences in urine this significantly reduces costs. Moreover, this approach facilitates retrospective analysis of archival tumor samples for allelic imbalance.

Published
2012

32. Diagnostic and prognostic microRNAs in stage II colon cancer

Author

Schepeler, T., Reinert, J.T., Ostenfeld, M.S., Christensen, L.L., Silahtaroglu, Asli, Dyrskjot, L., Wiuf, C., Sorensen, F.J., Kruhoffer, M., Laurberg, S., Kauppinen, S., Orntoft, T.F., Andersen, C.L., Schepeler, T., Reinert, J.T., Ostenfeld, M.S., Christensen, L.L., Silahtaroglu, Asli, Dyrskjot, L., Wiuf, C., Sorensen, F.J., Kruhoffer, M., Laurberg, S., Kauppinen, S., Orntoft, T.F., and Andersen, C.L.

Abstract

Udgivelsesdato: 2008/8/1

Published
2008

33. The DNA damage checkpoint precedes activation of ARF in response to escalating oncogenic stress during tumorigenesis

Author

Evangelou, K, primary, Bartkova, J, additional, Kotsinas, A, additional, Pateras, I S, additional, Liontos, M, additional, Velimezi, G, additional, Kosar, M, additional, Liloglou, T, additional, Trougakos, I P, additional, Dyrskjot, L, additional, Andersen, C L, additional, Papaioannou, M, additional, Drosos, Y, additional, Papafotiou, G, additional, Hodny, Z, additional, Sosa-Pineda, B, additional, Wu, X-R, additional, Klinakis, A, additional, Ørntoft, T, additional, Lukas, J, additional, Bartek, J, additional, and Gorgoulis, V G, additional

Published
2013
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43. miRNAs associated with chemo-sensitivity in cell lines and in advanced bladder cancer

Author

Nordentoft Iver, Birkenkamp-Demtroder Karin, Agerbæk Mads, Theodorescu Dan, Ostenfeld Marie, Hartmann Arndt, Borre Michael, Ørntoft Torben F, and Dyrskjøt Lars

Subjects
Internal medicine, RC31-1245, Genetics, QH426-470
Abstract

Abstract Background MicroRNA is a naturally occurring class of non-coding RNA molecules that mediate posttranscriptional gene regulation and are strongly implicated in cellular processes such as cell proliferation, carcinogenesis, cell survival and apoptosis. Consequently there is increasing focus on miRNA expression as prognostic factors for outcome and chemotherapy response. Only approximately 50% of patients with bladder cancer respond to chemotherapy. Therefore, predictive markers, such as miRNAs, that can identify subgroups of patients who will benefit from chemotherapy will have great value for treatment guidance. Methods We profiled the expression of 671 miRNAs in formalin fixed paraffin embedded tumors from patients with advanced bladder cancer treated with cisplatin based chemotherapy. We delineated differentially expressed miRNAs in tumors from patients with complete response vs. patients with progressive disease and in tumors form patients with short and long overall survival time. Furthermore, we studied the effect of up- and down regulation of key miRNAs on the cisplatin sensitivity in eight bladder cancer cell lines with different sensitivities to cisplatin. Results miRNA expression profiling identified 15 miRNAs that correlated with response to chemotherapy and 5 miRNAs that correlated with survival time. Three miRNAs were associated with both response and survival (886-3p, 923, 944). By changing the cellular level of the response-identified miRNAs in eight bladder cell lines with different cisplatin sensitivity we found that down-regulation of miR-27a, miR296-5p and miR-642 generally reduced the cell viability, whereas up-regulation of miR-138 and miR-886-3p reduced the viability of more than half of the cell lines. Decreasing miR-138 increased the cisplatin sensitivity in half of the cell lines and increasing miR-27a and miR-642 generally increased cisplatin sensitivity. Conclusions MiRNAs seem to be involved in cisplatin based chemo response and may form a new target for therapy and serve as biomarkers for treatment response.

