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4. Recommendations on scuba diving in Birt-Hogg-Dubé syndrome

Author

van Riel, L., van Hulst, R. A., van Hest, L., van Moorselaar, R. J.A., Boerrigter, B. G., Franken, S. M., Wolthuis, R. M.F., Dubbink, H. J., Marciniak, S. J., Gupta, N., van de Beek, I., Houweling, A. C., van Riel, L., van Hulst, R. A., van Hest, L., van Moorselaar, R. J.A., Boerrigter, B. G., Franken, S. M., Wolthuis, R. M.F., Dubbink, H. J., Marciniak, S. J., Gupta, N., van de Beek, I., and Houweling, A. C.

Abstract

Introduction: Although very uncommon, severe injury and death can occur during scuba diving. One of the main causes of scuba diving fatalities is pulmonary barotrauma due to significant changes in ambient pressure. Pathology of the lung parenchyma, such as cystic lesions, might increase the risk of pulmonary barotrauma. Areas covered: Birt–Hogg–Dubé syndrome (BHD), caused by pathogenic variants in the FLCN gene, is characterized by skin fibrofolliculomas, an increased risk of renal cell carcinoma, multiple lung cysts and spontaneous pneumothorax. Given the pulmonary involvement, in some countries patients with BHD are generally recommended to avoid scuba diving, although evidence-based guidelines are lacking. We aim to provide recommendations on scuba diving for patients with BHD, based on a survey of literature on pulmonary cysts and pulmonary barotrauma in scuba diving. Expert opinion: In our opinion, although the absolute risks are likely to be low, caution is warranted. Given the relative paucity of literature and the potential fatal outcome, patients with BHD with a strong desire for scuba diving should be informed of the potential risks in a personal assessment. If available a diving physician should be consulted, and a low radiation dose chest computed tomography (CT)-scan to assess pulmonary lesions could be considered.

Published
2023

5. Molecular alterations and potential actionable mutations in peritoneal mesothelioma:a scoping review of high-throughput sequencing studies

Author

Dietz, M V, van Kooten, J P, Paats, M S, Aerts, J G V J, Verhoef, C, Madsen, E V E, Dubbink, H J, von der Thüsen, J H, Dietz, M V, van Kooten, J P, Paats, M S, Aerts, J G V J, Verhoef, C, Madsen, E V E, Dubbink, H J, and von der Thüsen, J H

Abstract

BACKGROUND:Peritoneal mesothelioma (PeM) is a rare malignancy with a poor prognosis. Currently there is a lack of effective systemic therapies. Due to the rarity of PeM, it is challenging to study new treatment options. Off-label use of targeted drugs could be an effective approach. This scoping review aims to explore the genomic landscape of PeM to identify potential therapeutic targets.MATERIALS AND METHODS:A systematic literature search of Embase, Medline, Web of Science, the Cochrane Library, and Google Scholar was carried out up to 1 November 2022. Studies that reported on molecular alterations in PeM detected by high-throughput sequencing techniques were included. Genes that were altered in ≥1% of PeMs were selected for the identification of potential targeted therapies.RESULTS: Thirteen articles were included, comprising 824 PeM patients. In total, 142 genes were altered in ≥1% of patients, of which 7 genes were altered in ≥10%. BAP1 was the most commonly altered gene (50%). Other commonly altered genes were NF2 (25%), CDKN2A (23%), CDKN2B (17%), PBRM1 (15%), TP53 (14%), and SETD2 (13%). In total, 17% of PeM patients were carriers of a germline mutation, mainly in BAP1 (7%).CONCLUSIONS: This scoping review provides an overview of the mutational landscape of PeM. Germline mutations might be a larger contributor to the incidence of PeM than previously thought. Currently available targeted therapy options are limited, but several targeted agents [such as poly (ADP-ribose) polymerase (PARP), enhancer of zeste homolog 2 (EZH2), and cyclin-dependent kinase 4/6 (CDK4/6) inhibitors] were identified that might provide new targeted therapy options in the future.

Published
2023

6. Medulloblastoma in adults:evaluation of the Dutch society for neuro-oncology treatment protocol

Author

Bleeker, L., Kouwenhoven, M. C.M., de Heer, I., Lissenberg-Witte, B. I., Gijsbers, A. H., Dubbink, H. J., Kros, J. M., Gijtenbeek, J. M.M., Kurt, E., van der Rijt, C. C.D., Swaak-Kragten, A. T., de Vos, F. Y., van der Weide, H. L., French, P. J., van den Bent, M. J., Wesseling, P., Bromberg, J. E.C., Bleeker, L., Kouwenhoven, M. C.M., de Heer, I., Lissenberg-Witte, B. I., Gijsbers, A. H., Dubbink, H. J., Kros, J. M., Gijtenbeek, J. M.M., Kurt, E., van der Rijt, C. C.D., Swaak-Kragten, A. T., de Vos, F. Y., van der Weide, H. L., French, P. J., van den Bent, M. J., Wesseling, P., and Bromberg, J. E.C.

Abstract

Purpose: Medulloblastoma is a rare tumor in adults. The objective of this nationwide, multicenter study was to evaluate the toxicity and efficacy of the Dutch treatment protocol for adult medulloblastoma patients. Methods: Adult medulloblastoma patients diagnosed between 2010 and 2018 were identified in the Dutch rare tumors registry or nationwide pathology database. Patients with intention to treat according to the national treatment protocol were included. Risk stratification was performed based on residual disease, histological subtype and extent of disease. All patients received postoperative radiotherapy [craniospinal axis 36 Gy/fossa posterior boost 19.8 Gy (14.4 Gy in case of metastases)]. High-risk patients received additional neoadjuvant (carboplatin-etoposide), concomitant (vincristine) and adjuvant chemotherapy (carboplatin-vincristine-cyclophosphamide) as far as feasible by toxicity. Methylation profiling, and additional next-generation sequencing in case of SHH-activated medulloblastomas, were performed. Results: Forty-seven medulloblastoma patients were identified, of whom 32 were treated according to the protocol. Clinical information and tumor material was available for 28 and 20 patients, respectively. The histological variants were mainly classic (43%) and desmoplastic medulloblastoma (36%). Sixteen patients (57%) were considered standard-risk and 60% were SHH-activated medulloblastomas. Considerable treatment reductions and delays in treatment occurred due to especially hematological and neurotoxicity. Only one high-risk patient could complete all chemotherapy courses. 5-years progression-free survival (PFS) and overall survival (OS) for standard-risk patients appeared worse than for high-risk patients (PFS 69% vs. 90%, OS 81% vs. 90% respectively), although this wasn’t statistically significant. Conclusion: Combined chemo-radiotherapy is a toxic regimen for adult medulloblastoma patients that may result in improved

Published
2023

7. Medulloblastoma in adults: evaluation of the Dutch society for neuro-oncology treatment protocol

Author

MS Medische Oncologie, Cancer, Bleeker, L, Kouwenhoven, M C M, de Heer, I, Lissenberg-Witte, B I, Gijsbers, A H, Dubbink, H J, Kros, J M, Gijtenbeek, J M M, Kurt, E, van der Rijt, C C D, Swaak-Kragten, A T, de Vos, F Y, van der Weide, H L, French, P J, van den Bent, M J, Wesseling, P, Bromberg, J E C, MS Medische Oncologie, Cancer, Bleeker, L, Kouwenhoven, M C M, de Heer, I, Lissenberg-Witte, B I, Gijsbers, A H, Dubbink, H J, Kros, J M, Gijtenbeek, J M M, Kurt, E, van der Rijt, C C D, Swaak-Kragten, A T, de Vos, F Y, van der Weide, H L, French, P J, van den Bent, M J, Wesseling, P, and Bromberg, J E C

Published
2023

8. P11.69.B IDH1/2wildtype gliomas grade 2 and 3 with molecular glioblastoma-like profile have a distinct course of epilepsy compared toIDH1/2wildtype glioblastomas

Author

van Opijnen, M P, primary, Tesileanu, C M S, additional, Dirven, L, additional, van der Meer, P B, additional, Wijnenga, M M J, additional, Vincent, A J P E, additional, Broekman, M L D, additional, Dubbink, H J, additional, Kros, J M, additional, van Duinen, S G, additional, Smits, M, additional, French, P J, additional, van den Bent, M J, additional, Taphoorn, M J B, additional, and Koekkoek, J A F, additional

Published
2022
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9. Prognostic significance of genome-wide DNA methylation profiles within the randomised, phase 3, EORTC CATNON trial on non-1p/19q deleted anaplastic glioma.

