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2. Socio-Sexual Experiences and Access to Healthcare Among Informal PrEP Users in the Netherlands

Author

van Dijk, M., de Wit, J.B.F., Kamps, R., Guadamuz, T.E., Martinez, J.E., Jonas, K.J., Leerstoel de Wit, and Social Policy and Public Health

Subjects
Sexual behavior, Informal PrEP, Infectious Diseases, Social Psychology, HIV prevention, Public Health, Environmental and Occupational Health, MSM, PrEP
Abstract

The aim of this qualitative study was to explore the experiences of informal PrEP users regarding access to PrEP and PrEP-related healthcare, community responses, sexual behavior and well-being. We interviewed 30 men who have sex with men (MSM) in semi-structured online interviews between March and August 2018. Interviews were analyzed using interpretive description. Informal PrEP users were well informed about the use of PrEP, but sometimes did not make use of renal testing. Participants reported a lack of PrEP knowledge among healthcare providers, which limited their access to PrEP and put them at risk, as they received incorrect information. Although some participants reported negative reactions from potential sex partners, most received positive reactions and were sometimes seen as more desirable sex partners. PrEP healthcare services should not only be accessible to formal PrEP users, but also to PrEP users who procure PrEP informally.

Published
2021

11. Gebruik Ecologische Sleutelfactoren - een eerste toepassing door Rijkswaterstaat

Author

Sollie, S., Hulsbos-Bloemerts, M., Boon, S., Kamps, R., Sollie, S., Hulsbos-Bloemerts, M., Boon, S., and Kamps, R.

Abstract

Rijkswaterstaat Midden-Nederland heeft een watersysteemanalyse uitgevoerd voor Randmeren-Oost. Het was de eerste keer dat Rijkswaterstaat hiervoor gebruik maakte van de Ecologische Sleutelfactoren (ESF’s). De systeemanalyse was vooral gericht op het creëren van systeembegrip. Uit de analyse blijkt dat het denkkader van de ESF-systematiek goed toepasbaar is op grotere rijkswateren. Er is meer inzicht in het functioneren van het systeem. Knelpunt in de watersysteemanalyse is het huidige meetnet. Voor sommige parameters is er te weinig informatie om het heterogene gebied goed in de vingers krijgen. Aanpassing van het meetnet wordt geadviseerd.

Published
2020

13. Whole exome sequencing is the preferred strategy to identify the genetic defect in patients with a probable or possible mitochondrial cause

Author

Theunissen, T.E.J. (Tom E.J.), Nguyen, M. (Minh), Kamps, R. (Rick), Hendrickx, A. (Alexandra), Sallevelt, S.C.E.H. (Suzanne), Gottschalk, R.W.H. (Ralph W.H.), Calis, C. (Chantal), Stassen, A.P.M. (Alphons P.M.), De Koning, B. (Bart), Mulder-Den Hartog, E.N.M. (Elvira N.M.), Schoonderwoerd, K. (Kees), Fuchs, S.A. (Sabine A.), Hilhorst-Hofstee, Y. (Yvonne), Visser, M. (Marianne) de, Vanoevelen, J. (Jo), Szklarczyk, R. (Radek), Gerards, M. (Mike), Coo, I.F.M. (René) de, Hellebrekers, D.M.E.I. (Debby), Smeets, H.J.M. (Hubert), Theunissen, T.E.J. (Tom E.J.), Nguyen, M. (Minh), Kamps, R. (Rick), Hendrickx, A. (Alexandra), Sallevelt, S.C.E.H. (Suzanne), Gottschalk, R.W.H. (Ralph W.H.), Calis, C. (Chantal), Stassen, A.P.M. (Alphons P.M.), De Koning, B. (Bart), Mulder-Den Hartog, E.N.M. (Elvira N.M.), Schoonderwoerd, K. (Kees), Fuchs, S.A. (Sabine A.), Hilhorst-Hofstee, Y. (Yvonne), Visser, M. (Marianne) de, Vanoevelen, J. (Jo), Szklarczyk, R. (Radek), Gerards, M. (Mike), Coo, I.F.M. (René) de, Hellebrekers, D.M.E.I. (Debby), and Smeets, H.J.M. (Hubert)