Published
2012
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44. Tumor-specific usage of alternative transcription start sites in colorectal cancer identified by genome-wide exon array analysis

Author

Laurila Kirsti, Mansilla Francisco, Eller Asger, Pedersen Jakob, Lamy Philippe, Hansen Kristian Q, Wang Kai, Vang Søren, Rasmussen Mads H, Øster Bodil, Schepeler Troels, Thorsen Kasper, Wiuf Carsten, Laurberg Søren, Dyrskjøt Lars, Ørntoft Torben F, and Andersen Claus L

Subjects
Biotechnology, TP248.13-248.65, Genetics, QH426-470
Abstract

Abstract Background Approximately half of all human genes use alternative transcription start sites (TSSs) to control mRNA levels and broaden the transcriptional output in healthy tissues. Aberrant expression patterns promoting carcinogenesis, however, may arise from alternative promoter usage. Results By profiling 108 colorectal samples using exon arrays, we identified nine genes (TCF12, OSBPL1A, TRAK1, ANK3, CHEK1, UGP2, LMO7, ACSL5, and SCIN) showing tumor-specific alternative TSS usage in both adenoma and cancer samples relative to normal mucosa. Analysis of independent exon array data sets corroborated these findings. Additionally, we confirmed the observed patterns for selected mRNAs using quantitative real-time reverse-transcription PCR. Interestingly, for some of the genes, the tumor-specific TSS usage was not restricted to colorectal cancer. A comprehensive survey of the nine genes in lung, bladder, liver, prostate, gastric, and brain cancer revealed significantly altered mRNA isoform ratios for CHEK1, OSBPL1A, and TCF12 in a subset of these cancer types. To identify the mechanism responsible for the shift in alternative TSS usage, we antagonized the Wnt-signaling pathway in DLD1 and Ls174T colorectal cancer cell lines, which remarkably led to a shift in the preferred TSS for both OSBPL1A and TRAK1. This indicated a regulatory role of the Wnt pathway in selecting TSS, possibly also involving TP53 and SOX9, as their transcription binding sites were enriched in the promoters of the tumor preferred isoforms together with their mRNA levels being increased in tumor samples. Finally, to evaluate the prognostic impact of the altered TSS usage, immunohistochemistry was used to show deregulation of the total protein levels of both TCF12 and OSBPL1A, corresponding to the mRNA levels observed. Furthermore, the level of nuclear TCF12 had a significant correlation to progression free survival in a cohort of 248 stage II colorectal cancer samples. Conclusions Alternative TSS usage in colorectal adenoma and cancer samples has been shown for nine genes, and OSBPL1A and TRAK1 were found to be regulated in vitro by Wnt signaling. TCF12 protein expression was upregulated in cancer samples and correlated with progression free survival.

Published
2011
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45. Evaluation of two commercial global miRNA expression profiling platforms for detection of less abundant miRNAs

Author

Ørntoft Torben F, Dyrskjøt Lars, Ostenfeld Marie S, Rasmussen Mads H, Lamy Philippe, Jensen Steffen G, and Andersen Claus L

Subjects
Biotechnology, TP248.13-248.65, Genetics, QH426-470
Abstract

Abstract Background microRNAs (miRNA) are short, endogenous transcripts that negatively regulate the expression of specific mRNA targets. miRNAs are found both in tissues and body fluids such as plasma. A major perspective for the use of miRNAs in the clinical setting is as diagnostic plasma markers for neoplasia. While miRNAs are abundant in tissues, they are often scarce in plasma. For quantification of miRNA in plasma it is therefore of importance to use a platform with high sensitivity and linear performance in the low concentration range. This motivated us to evaluate the performance of three commonly used commercial miRNA quantification platforms: GeneChip miRNA 2.0 Array, miRCURY Ready-to-Use PCR, Human panel I+II V1.M, and TaqMan Human MicroRNA Array v3.0. Results Using synthetic miRNA samples and plasma RNA samples spiked with different ratios of 174 synthetic miRNAs we assessed the performance characteristics reproducibility, recovery, specificity, sensitivity and linearity. It was found that while the qRT-PCR based platforms were sufficiently sensitive to reproducibly detect miRNAs at the abundance levels found in human plasma, the array based platform was not. At high miRNA levels both qRT-PCR based platforms performed well in terms of specificity, reproducibility and recovery. At low miRNA levels, as in plasma, the miRCURY platform showed better sensitivity and linearity than the TaqMan platform. Conclusion For profiling clinical samples with low miRNA abundance, such as plasma samples, the miRCURY platform with its better sensitivity and linearity would probably be superior.