Author

UCL - SSS/IREC/MIRO - Pôle d'imagerie moléculaire, radiothérapie et oncologie, Tesileanu, C M S, van den Bent, M J, Sanson, M, Wick, W, Brandes, A A, Clement, P M, Erridge, S C, Vogelbaum, M A, Nowak, A K, Baurain, Jean-François, Mason, W P, Wheeler, H, Chinot, O L, Gill, S, Griffin, M, Rogers, L, Taal, W, Rudà, R, Weller, M, McBain, C, van Linde, M E, Sabedot, T S, Hoogstrate, Y, von Deimling, A, de Heer, I, van IJcken, W F J, Brouwer, R W W, Aldape, K, Jenkins, R B, Dubbink, H J, Kros, J M, Wesseling, P, Cheung, K J, Golfinopoulos, V, Baumert, B G, Gorlia, T, Noushmehr, H, French, P J, UCL - SSS/IREC/MIRO - Pôle d'imagerie moléculaire, radiothérapie et oncologie, Tesileanu, C M S, van den Bent, M J, Sanson, M, Wick, W, Brandes, A A, Clement, P M, Erridge, S C, Vogelbaum, M A, Nowak, A K, Baurain, Jean-François, Mason, W P, Wheeler, H, Chinot, O L, Gill, S, Griffin, M, Rogers, L, Taal, W, Rudà, R, Weller, M, McBain, C, van Linde, M E, Sabedot, T S, Hoogstrate, Y, von Deimling, A, de Heer, I, van IJcken, W F J, Brouwer, R W W, Aldape, K, Jenkins, R B, Dubbink, H J, Kros, J M, Wesseling, P, Cheung, K J, Golfinopoulos, V, Baumert, B G, Gorlia, T, Noushmehr, H, and French, P J

Abstract

Survival in patients with IDH1/2 mutant (mt) anaplastic astrocytomas is highly variable. We have used the prospective phase 3 CATNON trial to identify molecular factors related to outcome in IDH1/2mt anaplastic astrocytoma patients. The CATNON trial randomized 751 adult patients with newly diagnosed 1p/19q non-codeleted anaplastic glioma to 59.4 Gy radiotherapy +/- concurrent and/or adjuvant temozolomide. The presence of necrosis and/or microvascular proliferation was scored at central pathology review. Infinium MethylationEPIC BeadChip arrays were used for genome-wide DNA methylation analysis and the determination of copy number variations (CNV). Two DNA methylation-based tumour classifiers were used for risk stratification. Next-generation sequencing (NGS) was performed using one of two glioma-tailored NGS panels. The primary endpoint was overall survival measured from date of randomization. Full analysis (genome-wide DNA methylation and NGS) was successfully performed on 654 tumours. Of these, 432 tumours were IDH1/2mt anaplastic astrocytomas. Both epigenetic classifiers identified poor prognosis patients that partially overlapped. A predictive prognostic Cox proportional hazards model identified that independent prognostic factors for IDH1/2mt anaplastic astrocytoma patients included; age, mini-mental state examination score, treatment with concurrent and/or adjuvant temozolomide, the epigenetic classifiers, PDGFRA amplification, CDKN2A/B homozygous deletion, PI3K mutations and total CNV load. Independent recursive partitioning analysis highlights the importance of these factors for patient prognostication. Both clinical and molecular factors identify IDH1/2mt anaplastic astrocytoma patients with worse outcome. These results will further refine the current WHO criteria for glioma classification.

Published
2021

10. Corrigendum to INTELLANCE 2/EORTC 1410 randomized phase II study of Depatux-M alone and with temozolomide vs temozolomide or lomustine in recurrent EGFR amplified glioblastoma

Author

van den Bent, Martin, Eoli, Marica, Sepulveda, Juan Manuel, Smits, Marion, Walenkamp, Annemiek, Frenel, Jean-Sebastian, Franceschi, Enrico, Clement, Paul M, Chinot, Olivier, de Vos, Filip, Whenham, Nicolas, Sanghera, Paul, Weller, Michael, Dubbink, H J, French, Pim, Looman, Jim, Dey, Jyotirmoy, Krause, Scott, Ansell, Pete, Nuyens, Sarah, Spruyt, Maarten, Brilhante, Joana, Coens, Corneel, Gorlia, Thierry, Golfinopoulos, Vassilis, van den Bent, Martin, Eoli, Marica, Sepulveda, Juan Manuel, Smits, Marion, Walenkamp, Annemiek, Frenel, Jean-Sebastian, Franceschi, Enrico, Clement, Paul M, Chinot, Olivier, de Vos, Filip, Whenham, Nicolas, Sanghera, Paul, Weller, Michael, Dubbink, H J, French, Pim, Looman, Jim, Dey, Jyotirmoy, Krause, Scott, Ansell, Pete, Nuyens, Sarah, Spruyt, Maarten, Brilhante, Joana, Coens, Corneel, Gorlia, Thierry, and Golfinopoulos, Vassilis

Published
2021

11. Corrigendum to INTELLANCE 2/EORTC 1410 randomized phase II study of Depatux-M alone and with temozolomide vs temozolomide or lomustine in recurrent EGFR amplified glioblastoma

Author

MS Medische Oncologie, Cancer, van den Bent, Martin, Eoli, Marica, Sepulveda, Juan Manuel, Smits, Marion, Walenkamp, Annemiek, Frenel, Jean-Sebastian, Franceschi, Enrico, Clement, Paul M, Chinot, Olivier, de Vos, Filip, Whenham, Nicolas, Sanghera, Paul, Weller, Michael, Dubbink, H J, French, Pim, Looman, Jim, Dey, Jyotirmoy, Krause, Scott, Ansell, Pete, Nuyens, Sarah, Spruyt, Maarten, Brilhante, Joana, Coens, Corneel, Gorlia, Thierry, Golfinopoulos, Vassilis, MS Medische Oncologie, Cancer, van den Bent, Martin, Eoli, Marica, Sepulveda, Juan Manuel, Smits, Marion, Walenkamp, Annemiek, Frenel, Jean-Sebastian, Franceschi, Enrico, Clement, Paul M, Chinot, Olivier, de Vos, Filip, Whenham, Nicolas, Sanghera, Paul, Weller, Michael, Dubbink, H J, French, Pim, Looman, Jim, Dey, Jyotirmoy, Krause, Scott, Ansell, Pete, Nuyens, Sarah, Spruyt, Maarten, Brilhante, Joana, Coens, Corneel, Gorlia, Thierry, and Golfinopoulos, Vassilis

Published
2021

15. Corrigendum to INTELLANCE 2/EORTC 1410 randomized phase II study of Depatux-M alone and with temozolomide vs temozolomide or lomustine in recurrent EGFR amplified glioblastoma

Author

van den Bent, Martin, primary, Eoli, Marica, additional, Sepulveda, Juan Manuel, additional, Smits, Marion, additional, Walenkamp, Annemiek, additional, Frenel, Jean-Sebastian, additional, Franceschi, Enrico, additional, Clement, Paul M, additional, Chinot, Olivier, additional, de Vos, Filip, additional, Whenham, Nicolas, additional, Sanghera, Paul, additional, Weller, Michael, additional, Dubbink, H J, additional, French, Pim, additional, Looman, Jim, additional, Dey, Jyotirmoy, additional, Krause, Scott, additional, Ansell, Pete, additional, Nuyens, Sarah, additional, Spruyt, Maarten, additional, Brilhante, Joana, additional, Coens, Corneel, additional, Gorlia, Thierry, additional, and Golfinopoulos, Vassilis, additional

Published
2020
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16. INTELLANCE 2/EORTC 1410 randomized phase II study of Depatux-M alone and with temozolomide vs temozolomide or lomustine in recurrent EGFR amplified glioblastoma

Author

Van Den Bent, Martin, Eoli, Marica, Sepulveda, Juan Manuel, Smits, Marion, Walenkamp, Annemiek, Frenel, Jean-Sebastian, Franceschi, Enrico, Clement, Paul M, Chinot, Olivier, De Vos, Filip, Whenham, Nicolas, Sanghera, Paul, Weller, Michael, Dubbink, H J, French, Pim, Looman, Jim, Dey, Jyotirmoy, Krause, Scott, Ansell, Pete, Nuyens, Sarah, Spruyt, Maarten, Brilhante, Joana, Coens, Corneel, Gorlia, Thierry, Golfinopoulos, Vassilis, Van Den Bent, Martin, Eoli, Marica, Sepulveda, Juan Manuel, Smits, Marion, Walenkamp, Annemiek, Frenel, Jean-Sebastian, Franceschi, Enrico, Clement, Paul M, Chinot, Olivier, De Vos, Filip, Whenham, Nicolas, Sanghera, Paul, Weller, Michael, Dubbink, H J, French, Pim, Looman, Jim, Dey, Jyotirmoy, Krause, Scott, Ansell, Pete, Nuyens, Sarah, Spruyt, Maarten, Brilhante, Joana, Coens, Corneel, Gorlia, Thierry, and Golfinopoulos, Vassilis