Abstract

Mitochondrial disorders, characterized by clinical symptoms and/or OXPHOS deficiencies, are caused by pathogenic variants in mitochondrial genes. However, pathogenic variants in some of these genes can lead to clinical manifestations which overlap with other neuromuscular diseases, which can be caused by pathogenic variants in non-mitochondrial genes as well. Mitochondrial pathogenic variants can be found in the mitochondrial DNA (mtDNA) or in any of the 1,500 nuclear genes with a mitochondrial function. We have performed a two-step next-generation sequencing approach in a cohort of 117 patients, mostly children, in whom a mitochondrial disease-cause could likely or possibly explain the phenotype. A total of 86 patients had a mitochondrial disorder, according to established clinical and biochemical criteria. The other 31 patients had neuromuscular symptoms, where in a minority a mitochondrial genetic cause is present, but a non-mitochondrial genetic cause is more likely. All patients were screened for pathogenic variants in the mtDNA and, if excluded, analyzed by whole exome sequencing (WES). Variants were filtered for being pathogenic and compatible with an autosomal or X-linked recessive mode of inheritance in families with multiple affected siblings and/or consanguineous parents. Non-consanguineous families with a single patient were additionally screened for autosomal and X-linked dominant mutations in a predefined gene-set. We identified causative pathogenic variants in the mtDNA in 20% of the patient-cohort, and in nuclear genes in 49%, implying an overall yield of 68%. We identified pathogenic variants in mitochondrial and non-mitochondrial genes in both groups with, obviously, a higher number of mitochondrial genes affected in mitochondrial disease patients. Furthermore, we show that 31% of the disease-causing genes in the mitochondrial patient group were not included in the MitoCarta database, and therefore would have been missed with MitoCarta based gene-p

Published
2018
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14. Whole Exome Sequencing Is the Preferred Strategy to Identify the Genetic Defect in Patients With a Probable or Possible Mitochondrial Cause

Author

Theunissen, T E J, Nguyen, M, Kamps, R, Hendrickx, AT, Sallevelt, S, Gottschalk, RWH, Calis, CM, Stassen, APM, Koning, BAE, Mulder-Den Hartog, E N M, Schoonderwoerd, Kees, Fuchs, SA, Hilhorst-Hofstee, Y, Visser, M, Vanoevelen, J, Szklarczyk, R, Gerards, M, de Coo, IFM, Hellebrekers, D, Smeets, HJM, Theunissen, T E J, Nguyen, M, Kamps, R, Hendrickx, AT, Sallevelt, S, Gottschalk, RWH, Calis, CM, Stassen, APM, Koning, BAE, Mulder-Den Hartog, E N M, Schoonderwoerd, Kees, Fuchs, SA, Hilhorst-Hofstee, Y, Visser, M, Vanoevelen, J, Szklarczyk, R, Gerards, M, de Coo, IFM, Hellebrekers, D, and Smeets, HJM

Published
2018

18. Selection and characterization of palmitic acid responsive patients with an OXPHOS complex i defect

Author

Theunissen, T.E.J. (Tom E. J.), Gerards, M. (Mike), Hellebrekers, D.M.E.I. (Debby), Tienen, F.H.J. van, Kamps, R. (Rick), Sallevelt, S.C.E.H. (Suzanne), Hartog, E.N.M.M.-D. (Elvira N. M. M.-D.), Scholte, H.R. (Hans), Verdijk, R.M. (Robert), Schoonderwoerd, K. (Kees), Coo, I.F.M. (René) de, Szklarczyk, R. (Radek), Smeets, H.J.M. (Hubert), Theunissen, T.E.J. (Tom E. J.), Gerards, M. (Mike), Hellebrekers, D.M.E.I. (Debby), Tienen, F.H.J. van, Kamps, R. (Rick), Sallevelt, S.C.E.H. (Suzanne), Hartog, E.N.M.M.-D. (Elvira N. M. M.-D.), Scholte, H.R. (Hans), Verdijk, R.M. (Robert), Schoonderwoerd, K. (Kees), Coo, I.F.M. (René) de, Szklarczyk, R. (Radek), and Smeets, H.J.M. (Hubert)

Abstract

Mitochondrial disorders are genetically and clinically heterogeneous, mainly affecting high energy-demanding organs due to impaired oxidative phosphorylation (OXPHOS). Currently, effective treatments for OXPHOS defects, with complex I deficiency being the most prevalent, are not available. Yet, clinical practice has shown that some complex I deficient patients benefit from a high-fat or ketogenic diet, but it is unclear how these therapeutic diets influence mitochondrial function and more importantly, which complex I patients could benefit from such treatment. Dietary studies in a complex I deficient patient with exercise intolerance showed increased muscle endurance on a high-fat diet compared to a high-carbohydrate diet. We performed whole-exome sequencing to characterize the genetic defect. A pathogenic homozygous p.