Published
2011
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46. Increased expression of transcription factor TFAP2α correlates with chemosensitivity in advanced bladder cancer

Author

Lehmann Jan, Bertz Simone, Hartmann Arndt, Wild Peter J, Bødker Julie S, Dyrskjøt Lars, Nordentoft Iver, Ørntoft Torben F, and Birkenkamp-Demtroder Karin

Subjects
Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282
Abstract

Abstract Background The standard treatment for patients with advanced transitional cell carcinoma of the bladder is platin based chemotherapy. Only approximately 50% of the patients respond to chemotherapy. Therefore, molecular predictive markers for identification of chemotherapy sensitive subgroups of patients are highly needed. We selected the transcription factor TFAP2α from a previously identified gene expression signature for chemotherapy response. Methods TFAP2α expression and localization was assessed by immunohistochemistry using a tissue microarray (TMA) containing 282 bladder cancer tumors from patients with locally advanced (pT2-T4b and N1-3) or metastatic (M1) disease. All patients had received cisplatin containing chemotherapy. Furthermore, QPCR analysis of three TFAP2α isoforms was performed on tumor specimens of advanced muscle invasive bladder cancers (T2-4). Using the bladder cell lines T24 and SW780 the relation of TFAP2α and cisplatin and gemcitabine sensitivity as well as cell proliferation was examined using siRNA directed TFAP2α knockdown. Results TFAP2α protein expression was analyzed on a TMA with cores from 282 advanced bladder cancer tumors from patients treated with cisplatin based combinational chemotherapy. TFAP2α was identified as a strong independent predictive marker for a good response and survival after cisplatin-containing chemotherapy in patients with advanced bladder cancer. Strong TFAP2α nuclear and cytoplasmic staining predicted good response to chemotherapy in patients with lymph node metastasis, whereas weak TFAP2α nuclear staining predicted good response in patients without lymph node metastasis. In vitro studies showed that siRNA mediated knockdown of TFAP2α increased the proliferation of SW780 cells and rendered the cells less sensitive to cisplatin and gemcitabine. In contrast to that T24 bladder cells with mutated p53 showed to be more drug sensitive upon TFAP2α depletion. Conclusions High levels of nuclear and cytoplasmic TFAP2α protein were a predictor of increased overall survival and progression free survival in patients with advanced bladder cancer treated with cisplatin based chemotherapy. TFAP2α knockdown increased the proliferation of the SW780 bladder cells and reduced cisplatin and gemcitabine induced cell death. The inverse effect was observed in the TP53 mutated T24 cell line where TFAP2α silencing augmented cisplatin and gemcitabine sensitivity and did not stimulate proliferation.

Published
2011
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47. Prediction and diagnosis of bladder cancer recurrence based on urinary content of hTERT, SENP1, PPP1CA, and MCM5 transcripts

Author

Munksgaard Pia P, Mansilla Francisco, Higuchi Russell, Holcomb Cherie, Toldbod Helle, Zieger Karsten, Brems-Eskildsen Anne, Borre Michael, Ørntoft Torben F, and Dyrskjøt Lars