Abstract

BACKGROUND: Depatuxizumab mafodotin (Depatux-M) is a tumor-specific antibody-drug conjugate consisting of an antibody (ABT-806) directed against activated epidermal growth factor receptor (EGFR) and the toxin monomethylauristatin-F. We investigated Depatux-M in combination with temozolomide or as a single agent in a randomized controlled phase II trial in recurrent EGFR amplified glioblastoma. METHODS: Eligible were patients with centrally confirmed EGFR amplified glioblastoma at first recurrence after chemo-irradiation with temozolomide. Patients were randomized to either Depatux-M 1.25 mg/kg every 2 weeks intravenously, or this treatment combined with temozolomide 150-200 mg/m2 day 1-5 every 4 weeks, or either lomustine or temozolomide. The primary endpoint of the study was overall survival. RESULTS: Two hundred sixty patients were randomized. In the primary efficacy analysis with 199 events (median follow-up 15.0 mo), the hazard ratio (HR) for the combination arm compared with the control arm was 0.71 (95% CI = 0.50, 1.02; P = 0.062). The efficacy of Depatux-M monotherapy was comparable to that of the control arm (HR = 1.04, 95% CI = 0.73, 1.48; P = 0.83). The most frequent toxicity in Depatux-M treated patients was a reversible corneal epitheliopathy, occurring as grades 3-4 adverse events in 25-30% of patients. In the long-term follow-up analysis with median follow-up of 28.7 months, the HR for the comparison of the combination arm versus the control arm was 0.66 (95% CI = 0.48, 0.93). CONCLUSION: This trial suggests a possible role for the use of Depatux-M in combination with temozolomide in EGFR amplified recurrent glioblastoma, especially in patients relapsing well after the end of first-line adjuvant temozolomide treatment. (NCT02343406).

Published
2020

17. Prognostic value of TERT promoter mutations in conjunctival melanomas in addition to clinicopathological features.

Author

van Ipenburg, J. A., Naus, N. C., Dubbink, H. J., van Ginderdeuren, R., Missotten, G. S., Paridaens, D., and Verdijk, R. M.

Abstract

Aims To evaluate the prognostic value of clinical, histopathological and molecular features and to relate different treatment modalities to clinical outcome in conjunctival melanomas (CM). Methods Retrospective review of clinical, histopathological and BRAF V600E and telomerase reverse transcriptase (TERT) promoter mutation status and treatment modalities, correlated to recurrence and metastasis in 79 patients with CM, diagnosed between 1987 and 2015 in three tertiary referral centres in the Netherlands and Belgium. Results Out of 78 evaluable patients, recurrences occurred in 16 patients and metastasis in 12 patients (median follow-up time 35 months (0-260 months)). Tumour thickness >2 mm, pT status, the presence of epithelioid cells, ulceration and mitoses was significantly correlated with metastasis (p value 0.046, 0.01, 0.02, 0.001 and 0.003, respectively). Furthermore, CM frequently harbour BRAF V600E and TERT promoter mutations (29% and 43%, respectively). TERT promoter mutations were correlated to shorter metastasis-free survival (p value 0.002). No significant correlation was found for clinical parameters and metastatic disease. Palpebral, forniceal and caruncular melanomas were more prone to develop recurrences (p value: 0.03). Most CM were treated with excision with adjuvant therapy. Conclusion In line with the recommendations in the Eighth Edition of the American Joint Committee on Cancer Staging for CM, the pathology report should include information about pT status, tumour thickness, presence of epithelioid cells, ulceration and mitoses. Furthermore, information about the presence of a TERT promoter mutation and BRAF V600E mutation is of interest for therapeutic decision making. The presence of a TERT promoter mutation is correlated to metastatic disease. [ABSTRACT FROM AUTHOR]

Published
2021
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18. INTELLANCE 2/EORTC 1410 randomized phase II study of Depatux-M alone and with temozolomide vs temozolomide or lomustine in recurrent EGFR amplified glioblastoma

Author

Van Den Bent, Martin, primary, Eoli, Marica, primary, Sepulveda, Juan Manuel, primary, Smits, Marion, primary, Walenkamp, Annemiek, primary, Frenel, Jean-Sebastian, primary, Franceschi, Enrico, primary, Clement, Paul M, primary, Chinot, Olivier, primary, De Vos, Filip, primary, Whenham, Nicolas, primary, Sanghera, Paul, primary, Weller, Michael, primary, Dubbink, H J, primary, French, Pim, primary, Looman, Jim, primary, Dey, Jyotirmoy, primary, Krause, Scott, primary, Ansell, Pete, primary, Nuyens, Sarah, primary, Spruyt, Maarten, primary, Brilhante, Joana, primary, Coens, Corneel, primary, Gorlia, Thierry, primary, and Golfinopoulos, Vassilis, primary

Published
2019
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21. INTELLANCE 2/EORTC 1410 randomized phase II study of Depatux-M alone and with temozolomide vs temozolomide or lomustine in recurrent EGFR amplified glioblastoma.

Author

Bent, Martin Van Den, Eoli, Marica, Sepulveda, Juan Manuel, Smits, Marion, Walenkamp, Annemiek, Frenel, Jean-Sebastian, Franceschi, Enrico, Clement, Paul M, Chinot, Olivier, Vos, Filip De, Whenham, Nicolas, Sanghera, Paul, Weller, Michael, Dubbink, H J, French, Pim, Looman, Jim, Dey, Jyotirmoy, Krause, Scott, Ansell, Pete, and Nuyens, Sarah

Published
2020
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22. MGMT promoter methylation is prognostic but not predictive for outcome to adjuvant PCV chemotherapy in anaplastic oligodendroglial tumors: A report from EORTC Brain Tumor Group Study 26951

Author

van den Bent M. J., Dubbink H. J., Sanson M., van der Lee-Haarloo C. R., Hegi M., Jeuken J. W., Ibdaih A., Brandes A. A., Taphoorn M. J., Frenay M., Lacombe D., Gorlia T., Dinjens W. N., and Kros J. M.

Subjects
neoplasms, digestive system diseases
Abstract

PURPOSE: O6 methylguanine methyltransferase (MGMT) promoter methylation has been shown to predict survival of patients with glioblastomas if temozolomide is added to radiotherapy (RT). It is unknown if MGMT promoter methylation is also predictive to outcome to RT followed by adjuvant procarbazine lomustine and vincristine (PCV) chemotherapy in patients with anaplastic oligodendroglial tumors (AOT). PATIENTS AND METHODS: In the European Organisation for the Research and Treatment of Cancer study 26951 368 patients with AOT were randomly assigned to either RT alone or to RT followed by adjuvant PCV. From 165 patients of this study formalin fixed paraffin embedded tumor tissue was available for MGMT promoter methylation analysis. This was investigated with methylation specific multiplex ligation dependent probe amplification. RESULTS: In 152 cases an MGMT result was obtained in 121 (80) cases MGMT promoter methylation was observed. Methylation strongly correlated with combined loss of chromosome 1p and 19q loss (P = .00043). In multivariate analysis MGMT promoter methylation 1p/19q codeletion tumor necrosis and extent of resection were independent prognostic factors. The prognostic significance of MGMT promoter methylation was equally strong in the RT arm and the RT/PCV arm for both progression free survival and overall survival. In tumors diagnosed at central pathology review as glioblastoma no prognostic effect of MGMT promoter methylation was observed. CONCLUSION: In this study on patients with AOT MGMT promoter methylation was of prognostic significance and did not have predictive significance for outcome to adjuvant PCV chemotherapy. The biologic effect of MGMT promoter methylation or pathogenetic features associated with MGMT promoter methylation may be different for AOT compared with glioblastoma.