Published
2017
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19. Selection and Characterization of Palmitic Acid Responsive Patients with an OXPHOS Complex I Defect

Author

Theunissen, T E J, Gerards, M, Hellebrekers, D, van Tienen, FH, Kamps, R, Sallevelt, S, Hartog, E, Scholte, Jasper, Verdijk, Rob, Schoonderwoerd, Kees, Coo, IFM, Szklarczyk, R, Smeets, HJM, Theunissen, T E J, Gerards, M, Hellebrekers, D, van Tienen, FH, Kamps, R, Sallevelt, S, Hartog, E, Scholte, Jasper, Verdijk, Rob, Schoonderwoerd, Kees, Coo, IFM, Szklarczyk, R, and Smeets, HJM

Published
2017

20. Pathogenic CWF19L1 variants as a novel cause of autosomal recessive cerebellar ataxia and atrophy

Author

Nguyen, M. (Minh), Boesten, I. (Iris), Hellebrekers, D.M.E.I. (Debby), Vanoevelen, J. (Jo), Kamps, R. (Rick), De Koning, B. (Bart), Coo, I.F.M. (René) de, Gerards, M. (Mike), Smeets, H.J.M. (Hubert), Nguyen, M. (Minh), Boesten, I. (Iris), Hellebrekers, D.M.E.I. (Debby), Vanoevelen, J. (Jo), Kamps, R. (Rick), De Koning, B. (Bart), Coo, I.F.M. (René) de, Gerards, M. (Mike), and Smeets, H.J.M. (Hubert)

Abstract

Autosomal recessive cerebellar ataxia (ARCA) is a group of neurological disorders characterized by degeneration or abnormal development of the cerebellum and spinal cord. ARCA is clinically and genetically highly heterogeneous, with over 20 genes involved. Exome sequencing of a girl with ARCA from non-consanguineous Dutch parents revealed two pathogenic variants c.37G>C; p.D13H and c.946A>T; p.K316∗ in CWF19L1, a gene with an unknown function, recently reported to cause ARCA in a Turkish family. Sanger sequencing showed that the c.37G>C variant was inherited from the father and the c.946A>T variant from the mother. Pathogenicity was based on the damaging effect on protein function as the c.37G>C variant changed the highly conserved, negatively charged aspartic acid to the positively charged histidine and the c.946A>T variant introduced a premature stop codon. In addition, 27 patients with ARCA were tested for pathogenic variants in CWF19L1, however, no pathogenic variants were identified. Our data confirm CWF19L1 as a novel but rare gene causing ARCA.

Published
2016
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21. Specific MRI abnormalities reveal severe perrault syndrome due to CLPP defects

Author

Theunissen, T.E.J. (Tom E.J.), Szklarczyk, R. (Radek), Gerards, M. (Mike), Hellebrekers, D.M.E.I. (Debby), Mulder-Den Hartog, E.N.M. (Elvira N.M.), Vanoevelen, J. (Jo), Kamps, R. (Rick), De Koning, B. (Bart), Lane Rutledge, S., Schmitt-Mechelke, T. (Thomas), Berkel, C.G.M. (Carola) van, Knaap, M.S. (Marjo) van der, Coo, I.F.M. (René) de, Smeets, H.J.M. (Hubert), Theunissen, T.E.J. (Tom E.J.), Szklarczyk, R. (Radek), Gerards, M. (Mike), Hellebrekers, D.M.E.I. (Debby), Mulder-Den Hartog, E.N.M. (Elvira N.M.), Vanoevelen, J. (Jo), Kamps, R. (Rick), De Koning, B. (Bart), Lane Rutledge, S., Schmitt-Mechelke, T. (Thomas), Berkel, C.G.M. (Carola) van, Knaap, M.S. (Marjo) van der, Coo, I.F.M. (René) de, and Smeets, H.J.M. (Hubert)

Abstract

In establishing a genetic diagnosis in heterogeneous neurological disease, clinical characterization and whole exome sequencing (WES) go hand-in-hand. Clinical data are essential, not only to guide WES variant selection and define the clinical severity of a genetic defect but also to identify other patients with defects in the same gene. In an infant patient with sensorineural hearing loss, psychomotor retardation, and epilepsy, WES resulted in identification of a novel homozygous CLPP frameshift mutation (c.21delA). Based on the gene defect and clinical symptoms, the diagnosis Perrault syndrome type 3 (PRLTS3) was established. The patient's brain-MRI revealed specific abnormalities of the subcortical and deep cerebral white matter and the middle blade of the corpus callosum, which was used to identify similar patients in the Amsterdam brain-MRI database, containing over 3000 unclassified leukoencephalopathy cases. In three unrelated patients with similar MRI abnormalities the CLPP gene was sequenced, and in two of them novel missense mutations were identified together with a large deletion that covered part of the CLPP gene on the other allele. The severe neurological and MRI abnormalities in these young patients were due to the drastic impact of the CLPP mutations, correlating with the variation in clinical manifestations among previously reported patients. Our data show that similarity in brain-MRI patterns can be used to identify novel PRLTS3 patients, especially during early disease stages, when only part of the disease manifestations are present. This seems especially applicable to the severely affected cases in which CLPP function is drastically affected and MRI abnormalities are pronounced.