Subjects
Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282
Abstract

Abstract Background Identification of urinary biomarkers for detection of bladder cancer recurrence would be beneficial to minimize the frequency of cystoscopy. Our objective was to determine the usability of urine content of mRNA in the detection and prediction of bladder cancer recurrence. Methods We analyzed 123 prospectively cross-sectional collected urine samples from 117 patients with bladder cancer (12 incident cancers and 111 control visits). We used biopsies from cystoscopies as diagnostic criteria for recurrence, and followed the patients for a median time of 28.5 months (range 0-44 months). We measured the levels of hTERT, SENP1, PPP1CA, and MCM5 mRNA in urine by q-RT- PCR. Results We found significant differences in urinary content of hTERT (p < 0.001), SENP1 (p < 0.001), MCM5 (p < 0.001), and PPP1CA (p < 0.001) transcripts, when comparing urine samples from patients with and without tumor present in the bladder. We obtained sensitivity and specificity values for hTERT: 63/73, SENP1: 56/78, MCM5: 63/66, and PPP1CA: 69/63, respectively. Including follow-up data resulted in sensitivity and specificity values for hTERT: 62/84, SENP1:53/84, MCM5: 61/73, and PPP1CA: 65/66. Interestingly, at non-tumor visits the urinary content of especially hTERT (p = 0.0001) and MCM5 (p = 0.02) were significantly associated with subsequent tumour recurrence. Combining the markers with cytology improved the detection. The best combination was hTERT and cytology with a sensitivity of 71% and a specificity of 86% after follow-up. Further prospective validation or registration studies needs to be carried out before clinical use. Conclusions We could use the urinary content of hTERT, SENP1, PPP1CA, and MCM5 to detect bladder cancer recurrence. All markers showed a higher sensitivity than cytology. The detection rate improved when including cytology results, but also the combination of hTERT and MCM5 increased the detection rate. Furthermore, hTERT and MCM5 levels predicted subsequent tumor recurrences.

Published
2010
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48. High frequency of tumor cells with nuclear Egr-1 protein expression in human bladder cancer is associated with disease progression

Author

Oleksiewicz Martin B, Ørntoft Torben F, Borre Michael, Fristrup Niels, Bartels Annette, Egerod Frederikke, Brünner Nils, and Dyrskjøt Lars

Subjects
Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282
Abstract

Abstract Background Egr-1 (early growth response-1 transcription factor) has been proposed to be involved in invasion and metastasis processes of human bladder cancer, but Egr-1 protein expression levels in human bladder cancer have not been investigated. In the present study we investigated the expression levels of Egr-1 protein in early stages of human bladder cancer and correlated it to later progression. Methods Expression of Egr-1 protein in human bladder cancer was examined by immunohistochemistry, on a tissue microarray constructed from tumors from 289 patients with non-muscle invasive urothelial bladder cancer. Results The frequency of tumor cells with nuclear Egr-1 immunolabelling correlated to bladder cancer stage, grade and to later progression to muscle-invasive bladder cancer (T2-4). Stage T1 tumors exhibited significantly higher frequencies of tumor cells with nuclear Egr-1 immunolabelling than Ta tumors (P = 0.001). Furthermore, Kaplan-Meier survival analysis showed that a high frequency of tumor cells with nuclear Egr-1 immunolabelling was significantly associated with a higher risk of progression to stage T2-4 (log-rank test, P = 0.035). Tumor cells with nuclear Egr-1 immunolabelling were found to localize at the tumor front in some of the tumor biopsies. Conclusion The results from this study support a potential involvement of Egr-1 in the progression from non-muscle invasive bladder cancers to muscle invasive bladder cancer.