Published
2009

23. Evaluation of current prediction models for Lynch syndrome: updating the PREMM5 model to identify PMS2 mutation carriers

Author

Goverde, A., primary, Spaander, M. C. W., additional, Nieboer, D., additional, van den Ouweland, A. M. W., additional, Dinjens, W. N. M., additional, Dubbink, H. J., additional, Tops, C. J., additional, ten Broeke, S. W., additional, Bruno, M. J., additional, Hofstra, R. M. W., additional, Steyerberg, E. W., additional, and Wagner, A., additional

Published
2017
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24. Prognostic value of TERTpromoter mutations in conjunctival melanomas in addition to clinicopathological features

Author

van Ipenburg, J A, Naus, N C, Dubbink, H J, van Ginderdeuren, R, Missotten, G S, Paridaens, D, and Verdijk, R M

Abstract

AimsTo evaluate the prognostic value of clinical, histopathological and molecular features and to relate different treatment modalities to clinical outcome in conjunctival melanomas (CM).MethodsRetrospective review of clinical, histopathological and BRAFV600E and telomerase reverse transcriptase (TERT) promoter mutation status and treatment modalities, correlated to recurrence and metastasis in 79 patients with CM, diagnosed between 1987 and 2015 in three tertiary referral centres in the Netherlands and Belgium.ResultsOut of 78 evaluable patients, recurrences occurred in 16 patients and metastasis in 12 patients (median follow-up time 35 months (0–260 months)). Tumour thickness >2 mm, pT status, the presence of epithelioid cells, ulceration and mitoses was significantly correlated with metastasis (p value 0.046, 0.01, 0.02, 0.001 and 0.003, respectively). Furthermore, CM frequently harbour BRAFV600E and TERTpromoter mutations (29% and 43%, respectively). TERTpromoter mutations were correlated to shorter metastasis-free survival (p value 0.002). No significant correlation was found for clinical parameters and metastatic disease. Palpebral, forniceal and caruncular melanomas were more prone to develop recurrences (p value: 0.03). Most CM were treated with excision with adjuvant therapy.ConclusionIn line with the recommendations in the Eighth Edition of the American Joint Committee on Cancer Staging for CM, the pathology report should include information about pT status, tumour thickness, presence of epithelioid cells, ulceration and mitoses. Furthermore, information about the presence of a TERTpromoter mutation and BRAFV600E mutation is of interest for therapeutic decision making. The presence of a TERTpromoter mutation is correlated to metastatic disease.

Published
2021
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25. Evaluation of current prediction models for Lynch syndrome: updating the PREMM5 model to identify PMS2 mutation carriers.

Author

Goverde, A., Spaander, M. C. W., Nieboer, D., van den Ouweland, A. M. W., Dinjens, W. N. M., Dubbink, H. J., Tops, C. J., ten Broeke, S. W., Bruno, M. J., Hofstra, R. M. W., Steyerberg, E. W., and Wagner, A.

Abstract

Until recently, no prediction models for Lynch syndrome (LS) had been validated for PMS2 mutation carriers. We aimed to evaluate MMRpredict and PREMM5 in a clinical cohort and for PMS2 mutation carriers specifically. In a retrospective, clinic-based cohort we calculated predictions for LS according to MMRpredict and PREMM5. The area under the operator receiving characteristic curve (AUC) was compared between MMRpredict and PREMM5 for LS patients in general and for different LS genes specifically. Of 734 index patients, 83 (11%) were diagnosed with LS; 23 MLH1, 17 MSH2, 31 MSH6 and 12 PMS2 mutation carriers. Both prediction models performed well for MLH1 and MSH2 (AUC 0.80 and 0.83 for PREMM5 and 0.79 for MMRpredict) and fair for MSH6 mutation carriers (0.69 for PREMM5 and 0.66 for MMRpredict). MMRpredict performed fair for PMS2 mutation carriers (AUC 0.72), while PREMM5 failed to discriminate PMS2 mutation carriers from non-mutation carriers (AUC 0.51). The only statistically significant difference between PMS2 mutation carriers and non-mutation carriers was proximal location of colorectal cancer (77 vs. 28%, p < 0.001). Adding location of colorectal cancer to PREMM5 considerably improved the models performance for PMS2 mutation carriers (AUC 0.77) and overall (AUC 0.81 vs. 0.72). We validated these results in an external cohort of 376 colorectal cancer patients, including 158 LS patients. MMRpredict and PREMM5 cannot adequately identify PMS2 mutation carriers. Adding location of colorectal cancer to PREMM5 may improve the performance of this model, which should be validated in larger cohorts. [ABSTRACT FROM AUTHOR]

Published
2018
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26. 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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27. RESULTS OF THE INTERNATIONAL INTERLABORATORY COMPARISON OF MGMT PROMOTER METHYLATION ANALYSIS INVOLVING TWENTY-THREE ACADEMIC CENTERS IN GERMANY, AUSTRIA AND THE NETHERLANDS

Author

Reifenberger, G., primary, Malzkorn, B., additional, Acker, T., additional, Bettstetter, M., additional, Buslei, R., additional, von Deimling, A., additional, Dietmaier, W., additional, Dubbink, H. J., additional, Eigenbrod, S., additional, Garvalov, B. K., additional, Gerstenmaier, U., additional, Giese, A., additional, Haase, D., additional, Hasselblatt, M., additional, Kirches, E., additional, Koch, A., additional, Marienfeld, R., additional, Mittelbronn, M., additional, Montesinos-Rongen, M., additional, Pagenstecher, A., additional, Riemenschneider, M. J., additional, Prinz, M., additional, Romeike, B., additional, Roos, A., additional, Spiegl-Kreinecker, S., additional, Schittenhelm, J., additional, Schlegel, J., additional, Thal, D. R., additional, Tops, B. B. J., additional, Weis, J., additional, Westphal, G., additional, Worm, K., additional, and Felsberg, J., additional

Published
2014
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28. CLIN-PATHOLOGY

Author

Alexandru, D., primary, Satyadev, R., additional, So, W., additional, Lee, S. H., additional, Lee, Y. S., additional, Hong, Y.-K., additional, Kang, C. S., additional, Rodgers, S. D., additional, Marascalchi, B. J., additional, Strom, R. G., additional, Riina, H., additional, Samadani, U., additional, Frempong-Boadu, A., additional, Babu, R., additional, Sen, C., additional, Zagzag, D., additional, Anderson, M. D., additional, Abel, T. W., additional, Moots, P. L., additional, Odia, Y., additional, Orr, B. A., additional, Eberhart, C. G., additional, Rodriguez, F., additional, Sweis, R. T., additional, Lavingia, J., additional, Connelly, J., additional, Cochran, E., additional, van den Bent, M., additional, Hartmann, C., additional, Preusser, M., additional, Strobel, T., additional, Dubbink, H. J., additional, Kros, J. M., additional, von Deimling, A., additional, Boisselier, B., additional, Sanson, M., additional, Halling, K. C., additional, Diefes, K. L., additional, Aldape, K., additional, Giannini, C., additional, Rodriguez, F. J., additional, Ligon, A. H., additional, Horkayne-Szakaly, I., additional, Rushing, E. J., additional, Ligon, K. L., additional, Vena, N., additional, Garcia, D. I., additional, Douglas Cameron, J., additional, Raghunathan, A., additional, Wani, K., additional, Armstrong, T. S., additional, Vera-Bolanos, E., additional, Fouladi, M., additional, Gajjar, A., additional, Goldman, S., additional, Lehman, N. L., additional, Metellus, P., additional, Mikkelsen, T., additional, Necesito-Reyes, M. J. T., additional, Omuro, A., additional, Packer, R. J., additional, Partap, S., additional, Pollack, I. F., additional, Prados, M. D., additional, Ian Robbins, H., additional, Soffietti, R., additional, Wu, J., additional, Gilbert, M. R., additional, Aldape, K. D., additional, Prosniak, M., additional, Harshyne, L. A., additional, Andrews, D. W., additional, Craig Hooper, D., additional, Kagawa, N., additional, Hosen, N., additional, Kijima, N., additional, Hirayama, R., additional, Chiba, Y., additional, Yamamoto, F., additional, Kinoshita, M., additional, Hashimoto, N., additional, Fujimoto, Y., additional, Yoshimine, T., additional, Hu, J., additional, Nuno, M., additional, Patil, C., additional, Rudnick, J., additional, Phuphanich, S., additional, Bannykh, S., additional, Chu, R., additional, Yu, J., additional, Black, K., additional, Choi, J., additional, Kim, D., additional, Shim, K. W., additional, Kim, S. H., additional, Kanno, H., additional, Nishihara, H., additional, Tanaka, S., additional, Yanagi, T., additional, Buczkowicz, P., additional, Khuong-Quang, D.-A., additional, Rakopoulos, P., additional, Bouffet, E., additional, Morrison, A., additional, Bartels, U., additional, Pfister, S. M., additional, Jabado, N., additional, Hawkins, C., additional, Weinberg, B. D., additional, Newell, K. L., additional, Kumar, P., additional, Wang, F., additional, Venneti, S., additional, Madden, M., additional, Coyne, T., additional, Phillips, J., additional, Gorovets, D., additional, Huse, J., additional, Kofler, J., additional, Lu, C., additional, Tihan, T., additional, Sullivan, L., additional, Santi, M., additional, Judkins, A., additional, Thompson, C., additional, Perry, A., additional, Iorgulescu, J. B., additional, Laufer, I., additional, Hameed, M., additional, Lis, E., additional, Boland, P., additional, Komotar, R., additional, Bilsky, M., additional, Amato-Watkins, A. C., additional, Neal, J., additional, Rees, A. D., additional, Davies, J. S., additional, Hayhurst, C., additional, Lu-Emerson, C., additional, Snuderl, M., additional, Davidson, C., additional, Kirkpatrick, N. D., additional, Huang, Y., additional, Duda, D. G., additional, Ancukiewicz, M., additional, Stemmer-Rachamimov, A., additional, Batchelor, T. T., additional, Jain, R. K., additional, Ellezam, B., additional, Theeler, B. J., additional, Sadighi, Z. S., additional, Mehta, V., additional, Tran, M.-D. T., additional, Adesina, A. M., additional, Puduvalli, V. K., additional, and Bruner, J. M., additional