Published
2016
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22. Specific MRI Abnormalities Reveal Severe Perrault Syndrome due to CLPP Defects

Author

Theunissen, T E J, Szklarczyk, R, Gerards, M, Hellebrekers, DMEI, den Hartog, NM (Elvira), Vanoevelen, J, Kamps, R, de Koning, B, Rutledge, S L, Schmitt-Mechelke, T, van Berkel, CGM, van der Knaap, MS, Coo, IFM, Smeets, HJM, Theunissen, T E J, Szklarczyk, R, Gerards, M, Hellebrekers, DMEI, den Hartog, NM (Elvira), Vanoevelen, J, Kamps, R, de Koning, B, Rutledge, S L, Schmitt-Mechelke, T, van Berkel, CGM, van der Knaap, MS, Coo, IFM, and Smeets, HJM

Published
2016

23. Next-generation sequencing-based genome diagnostics across clinical genetics centers: implementation choices and their effects

Author

Vrijenhoek, T., Kraaijeveld, K., Elferink, M., Ligt, J. de, Kranendonk, E., Santen, G., Nijman, IJ, Butler, D., Claes, G., Costessi, A., Dorlijn, W., Eyndhoven, W. van, Halley, D.J., Hout, M.C. van den, Hove, S. van, Johansson, L.F., Jongbloed, J.D., Kamps, R., Kockx, C.E., Koning, B. de, Kriek, M., Deprez, R.L., Lunstroo, H., Mannens, M., Mook, O.R., Nelen, M.R., Ploem, C., Rijnen, M., Saris, J.J., Sinke, R., Sistermans, E., Slegtenhorst, M. van, Sleutels, F., Stoep, N. van der, Tienhoven, M. van, Vermaat, M., Vogel, M., Waisfisz, Q., Weiss, J.M., Wijngaard, A. van den, Workum, W. van, IJntema, H., Zwaag, B. van der, van, I.W.F., Dunnen, J.T. den, Veltman, J.A., Hennekam, R., Cuppen, E., Vrijenhoek, T., Kraaijeveld, K., Elferink, M., Ligt, J. de, Kranendonk, E., Santen, G., Nijman, IJ, Butler, D., Claes, G., Costessi, A., Dorlijn, W., Eyndhoven, W. van, Halley, D.J., Hout, M.C. van den, Hove, S. van, Johansson, L.F., Jongbloed, J.D., Kamps, R., Kockx, C.E., Koning, B. de, Kriek, M., Deprez, R.L., Lunstroo, H., Mannens, M., Mook, O.R., Nelen, M.R., Ploem, C., Rijnen, M., Saris, J.J., Sinke, R., Sistermans, E., Slegtenhorst, M. van, Sleutels, F., Stoep, N. van der, Tienhoven, M. van, Vermaat, M., Vogel, M., Waisfisz, Q., Weiss, J.M., Wijngaard, A. van den, Workum, W. van, IJntema, H., Zwaag, B. van der, van, I.W.F., Dunnen, J.T. den, Veltman, J.A., Hennekam, R., and Cuppen, E.

Abstract

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Published
2015

24. Next-generation sequencing-based genome diagnostics across clinical genetics centers: Implementation choices and their effects