Published
2009
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49. Chromosomal imbalance in the progression of high-risk non-muscle invasive bladder cancer

Author

Ørntoft Torben, Jensen Klaus, Wiuf Carsten, Zieger Karsten, and Dyrskjøt Lars

Subjects
Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282
Abstract

Abstract Background Non-muscle invasive bladder neoplasms with invasion of the lamina propria (stage T1) or high grade of dysplasia are at "high risk" of progression to life-threatening cancer. However, the individual course is difficult to predict. Chromosomal instability (CI) is associated with high tumor stage and grade, and possibly with the risk of progression. Methods To investigate the relationship between CI and subsequent disease progression, we performed a case-control-study of 125 patients with "high-risk" non-muscle invasive bladder neoplasms, 67 with later disease progression, and 58 with no progression. Selection criteria were conservative (non-radical) resections and full prospective clinical follow-up (> 5 years). We investigated primary lesions in 59, and recurrent lesions in 66 cases. We used Affymetrix GeneChip® Mapping 10 K and 50 K SNP microarrays to evaluate genome wide chromosomal imbalance (loss-of-heterozygosity and DNA copy number changes) in 48 representative tumors. DNA copy number changes of 15 key instability regions were further investigated using QPCR in 101 tumors (including 25 tumors also analysed on 50 K SNP microarrays). Results Chromosomal instability did not predict any higher risk of subsequent progression. Stage T1 and high-grade tumors had generally more unstable genomes than tumors of lower stage and grade (mostly non-primary tumors following a "high-risk" tumor). However, about 25% of the "high-risk" tumors had very few alterations. This was independent of subsequent progression. Recurrent lesions represent underlying field disease. A separate analysis of these lesions did neither reflect any difference in the risk of progression. Of specific chromosomal alterations, a possible association between loss of chromosome 8p11 and the risk of progression was found. However, the predictive value was limited by the heterogeneity of the changes. Conclusion Chromosomal instability (CI) was associated with "high risk" tumors (stage T1 or high-grade), but did not predict subsequent progression. Recurrences after "high-risk" tumors had fewer chromosomal alterations, but there was no association with the risk of progression in this group either. Thus, the prediction of progression of "high risk" non-muscle invasive bladder tumors using chromosomal changes is difficult. Loss of chromosome 8p11 may play a role in the progression process. About 25% of the "high risk" tumors were chromosomal stable.

Published
2009
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50. Increased cell motility and invasion upon knockdown of lipolysis stimulated lipoprotein receptor (LSR) in SW780 bladder cancer cells

Author

Ørntoft Torben F, Hein Anne-Mette K, Wiuf Carsten, Thykjaer Thomas, Birkenkamp-Demtroder Karin, Herbsleb Malene, and Dyrskjøt Lars

Subjects
Internal medicine, RC31-1245, Genetics, QH426-470
Abstract

Abstract Background Mechanisms underlying the malignant development in bladder cancer are still not well understood. Lipolysis stimulated lipoprotein receptor (LSR) has previously been found to be upregulated by P53. Furthermore, we have previously found LSR to be differentially expressed in bladder cancer. Here we investigated the role of LSR in bladder cancer. Methods A time course siRNA knock down experiment was performed to investigate the functional role of LSR in SW780 bladder cancer cells. Since LSR was previously shown to be regulated by P53, siRNA against TP53 was included in the experimental setup. We used Affymetrix GeneChips for measuring gene expression changes and we used Ingenuity Pathway Analysis to investigate the relationship among differentially expressed genes upon siRNA knockdown. Results By Ingenuity Pathway analysis of the microarray data from the different timepoints we identified six gene networks containing genes mainly related to the functional categories "cancer", "cell death", and "cellular movement". We determined that genes annotated to the functional category "cellular movement" including "invasion" and "cell motility" were highly significantly overrepresented. A matrigel assay showed that 24 h after transfection the invasion capacity was significantly increased 3-fold (p < 0.02) in LSR-siRNA transfected cells, and 2.7-fold (p < 0.02) in TP53-siRNA transfected cells compared to controls. After 48 h the motility capacity was significantly increased 3.5-fold (p < 0.004) in LSR-siRNA transfected cells, and 4.7-fold (p < 0.002) in TP53-siRNA transfected cells compared to controls. Conclusion We conclude that LSR may impair bladder cancer cells from gaining invasive properties.

Published
2008
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