Published
2012
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29. IDH1 mutations in low-grade astrocytomas predict survival but not response to temozolomide

Author

Dubbink, H. J., primary, Taal, W., additional, van Marion, R., additional, Kros, J. M., additional, van Heuvel, I., additional, Bromberg, J. E., additional, Zonnenberg, B. A., additional, Zonnenberg, C.B.L., additional, Postma, T. J., additional, Gijtenbeek, J. M.M., additional, Boogerd, W., additional, Groenendijk, F. H., additional, Smitt, P. A.E. Sillevis, additional, Dinjens, W. N.M., additional, and van den Bent, M. J., additional

Published
2009
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30. IDH1mutations in low-grade astrocytomas predict survival but not response to temozolomide

Author

Dubbink, H J., Taal, W, van Marion, R, Kros, J M., van Heuvel, I, Bromberg, J E., Zonnenberg, B A., Zonnenberg, C B.L., Postma, T J., Gijtenbeek, J M.M., Boogerd, W, Groenendijk, F H., Smitt, P A.E. Sillevis, Dinjens, W N.M., and Bent, M J. van den

Abstract

Mutations in isocitrate dehydrogenase 1 and 2 (IDH1and IDH2) have been implicated in tumorigenesis of gliomas. Patients with high-grade astrocytomas with IDH1or IDH2mutations were reported to have a better survival, but it is unknown if this improved survival also holds for low-grade astrocytoma and whether these mutations predict outcome to specific treatment.

Published
2009
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33. 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., Oosterkamp, H. M., Walenkamp, A. M. E., Dubbink, H. J., Beerepoot, L. V., Hanse, M., Buter, J., Honkoop, A., Boerman, D., Vos, F. Y. F., Dinjens, W. N. M., Enting, R. H., Taphoorn, M. J. B., van den Berkmortel, F. W. P. J., Jansen, R., Brandsma, D., Bromberg, J. E., van Heuvel, I., Vernhout, R. M., van der Holt, B., van den Bent, M. J., and Guided Treatment in Optimal Selected Cancer Patients (GUTS)

34. Molecular Tumor Board of the University Medical Center Groningen (UMCG-MTB): outcome of patients with rare or complex mutational profiles receiving MTB-advised targeted therapy.

Author

de Jager VD, Plomp P, Paats MS, van Helvert S, Elst AT, van den Berg A, Dubbink HJ, van Geffen WH, Zhang L, Hendriks LEL, Hiltermann TJN, Hiddinga BI, Hijmering-Kappelle LBM, Jalving M, Kluiver J, Koopman B, van Kruchten M, van der Logt EMJ, Piet B, van Putten J, Reitsma BH, Rutgers SR, de Vries M, Stigt JA, Groves MR, Timens W, Willems SM, van Kempen LC, Schuuring E, and van der Wekken AJ

Subjects
Humans, Retrospective Studies, Male, Female, Middle Aged, Aged, Academic Medical Centers, Follow-Up Studies, Adult, Treatment Outcome, Aged, 80 and over, Neoplasms drug therapy, Neoplasms genetics, Mutation, Molecular Targeted Therapy methods
Abstract

Purpose: Molecular tumor boards (MTBs) are considered beneficial for treatment decision making for patients with cancer with uncommon, rare, or complex mutational profiles. The lack of international MTB guidelines results in significant variation in practices and recommendations. Therefore, periodic follow-up is necessary to assess and govern MTB functioning. The objective of this study was to determine the effectiveness of MTB treatment recommendations for patients with rare and complex mutational profiles as implemented in the MTB of the University Medical Center Groningen (UMCG-MTB) in 2019-2020., Patients and Methods: A retrospective follow-up study was carried out to determine the clinical outcome of patients with uncommon or rare (combinations of) molecular aberrations for whom targeted therapy was recommended as the next line of treatment by the UMCG-MTB in 2019 and 2020., Results: The UMCG-MTB recommended targeted therapy as the next line of treatment in 132 of 327 patients: 37 in clinical trials, 67 in the on-label setting, and 28 in the off-label setting. For on- and off-label treatment recommendations, congruence of recommended and received treatment was 85% in patients with available follow-up (67/79). Treatment with on-label therapy resulted in a response rate of 50% (21/42), a median progression-free survival (PFS) of 6.3 months [interquartile range (IQR) 2.9-14.9 months], and median overall survival (OS) of 15.8 months (IQR 6.4-34.2 months). Treatment with off-label therapy resulted in a response rate of 53% (8/15), a median PFS of 5.1 months (IQR 1.9-7.3 months), and a median OS of 17.7 months (IQR 5.1-23.7 months)., Conclusion: Treatment with MTB-recommended next-line targeted therapy for patients with often heavily pretreated cancer with rare and complex mutational profiles resulted in positive overall responses in over half of patients. Off-label use of targeted therapies, for which there is sufficient rationale as determined by an MTB, is an effective treatment strategy. This study underlines the relevance of discussing patients with rare and complex mutational profiles in an MTB., (Copyright © 2024 The Authors. Published by Elsevier Ltd.. All rights reserved.)

Published
2024
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35. Molecular alterations and potential actionable mutations in peritoneal mesothelioma: a scoping review of high-throughput sequencing studies.

Author

Dietz MV, van Kooten JP, Paats MS, Aerts JGVJ, Verhoef C, Madsen EVE, Dubbink HJ, and von der Thüsen JH

Subjects
Humans, Mutation, High-Throughput Nucleotide Sequencing methods, Lung Neoplasms genetics, Mesothelioma, Malignant genetics, Mesothelioma genetics, Mesothelioma pathology, Peritoneal Neoplasms genetics, Peritoneal Neoplasms pathology
Abstract

Background: Peritoneal mesothelioma (PeM) is a rare malignancy with a poor prognosis. Currently there is a lack of effective systemic therapies. Due to the rarity of PeM, it is challenging to study new treatment options. Off-label use of targeted drugs could be an effective approach. This scoping review aims to explore the genomic landscape of PeM to identify potential therapeutic targets., Materials and Methods: A systematic literature search of Embase, Medline, Web of Science, the Cochrane Library, and Google Scholar was carried out up to 1 November 2022. Studies that reported on molecular alterations in PeM detected by high-throughput sequencing techniques were included. Genes that were altered in ≥1% of PeMs were selected for the identification of potential targeted therapies., Results: Thirteen articles were included, comprising 824 PeM patients. In total, 142 genes were altered in ≥1% of patients, of which 7 genes were altered in ≥10%. BAP1 was the most commonly altered gene (50%). Other commonly altered genes were NF2 (25%), CDKN2A (23%), CDKN2B (17%), PBRM1 (15%), TP53 (14%), and SETD2 (13%). In total, 17% of PeM patients were carriers of a germline mutation, mainly in BAP1 (7%)., Conclusions: This scoping review provides an overview of the mutational landscape of PeM. Germline mutations might be a larger contributor to the incidence of PeM than previously thought. Currently available targeted therapy options are limited, but several targeted agents [such as poly (ADP-ribose) polymerase (PARP), enhancer of zeste homolog 2 (EZH2), and cyclin-dependent kinase 4/6 (CDK4/6) inhibitors] were identified that might provide new targeted therapy options in the future., (Copyright © 2023 The Author(s). Published by Elsevier Ltd.. All rights reserved.)