Author

Vrijenhoek, T. (T.), Kraaijeveld, K. (Ken), Elferink, M.G. (Martin), Ligt, J. (Joep) de, Kranendonk, E. (Elcke), Santen, G.W.E. (Gijs), Nijman, I.J. (Isaac ), Butler, D. (Derek), Claes, G. (Godelieve), Costessi, A. (Adalberto), Dorlijn, W. (Wim), Van Eyndhoven, W. (Winfried), Halley, D.J.J. (Dicky), Van Den Hout, M.C.G.N. (Mirjam C.G.N.), Van Hove, S. (Steven), Johansson, L.F. (Lennart F.), Jongbloed, J.D.H. (Jan), Kamps, R. (Rick), Kockx, C. (Christel), De Koning, B. (Bart), Kriek, N. (Nadia), Lekanne Dit Deprez, R.H., Lunstroo, H. (Hans), Mannens, M.M.A.M. (Marcel), Mook, O. (Olaf), Nelen, M.R. (Marcel), Ploem, C. (Corrette), Rijnen, M. (Marco), Saris, J.J. (Jasper), Sinke, R.J. (Richard J), Sistermans, E. (Erik), Slegtenhorst, M.A. (Marjon) van, Sleutels, F. (Frank), Stoep, N. (Nienke) van der, Tienhoven, M. (Marianne) van, Vermaat, M. (Martijn), Vogel, M.J. (Maartje), Waisfisz, Q. (Quinten), Weiss, J.M. (Janneke), Wijngaard, A. (Arthur) van den, Workum, W. (W) van, Ijntema, H. (Helger), Zwaag, B. (Bert) van der, IJcken, W.F.J. (Wilfred) van, Dunnen, J.T. (Johan) den, Veltman, J.A. (Joris), Hennekam, R.C.M. (Raoul), Cuppen, E. (Edwin), Vrijenhoek, T. (T.), Kraaijeveld, K. (Ken), Elferink, M.G. (Martin), Ligt, J. (Joep) de, Kranendonk, E. (Elcke), Santen, G.W.E. (Gijs), Nijman, I.J. (Isaac ), Butler, D. (Derek), Claes, G. (Godelieve), Costessi, A. (Adalberto), Dorlijn, W. (Wim), Van Eyndhoven, W. (Winfried), Halley, D.J.J. (Dicky), Van Den Hout, M.C.G.N. (Mirjam C.G.N.), Van Hove, S. (Steven), Johansson, L.F. (Lennart F.), Jongbloed, J.D.H. (Jan), Kamps, R. (Rick), Kockx, C. (Christel), De Koning, B. (Bart), Kriek, N. (Nadia), Lekanne Dit Deprez, R.H., Lunstroo, H. (Hans), Mannens, M.M.A.M. (Marcel), Mook, O. (Olaf), Nelen, M.R. (Marcel), Ploem, C. (Corrette), Rijnen, M. (Marco), Saris, J.J. (Jasper), Sinke, R.J. (Richard J), Sistermans, E. (Erik), Slegtenhorst, M.A. (Marjon) van, Sleutels, F. (Frank), Stoep, N. (Nienke) van der, Tienhoven, M. (Marianne) van, Vermaat, M. (Martijn), Vogel, M.J. (Maartje), Waisfisz, Q. (Quinten), Weiss, J.M. (Janneke), Wijngaard, A. (Arthur) van den, Workum, W. (W) van, Ijntema, H. (Helger), Zwaag, B. (Bert) van der, IJcken, W.F.J. (Wilfred) van, Dunnen, J.T. (Johan) den, Veltman, J.A. (Joris), Hennekam, R.C.M. (Raoul), and Cuppen, E. (Edwin)

Abstract

Implementation of next-generation DNA sequencing (NGS) technology into routine diagnostic genome care requires strategic choices. Instead of theoretical discussions on the consequences of such choices, we compared NGS-based diagnostic practices in eight clinical genetic centers in the Netherlands, based on genetic testing of nine pre-selected patients with cardiomyopathy. We highlight critical implementation choices, including the specific contributions of laboratory and medical specialists, bioinformaticians and researchers to diagnostic genome care, and how these affect interpretation and reporting of variants. Reported pathogenic mutations were consistent for all but one patient. Of the two centers that were inconsistent in their diagnosis, one reported to have found 'no causal variant', thereby underdiagnosing this patient. The other provided an alternative diagnosis, identifying another variant as causal than the other centers. Ethical and legal analysis showed that informed consent procedures in all centers were generally adequate for diagnostic NGS applications that target a limited set of genes, but not for exome- and genome-based diagnosis. We propose changes to further improve and align these procedures, taking into account the blurring boundary between diagnostics and research, and specific counseling options for exome- and genome-based diagnostics. We conclude that alternative diagnoses may infer a certain level of 'greediness' to come to a positive diagnosis in interpreting sequencing results. Moreover, there is an increasing interdependence of clinic, diagnostics and research departments for comprehensive diagnostic genome care. Therefore, we invite clinical geneticists, physicians, researchers, bioinformatics experts and patients to reconsider their role and position in future diagnostic genome care.

Published
2015
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25. Next-generation sequencing-based genome diagnostics across clinical genetics centers: implementation choices and their effects

Author

Vrijenhoek, T, Kraaijeveld, K, Elferink, M, de Ligt, J, Kranendonk, E, Santen, G, Nijman, IJ, Butler, D, Claes, G, Costessi, A, Dorlijn, W, van Eyndhoven, W, Halley, Dicky, Van den Hout - van Vroonhoven, Mirjam, van Hove, S, Johansson, LF, Jongbloed, JDH, Kamps, R, Kockx, Christel, de Koning, B, Kriek, M, Deprez, RLD, Lunstroo, H, Mannens, M, Mook, OR, Nelen, M, Ploem, C, Rijnen, M, Saris, Jasper, Sinke, R, Sistermans, E, van Slegtenhorst, Marjon, Sleutels, Frank, van der Stoep, N, Tienhoven, Marianne, Vermaat, M, Vogel, M, Waisfisz, Q, Weiss, JM, van den Wijngaard, A, van Workum, W, Ijntema, H, Van der Zwaag, B, van Ijcken, Wilfred, den Dunnen, J, Veltman, JA, Hennekam, R, Cuppen, E, Vrijenhoek, T, Kraaijeveld, K, Elferink, M, de Ligt, J, Kranendonk, E, Santen, G, Nijman, IJ, Butler, D, Claes, G, Costessi, A, Dorlijn, W, van Eyndhoven, W, Halley, Dicky, Van den Hout - van Vroonhoven, Mirjam, van Hove, S, Johansson, LF, Jongbloed, JDH, Kamps, R, Kockx, Christel, de Koning, B, Kriek, M, Deprez, RLD, Lunstroo, H, Mannens, M, Mook, OR, Nelen, M, Ploem, C, Rijnen, M, Saris, Jasper, Sinke, R, Sistermans, E, van Slegtenhorst, Marjon, Sleutels, Frank, van der Stoep, N, Tienhoven, Marianne, Vermaat, M, Vogel, M, Waisfisz, Q, Weiss, JM, van den Wijngaard, A, van Workum, W, Ijntema, H, Van der Zwaag, B, van Ijcken, Wilfred, den Dunnen, J, Veltman, JA, Hennekam, R, and Cuppen, E

Abstract

Implementation of next-generation DNA sequencing (NGS) technology into routine diagnostic genome care requires strategic choices. Instead of theoretical discussions on the consequences of such choices, we compared NGS-based diagnostic practices in eight clinical genetic centers in the Netherlands, based on genetic testing of nine pre-selected patients with cardiomyopathy. We highlight critical implementation choices, including the specific contributions of laboratory and medical specialists, bioinformaticians and researchers to diagnostic genome care, and how these affect interpretation and reporting of variants. Reported pathogenic mutations were consistent for all but one patient. Of the two centers that were inconsistent in their diagnosis, one reported to have found 'no causal variant', thereby underdiagnosing this patient. The other provided an alternative diagnosis, identifying another variant as causal than the other centers. Ethical and legal analysis showed that informed consent procedures in all centers were generally adequate for diagnostic NGS applications that target a limited set of genes, but not for exome-and genome-based diagnosis. We propose changes to further improve and align these procedures, taking into account the blurring boundary between diagnostics and research, and specific counseling options for exome- and genome-based diagnostics. We conclude that alternative diagnoses may infer a certain level of 'greediness' to come to a positive diagnosis in interpreting sequencing results. Moreover, there is an increasing interdependence of clinic, diagnostics and research departments for comprehensive diagnostic genome care. Therefore, we invite clinical geneticists, physicians, researchers, bioinformatics experts and patients to reconsider their role and position in future diagnostic genome care.

Published
2015

26. Status of the SRF Gun operation at ELBE

Author

Teichert, J., Arnold, A., Buettig, H., Janssen, D., Justus, M., Lehnert, U., Michel, P., Murcek, P., Schneider, C., Schurig, R., Staufenbiel, F., Kamps, R. X. T., Rudolph, J., Schenk, M., Klemz, G., and Will, I.

Abstract

The superconducting RF photo-injector (SRF gun) at FZD is the first operating electron injector of its kind. The gun with a 3½-cell cavity operating and a frequency of 1.3 GHz produces an electron beam of 3 MeV with a maximum bunch charge of about 400 pC. Also the design values for the acceleration gradient could not be reached with the cavity which is in use at present the SRF gun will improve the beam quality for ELBE users. End of 2009 the beamline was installed which connects the SRF gun with ELBE accelerator. We will report on the first test and on the progress in applying the SRF gun for user operation.