Published
2023
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36. Recommendations on scuba diving in Birt-Hogg-Dubé syndrome.

Author

van Riel L, van Hulst RA, van Hest L, van Moorselaar R, Boerrigter BG, Franken SM, Wolthuis R, Dubbink HJ, Marciniak SJ, Gupta N, van de Beek I, and Houweling AC

Subjects
Humans, Tumor Suppressor Proteins genetics, Birt-Hogg-Dube Syndrome diagnosis, Birt-Hogg-Dube Syndrome genetics, Birt-Hogg-Dube Syndrome complications, Diving adverse effects, Pneumothorax genetics, Lung Diseases etiology, Lung Injury, Cysts genetics, Cysts pathology, Barotrauma diagnosis, Barotrauma complications
Abstract

Introduction: Although very uncommon, severe injury and death can occur during scuba diving. One of the main causes of scuba diving fatalities is pulmonary barotrauma due to significant changes in ambient pressure. Pathology of the lung parenchyma, such as cystic lesions, might increase the risk of pulmonary barotrauma., Areas Covered: Birt-Hogg-Dubé syndrome (BHD), caused by pathogenic variants in the FLCN gene, is characterized by skin fibrofolliculomas, an increased risk of renal cell carcinoma, multiple lung cysts and spontaneous pneumothorax. Given the pulmonary involvement, in some countries patients with BHD are generally recommended to avoid scuba diving, although evidence-based guidelines are lacking. We aim to provide recommendations on scuba diving for patients with BHD, based on a survey of literature on pulmonary cysts and pulmonary barotrauma in scuba diving., Expert Opinion: In our opinion, although the absolute risks are likely to be low, caution is warranted. Given the relative paucity of literature and the potential fatal outcome, patients with BHD with a strong desire for scuba diving should be informed of the potential risks in a personal assessment. If available a diving physician should be consulted, and a low radiation dose chest computed tomography (CT)-scan to assess pulmonary lesions could be considered.

Published
2023
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37. Corrigendum to INTELLANCE 2/EORTC 1410 randomized phase II study of Depatux-M alone and with temozolomide vs temozolomide or lomustine in recurrent EGFR amplified glioblastoma.

Author

van den Bent M, Eoli M, Sepulveda JM, Smits M, Walenkamp A, Frenel JS, Franceschi E, Clement PM, Chinot O, de Vos F, Whenham N, Sanghera P, Weller M, Dubbink HJ, French P, Looman J, Dey J, Krause S, Ansell P, Nuyens S, Spruyt M, Brilhante J, Coens C, Gorlia T, and Golfinopoulos V

Published
2021
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38. RET Fluorescence In Situ Hybridization Analysis Is a Sensitive but Highly Unspecific Screening Method for RET Fusions in Lung Cancer.

Author

Radonic T, Geurts-Giele WRR, Samsom KG, Roemen GMJM, von der Thüsen JH, Thunnissen E, Meijssen IC, Sleddens HFBM, Dinjens WNM, Boelens MC, Weijers K, Speel EJM, Finn SP, O'Brien C, van Wezel T, Cohen D, Monkhorst K, Roepman P, and Dubbink HJ

Subjects
Anaplastic Lymphoma Kinase genetics, Early Detection of Cancer, Gene Rearrangement, Humans, In Situ Hybridization, Fluorescence, Oncogene Proteins, Fusion genetics, Proto-Oncogene Proteins genetics, Proto-Oncogene Proteins c-ret genetics, Lung Neoplasms genetics, Protein-Tyrosine Kinases genetics
Abstract

Introduction: RET gene fusions are established oncogenic drivers in 1% of NSCLC. Accurate detection of advanced patients with RET fusions is essential to ensure optimal therapy choice. We investigated the performance of fluorescence in situ hybridization (FISH) as a diagnostic test for detecting functional RET fusions., Methods: Between January 2016 and November 2019, a total of 4873 patients with NSCLC were routinely screened for RET fusions using either FISH (n = 2858) or targeted RNA next-generation sequencing (NGS) (n = 2015). If sufficient material was available, positive cases were analyzed by both methods (n = 39) and multiple FISH assays (n = 17). In an independent cohort of 520 patients with NSCLC, whole-genome sequencing data were investigated for disruptive structural variations and functional fusions in the RET and compared with ALK and ROS1 loci., Results: FISH analysis revealed RET rearrangement in 48 of 2858 cases; of 30 rearranged cases double tested with NGS, only nine had a functional RET fusion. RNA NGS yielded RET fusions in 14 of 2015 cases; all nine cases double tested by FISH had RET locus rearrangement. Of these 18 verified RET fusion cases, 16 had a split signal and two a complex rearrangement by FISH. By whole-genome sequencing, the prevalence of functional fusions compared with all disruptive events was lower in the RET (4 of 9, 44%) than the ALK (27 of 34, 79%) and ROS1 (9 of 12, 75%) loci., Conclusions: FISH is a sensitive but unspecific technique for RET screening, always requiring a confirmation using an orthogonal technique, owing to frequently occurring RET rearrangements not resulting in functional fusions in NSCLC., (Copyright © 2021 International Association for the Study of Lung Cancer. Published by Elsevier Inc. All rights reserved.)

Published
2021
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39. INTELLANCE 2/EORTC 1410 randomized phase II study of Depatux-M alone and with temozolomide vs temozolomide or lomustine in recurrent EGFR amplified glioblastoma.

Author

Van Den Bent M, Eoli M, Sepulveda JM, Smits M, Walenkamp A, Frenel JS, Franceschi E, Clement PM, Chinot O, De Vos F, Whenham N, Sanghera P, Weller M, Dubbink HJ, French P, Looman J, Dey J, Krause S, Ansell P, Nuyens S, Spruyt M, Brilhante J, Coens C, Gorlia T, and Golfinopoulos V

Subjects
Antibodies, Monoclonal, Humanized, Antineoplastic Agents, Alkylating therapeutic use, ErbB Receptors genetics, Humans, Lomustine therapeutic use, Temozolomide therapeutic use, Brain Neoplasms drug therapy, Glioblastoma drug therapy
Abstract

Background: Depatuxizumab mafodotin (Depatux-M) is a tumor-specific antibody-drug conjugate consisting of an antibody (ABT-806) directed against activated epidermal growth factor receptor (EGFR) and the toxin monomethylauristatin-F. We investigated Depatux-M in combination with temozolomide or as a single agent in a randomized controlled phase II trial in recurrent EGFR amplified glioblastoma., Methods: Eligible were patients with centrally confirmed EGFR amplified glioblastoma at first recurrence after chemo-irradiation with temozolomide. Patients were randomized to either Depatux-M 1.25 mg/kg every 2 weeks intravenously, or this treatment combined with temozolomide 150-200 mg/m2 day 1-5 every 4 weeks, or either lomustine or temozolomide. The primary endpoint of the study was overall survival., Results: Two hundred sixty patients were randomized. In the primary efficacy analysis with 199 events (median follow-up 15.0 mo), the hazard ratio (HR) for the combination arm compared with the control arm was 0.71 (95% CI = 0.50, 1.02; P = 0.062). The efficacy of Depatux-M monotherapy was comparable to that of the control arm (HR = 1.04, 95% CI = 0.73, 1.48; P = 0.83). The most frequent toxicity in Depatux-M treated patients was a reversible corneal epitheliopathy, occurring as grades 3-4 adverse events in 25-30% of patients. In the long-term follow-up analysis with median follow-up of 28.7 months, the HR for the comparison of the combination arm versus the control arm was 0.66 (95% CI = 0.48, 0.93)., Conclusion: This trial suggests a possible role for the use of Depatux-M in combination with temozolomide in EGFR amplified recurrent glioblastoma, especially in patients relapsing well after the end of first-line adjuvant temozolomide treatment. (NCT02343406)., (© The Author(s) 2019. Published by Oxford University Press on behalf of the Society for Neuro-Oncology.)

Published
2020
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40. Highly accurate DNA-based detection and treatment results of MET exon 14 skipping mutations in lung cancer.

Author

Pruis MA, Geurts-Giele WRR, von der TJH, Meijssen IC, Dinjens WNM, Aerts JGJV, Dingemans AMC, Lolkema MP, Paats MS, and Dubbink HJ

Subjects
Adenocarcinoma of Lung drug therapy, Adenocarcinoma of Lung genetics, Aged, Aged, 80 and over, Carcinoma, Non-Small-Cell Lung drug therapy, Carcinoma, Non-Small-Cell Lung genetics, Crizotinib therapeutic use, DNA, Neoplasm analysis, Diagnostic Tests, Routine, Female, Follow-Up Studies, High-Throughput Nucleotide Sequencing, Humans, Lung Neoplasms drug therapy, Lung Neoplasms genetics, Male, Middle Aged, Prognosis, Protein Kinase Inhibitors therapeutic use, Proto-Oncogene Proteins c-met antagonists & inhibitors, Retrospective Studies, Survival Rate, Adenocarcinoma of Lung pathology, Biomarkers, Tumor genetics, Carcinoma, Non-Small-Cell Lung pathology, DNA, Neoplasm genetics, Exons, Lung Neoplasms pathology, Mutation, Proto-Oncogene Proteins c-met genetics
Abstract

Objectives: The oncogenic MET exon 14 skipping mutation (METex14del) is described to drive 1.3 %-5.7 % of non-small-cell lung cancer (NSCLC) and multiple studies with cMET inhibitors show promising clinical responses. RNA-based analysis seems most optimal for METex14del detection, however, acquiring sufficient RNA material is often problematic. An alternative is DNA-based analysis, but commercially available DNA-based panels only detect up to 63 % of known METex14del alterations. The goal of this study is to describe an optimized DNA-based diagnostic test for METex14del in NSCLC, including clinical features and follow-up of patients treated with cMET-targeted therapy and consequent resistance mechanisms., Material and Methods: Routinely processed diagnostic pathology non-squamous NSCLC specimens were investigated by a custom-made DNA-based targeted amplicon-based next generation sequencing (NGS) panel, which includes 4 amplicons for METex14del detection. Retrospectively, histopathological characteristics and clinical follow up were investigated for advanced non-squamous NSCLC with METex14del., Results: In silico analysis showed that our NGS panel is able to detect 96 % of reported METex14 alterations. METex14del was found in 2 % of patients with non-squamous NSCLC tested for therapeutic purposes. In total, from May 2015 - Sep 2018, METex14del was found in 46 patients. Thirty-six of these patients had advanced non-squamous NSCLC, they were predominantly elderly (76.5 years [53-90]), male (25/36) and (ex)-smokers (23/36). Five patients received treatment with crizotinib (Pfizer Oncology), in a named patient based program, disease control was achieved for 4/5 patients (3 partial responses, 1 stable disease) and one patient had a mixed response. Two patients developed a MET D1228N mutation during crizotinib treatment, inducing a resistance mechanism to crizotinib., Conclusions: This study shows that METex14del can be reliably detected by routine DNA NGS analysis. Although a small cohort, patients responded well to targeted treatment, underlining the need for routine testing of METex14del in advanced non-squamous NSCLC to guarantee optimal personalized treatment., (Copyright © 2019 The Authors. Published by Elsevier B.V. All rights reserved.)

Published
2020
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41. Granular dot-like staining with MLH1 immunohistochemistry is a clone-dependent artefact.

Author

Dasgupta S, Ewing-Graham PC, Groenendijk FH, Stam O, Biermann KE, Doukas M, Dubbink HJ, van Velthuysen MF, Dinjens WNM, and Van Bockstal MR

Subjects
Biomarkers, Tumor metabolism, Colorectal Neoplasms, Hereditary Nonpolyposis diagnosis, Endometrial Neoplasms diagnosis, Female, Humans, Immunohistochemistry methods, Promoter Regions, Genetic genetics, Colorectal Neoplasms, Hereditary Nonpolyposis metabolism, Endometrial Neoplasms metabolism, Genetic Predisposition to Disease genetics, MutL Protein Homolog 1 metabolism
Abstract

Immunohistochemistry (IHC) for DNA mismatch repair proteins MLH1, PMS2, MSH2, and MSH6 is used for microsatellite instability (MSI) screening in colorectal carcinoma (CRC) and endometrial carcinoma (EC). Loss of PMS2, with retained MLH1 staining occurs in germline mutations of PMS2 gene, and is an indication for genetic testing. We report a pitfall of immunohistochemical interpretation in an EC, initially regarded as MLH1-positive and PMS2-negative. Review of the MLH1-IHC (M1-clone) revealed a granular, dot-like, nuclear staining. On repeating the MLH1-IHC with a different clone (ES05-clone), complete negativity was noted, and on molecular testing, MLH1 promotor methylation was detected. The dot-like pattern was therefore adjudged a clone-dependent artefact. On reviewing the archived MLH1-IHC slides, we observed the same dot-like pattern in two CRCs; in both cases the M1-clone had been used. Awareness of this artefact may prevent reporting errors, and unnecessary referrals for germline mutation testing., (Copyright © 2019 Elsevier GmbH. All rights reserved.)

Published
2020
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42. Functional analysis of novel androgen receptor mutations in a unique cohort of Indonesian patients with a disorder of sex development.

Author

Elfferich P, Juniarto AZ, Dubbink HJ, van Royen ME, Molier M, Hoogerbrugge J, Houtsmuller AB, Trapman J, Santosa A, de Jong FH, Drop SL, Faradz SM, Bruggenwirth H, and Brinkmann AO

Subjects
Androgen-Insensitivity Syndrome genetics, Child, Child, Preschool, Humans, Indonesia, Male, Disorders of Sex Development genetics, Mutation genetics, Receptors, Androgen genetics
Abstract

Mutations in the androgen receptor (AR) gene, rendering the AR protein partially or completely inactive, cause androgen insensitivity syndrome, which is a form of a 46,XY disorder of sex development (DSD). We present 3 novel AR variants found in a cohort of Indonesian DSD patients: p.I603N, p.P671S, and p.Q738R. The aim of this study was to determine the possible pathogenic nature of these newly found unclassified variants. To investigate the effect of these variants on AR function, we studied their impact on transcription activation, AR ligand-binding domain interaction with an FxxLF motif containing peptide, AR subcellular localization, and AR nuclear dynamics and DNA-binding. AR-I603N had completely lost its transcriptional activity due to disturbed DNA-binding capacity and did not show the 114-kDa hyperphosphorylated AR protein band normally detectable after hormone binding. The patient with AR-I603N displays a partial androgen insensitivity syndrome phenotype, which is explained by somatic mosaicism. A strongly reduced transcriptional activity was observed for AR-Q738R, together with diminished interaction with an FxxLF motif containing peptide. AR-P671S also showed reduced transactivation ability, but no change in DNA- or FxxLF-binding capacity and interferes with transcriptional activity for as yet unclear reasons., (Copyright 2009 S. Karger AG, Basel.)

Published
2009
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43. An Sp1 binding site is essential for basal activity of the human prostate-specific transglutaminase gene (TGM4) promoter.

Author

Dubbink HJ, Cleutjens KB, van der Korput HA, Trapman J, and Romijn JC

Subjects
Base Sequence, Binding Sites genetics, Binding, Competitive, DNA genetics, DNA metabolism, DNA-Binding Proteins metabolism, Electrophoresis, Polyacrylamide Gel, Humans, Luciferases genetics, Luciferases metabolism, Male, Molecular Sequence Data, Mutation, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Sequence Deletion, Sp3 Transcription Factor, Transcription Factors metabolism, Transglutaminases chemistry, Transglutaminases metabolism, Tumor Cells, Cultured, Promoter Regions, Genetic genetics, Prostate enzymology, Sp1 Transcription Factor metabolism, Transglutaminases genetics
Abstract

Human prostate-specific transglutaminase (hTG(P)) is a cross-linking enzyme encoded by the TGM4 gene. The TGM4 gene promoter was characterized by deletion mapping and mutational analysis. Promoter constructs, containing the minimal promoter requirements, could efficiently drive transcription in the prostate cancer cell lines PC346C and LNCaP and the hepatic cancer cell line Hep3B. The region between positions -113 and -61 was demonstrated to be essential for core promoter activity. Further analysis revealed the functional importance of an Sp1 binding motif, 5'-ACCCCGCCCC-3', at positions -96 to -87. This sequence is a binding site of the ubiquitous transcription factors Sp1 and Sp3.

Published
1999
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44. Human prostate-specific transglutaminase: a new prostatic marker with a unique distribution pattern.