Published
2010

27. Zwevend stof atlas Markermeer

Author

Kamps, R., Koster, E., Eleveld, M.A., Kuiper, M., Laanen, M., Institute for Environmental Studies, and Spatial analysis & Decision Support

Published
2007

29. Olfactomedin-4 regulation by estrogen in the human endometrium requires epidermal growth factor signaling

Author

Dassen, H., Punyadeera, C., Delvoux, B., Schulkens, I., Marchetti, C., Kamps, R., Klomp, J., Dijcks, F., De Goeij, A., D'Hooghe, T., Kyama, C., Ederveen, A., Dunselman, G., Groothuis, P., Romano, A., Marchetti C. (ORCID:0000-0001-7098-8956), Dassen, H., Punyadeera, C., Delvoux, B., Schulkens, I., Marchetti, C., Kamps, R., Klomp, J., Dijcks, F., De Goeij, A., D'Hooghe, T., Kyama, C., Ederveen, A., Dunselman, G., Groothuis, P., Romano, A., and Marchetti C. (ORCID:0000-0001-7098-8956)

Published
2010

30. Effects of selective oestrogen receptor modulators on proliferation in tissue cultures of pre- and postmenopausal human endometrium

Author

UCL - MD/GYPE - Département de gynécologie, d'obstétrique et de pédiatrie, Punyadeera, C., Kamps, R., Defrere, Sylvie, Dijcks, F., de Goeij, A., Ederveen, A., Dunselman, G., Groothuis, P., UCL - MD/GYPE - Département de gynécologie, d'obstétrique et de pédiatrie, Punyadeera, C., Kamps, R., Defrere, Sylvie, Dijcks, F., de Goeij, A., Ederveen, A., Dunselman, G., and Groothuis, P.

Abstract

We characterised the effects of selective oestrogen receptor modulators (SERM) in explant cultures of human endometrium tissue. Endometrium tissues were cultured for 24 h in Millicell-CM culture inserts in serum-free medium in the presence of vehicle,17 beta-estradiol (17 beta-E2,1 nM), oestrogen receptor (ER) antagonist ICI 164.384 (40 nM), and 4-OH-tamoxifen (40 nM), raloxifene (4 nM), lasofoxifene (4 nM)and acolbifene (4 nM). Protein expression of ER alpha, ER beta 1 and Ki-67 were evaluated by immunohistochemistry (IHC). The proliferative fraction was assessed by counting the number of Ki-67 positive cells. Nuclear staining of ER( and ER(1 was observed in the glandular epithelium and stroma of pre- and postmenopausal endometrium. ER(1 protein was also localized in the endothelial cells of blood vessels. Treating premenopausal endometrium tissue with 17 beta-E2 increased the fraction of Ki-67 positive cells (p < 0.001) by 55% in glands compared to the control. Raloxifene (4 nM) increased (p < 0.05) the Ki-67 positive fraction. All other SERMS did not affect proliferation in this model. Treating postmenopausal endometrium with 17(-E2 increased (p < 0.001) the fraction of Ki-67 positive cells by 250% in glands compared to the control. A similar effect was also seen for 4-OH-tamoxifen, whereas the rest of SERMs did not stimulate proliferation. We demonstrated that oestradiol increases the fraction of proliferating cells in short term explant cultures of postmenopausal endometrium. In addition, we were able to reveal the agonistic properties of 4-OH-tamoxifen and confirm that raloxifene and next-generation SERMs acolbifene and lasofoxifene were neutral on the human postmenopausal endometrium. (C) 2008 Elsevier Ltd. All rights reserved.

Published
2008

31. Effects of selective oestrogen receptor modulators on proliferation in tissue cultures of pre- and postmenopausal human endometrium

Author

Punyadeera, Chamindie, Kamps, R., Defrere, S., Dijcks, F., de Goeij, A., Ederveen, A., Dunselman, G., Groothuis, P., Punyadeera, Chamindie, Kamps, R., Defrere, S., Dijcks, F., de Goeij, A., Ederveen, A., Dunselman, G., and Groothuis, P.

Abstract

We characterised the effects of selective oestrogen receptor modulators (SERM) in explant cultures of human endometrium tissue. Endometrium tissues were cultured for 24 h in Millicell-CM culture inserts in serum-free medium in the presence of vehicle,17 beta-estradiol (17 beta-E2,1 nM), oestrogen receptor (ER) antagonist ICI 164.384 (40 nM), and 4-OH-tamoxifen (40 nM), raloxifene (4 nM), lasofoxifene (4 nM)and acolbifene (4 nM). Protein expression of ER alpha, ER beta 1 and Ki-67 were evaluated by immunohistochemistry (IHC). The proliferative fraction was assessed by counting the number of Ki-67 positive cells. Nuclear staining of ER( and ER(1 was observed in the glandular epithelium and stroma of pre- and postmenopausal endometrium. ER(1 protein was also localized in the endothelial cells of blood vessels. Treating premenopausal endometrium tissue with 17 beta-E2 increased the fraction of Ki-67 positive cells (p < 0.001) by 55% in glands compared to the control. Raloxifene (4 nM) increased (p < 0.05) the Ki-67 positive fraction. All other SERMS did not affect proliferation in this model. Treating postmenopausal endometrium with 17(-E2 increased (p < 0.001) the fraction of Ki-67 positive cells by 250% in glands compared to the control. A similar effect was also seen for 4-OH-tamoxifen, whereas the rest of SERMs did not stimulate proliferation. We demonstrated that oestradiol increases the fraction of proliferating cells in short term explant cultures of postmenopausal endometrium. In addition, we were able to reveal the agonistic properties of 4-OH-tamoxifen and confirm that raloxifene and next-generation SERMs acolbifene and lasofoxifene were neutral on the human postmenopausal endometrium. (C) 2008 Elsevier Ltd. All rights reserved.