Author

Dubbink HJ, Hoedemaeker RF, van der Kwast TH, Schröder FH, and Romijn JC

Subjects
Biomarkers, Biopsy, Needle, Blotting, Western, Body Fluids enzymology, Humans, Immunohistochemistry, Male, Prostate pathology, Reference Values, Semen enzymology, Seminal Vesicles enzymology, Tissue Distribution, Androgen-Binding Protein metabolism, Prostate enzymology
Abstract

Human prostate-specific transglutaminase (hTGp) is a cross-linking enzyme, the physiologic function of which has not been established unequivocally yet. To gain insight into its distribution, we raised antisera against hTGp. By using Western blotting analysis, we found that these antisera specifically recognize a 77-kDa protein in prostatic fluids, seminal plasmas, and prostatic tissues. The concentrations of hTGp in these fluids and tissues were found to be highly variable among individuals. Immunohistochemical examination of several formalin-fixed paraffin-embedded human tissues revealed an exclusive expression in the prostate. The histologic localization and distribution of hTGp within the prostate was assessed by studying multiple sections from tumor-containing prostatectomy specimens and needle biopsies. hTGp expression was entirely restricted to luminal epithelial cells. No basal epithelial cells or stromal cells were stained. Within the prostate, large areas without any hTGp-positive cells were seen. Immunopositive cells were present either in a scattered pattern or concentrated in single or multiple glands in which all luminal epithelial cells expressed hTGp. The latter staining pattern occurred frequently, but not exclusively, in the peripheral zone, whereas scattered expression was most often observed in the transitional zone. Expression of the hTGp protein could occasionally be observed in high-grade prostatic intraepithelial neoplasia, but was not detected in prostate carcinoma cells. The expression pattern as observed for hTGp has not been found thus far for any other prostate-specific marker.

Published
1999

45. The human prostate-specific transglutaminase gene (TGM4): genomic organization, tissue-specific expression, and promoter characterization.

Author

Dubbink HJ, de Waal L, van Haperen R, Verkaik NS, Trapman J, and Romijn JC

Subjects
Amino Acid Sequence, Base Sequence, Exons genetics, Genes, Reporter genetics, Humans, Introns genetics, Male, Molecular Sequence Data, Peptidylprolyl Isomerase chemistry, Protein Biosynthesis genetics, Pseudogenes genetics, RNA Splicing genetics, RNA, Messenger metabolism, Sequence Analysis, DNA, Transcription, Genetic genetics, Transfection genetics, Transglutaminases chemistry, Tumor Cells, Cultured, Gene Expression Regulation, Enzymologic genetics, Promoter Regions, Genetic genetics, Prostate enzymology, Transglutaminases genetics
Abstract

Human prostate-specific transglutaminase (hTGP) is a cross-linking enzyme secreted by the prostate. In this study, we performed dot blot analysis of 50 normal human tissues to demonstrate unambiguously the prostate-specific expression of hTGP. Furthermore, we elucidated the genomic organization of the TGM4 gene, the gene encoding hTGP. The structure of this gene displays striking similarity to that of other transglutaminase (TGase) genes. The TGM4 gene spans approximately 35 kb of genomic DNA and consists of 13 exons and 12 introns. The main transcription initiation site is located 52 bp upstream of the translational start codon. A hTGP splice variant of intron 1 was detected. This splice variant contains an in-frame antisense Alu element insertion. The TGM4 promoter was analyzed by sequencing and transfection experiments. At positions -1276 to -563, the promoter harbors a cyclophilin pseudogene with 94% similarity to the cyclophilin A cDNA. Deletion mapping of the TGM4 promoter in the transiently transfected human prostate cancer cell line PC346C showed comparable activity of 2.1-, 1.5-, and 0.5-kb promoter fragments., (Copyright 1998 Academic Press.)

Published
1998
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46. The aroA gene of Campylobacter jejuni.

Author

Wösten MM, Dubbink HJ, and van der Zeijst BA

Subjects
3-Phosphoshikimate 1-Carboxyvinyltransferase, Amino Acid Sequence, Base Sequence, Campylobacter jejuni genetics, Chromosomes, Bacterial, Cloning, Molecular, DNA, Bacterial, Genes, Bacterial, Molecular Sequence Data, RNA, Messenger genetics, Restriction Mapping, Sequence Homology, Amino Acid, Alkyl and Aryl Transferases, Campylobacter jejuni enzymology, Transferases genetics
Abstract

The gene for 5-enolpyruvylshikimate-3-phosphate (EPSP) synthase (aroA) cloned from Campylobacter jejuni (Cj) strain 81116 was identified by complementation of an Escherichia coli (Ec) auxotrophic aroA mutant. The Cj aroA gene has been sequenced. It encodes an enzyme of 428 amino acids (aa), that is homologous to other bacterial EPSP synthases, especially that of Bacillus subtilis with which it has a 39% aa identity. The transcriptional start point was mapped. It is present in an upstream open reading frame (ORF) that has a strong homology to the gene encoding phenylalanine tRNA synthetase (pheS). Downstream from aroA another ORF is present which is homologous to the lytB gene of Ec. The stop codon of the aroA gene overlaps the start codon of lytB.

Published
1996
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47. Tissue specific and androgen-regulated expression of human prostate-specific transglutaminase.

Author

Dubbink HJ, Verkaik NS, Faber PW, Trapman J, Schröder FH, and Romijn JC

Subjects
Amino Acid Sequence, Animals, Base Sequence, Chromosome Mapping, Chromosomes, Human, Pair 3 genetics, Cloning, Molecular, Cricetinae, DNA Probes genetics, DNA, Complementary genetics, Female, Gene Expression Regulation, Enzymologic, Humans, Hybrid Cells, Male, Mice, Molecular Sequence Data, Prostatic Neoplasms enzymology, Prostatic Neoplasms genetics, Sequence Homology, Amino Acid, Tissue Distribution, Transglutaminases genetics, Tumor Cells, Cultured, Androgens metabolism, Prostate enzymology, Transglutaminases metabolism
Abstract

Transglutaminases (TGases) are calcium-dependent enzymes catalysing the post-translational cross-linking of proteins. In the prostate at least two TGases are present, the ubiquitously expressed tissue-type TGase (TGC), and a prostate-restricted TGase (TGP). This paper deals with the molecular cloning and characterization of the cDNA encoding the human prostate TGase (hTGP). For this purpose we have screened a human prostate cDNA library with a probe from the active-site region of TGC. The largest isolated cDNA contained an open reading frame encoding a protein of 684 amino acids with a predicted molecular mass of 77 kDa as confirmed by in vitro transcription-translation and subsequent SDS/PAGE. The hTGP gene was tissue-specifically expressed in the prostate, yielding an mRNA of approx. 3.5 kb. Furthermore, a 3-fold androgen-induced upregulation of hTGP mRNA expression has been demonstrated in the recently developed human prostate cancer cell line, PC346C. Other well established human prostate cancer cell lines, LNCaP and PC-3, showed no detectable hTGP mRNA expression on a Northern bolt. The gene coding for prostate TGase was assigned to chromosome 3.

Published
1996
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48. Single point mutations in domain II of the yeast mitochondrial release factor mRF-1 affect ribosome binding.

Author

Pel HJ, Rep M, Dubbink HJ, and Grivell LA

Subjects
Alleles, Amino Acid Sequence, Base Sequence, Cloning, Molecular, DNA Primers chemistry, Fungal Proteins chemistry, Mitochondria chemistry, Mitochondria metabolism, Mitochondrial Proteins, Molecular Sequence Data, Point Mutation, Recombinant Fusion Proteins, Saccharomyces cerevisiae genetics, Sequence Alignment, Sequence Homology, Amino Acid, Structure-Activity Relationship, Fungal Proteins genetics, Fungal Proteins metabolism, Peptide Chain Termination, Translational, Ribosomes metabolism, Saccharomyces cerevisiae Proteins, Transcription Factors
Abstract

We have recently described two yeast strains that are mutated in the MRF1 gene encoding the mitochondrial release factor mRF-1. Both mutants provoke gene-specific defects in mitochondrial translational termination. In the present study we report the cloning, sequencing, as well as an analysis of residual activities of both mutant mrf1 alleles. Each allele specifies a different single amino acid substitution located one amino acid apart. The amino acid changes do not affect the level or cellular localization of the mutant proteins, since equal amounts of wild type and mutant mRF-1 were detected in the mitochondrial compartment. Over-expression of the mutant alleles in wild type and mrf1 mutant yeast strains produces a phenotype consistent with a reduced affinity of the mutant release factors for the ribosome, indicating that the mutations map in a release factor domain involved in ribosome binding. We also demonstrate that nonsense suppression caused by a mutation in the mitochondrial homolog of the E. coli small ribosomal protein S4 can be reversed by a slight over-expression of the MRF1 gene.

Published
1993
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