Published
2008

32. Oral contraceptives prevent the development of endometriosis in the chicken chorioallantoic membrane model

Author

Nap, Annemiek, Groothuis, P., Punyadeera, Chamindie, Klein-Hitpass, L., Kamps, R., Delvoux, B., Dunselman, G., Nap, Annemiek, Groothuis, P., Punyadeera, Chamindie, Klein-Hitpass, L., Kamps, R., Delvoux, B., and Dunselman, G.

Abstract

Background: Fundamental and genetic differences between women in the endometrium may cause some to develop endometriosis, whereas others (to not. Oral contraceptives (OC) may have in effect on the endometrium, rendering the development of endometriosis less likely. Study Design: Endometrium front women using CC (OCE) and menstrual endometrium (ME) from normal cycling women were transplanted onto the chicken chorioallantoic membrane (CAM), and endometriosis-like lesion formation was evalualed. Microarray gene expression profiling was performed to identify, differentially expressed genes in the endometrium front these groups. Microarray data were validated by real-time PCR. Results: Less endometriosis-like lesions were formed after transplantation of OCE than after transplantation of ME (p<.05). Most of the differentially expressed genes belong to the TGF beta superfamily. Real-time PCR validation revealed that inhibin beta A (INHBA) expression was significantly decreased in OCE its compared to ME. Conclusion: OC use affects the characteristics Of endometrium, rendering it less potent to develop into endometriosis. (C) 2008 Elsevier Inc. All rights reserved.

Published
2008

33. Identification of novel antigens in blood vessels in rectovaginal endometriosis.

Author

UCL - MD/GYPE - Département de gynécologie, d'obstétrique et de pédiatrie, Van Langendonckt, Anne, Punyadeera, C., Kamps, R., Dunselman, G., Klein-Hitpass, L, Schurgers, L J, Squifflet, Jean-Luc, Donnez, Jacques, Groothuis, P., UCL - MD/GYPE - Département de gynécologie, d'obstétrique et de pédiatrie, Van Langendonckt, Anne, Punyadeera, C., Kamps, R., Dunselman, G., Klein-Hitpass, L, Schurgers, L J, Squifflet, Jean-Luc, Donnez, Jacques, and Groothuis, P.

Abstract

To identify specific markers of rectovaginal endometriotic nodule vasculature, highly enriched preparations of vascular endothelial cells and pericytes were obtained from endometriotic nodules and control endometrial and myometrial tissue by laser capture microdissection (LCM), and gene expression profiles were screened by microarray analysis. Of the 18 400 transcripts on the arrays, 734 were significantly overexpressed in vessels from fibromuscular tissue and 923 in vessels from stromal tissue of endometriotic nodules, compared with vessels dissected from control tissues. The most frequently expressed transcripts included known endothelial cell-associated genes, as well as transcripts with little or no previous association with vascular cells. The higher expression in blood vessels was further corroborated by immunohistochemical staining of six potential markers, five of which showed strong expression in pericytes. The most promising marker was matrix Gla protein, which was found to be present in both glandular epithelial cells and vascular endothelial cells of endometriotic lesions, although it was barely expressed at all in normal endometrium. LCM, combined with microarray analysis, constitutes a powerful tool for mapping the transcriptome of vascular cells. After immunohistochemical validation, markers of vascular endothelial and perivascular cells from endometriotic nodules could be identified, which may provide targets to improve early diagnosis or to selectively deliver therapeutic agents.

Published
2007

34. Estrogen metabolizing enzymes in endometrium and endometriosis.

Author

UCL - MD/GYPE - Département de gynécologie, d'obstétrique et de pédiatrie, UCL - (SLuc) Service de gynécologie et d'andrologie, Dassen, H, Punyadeera, C., Kamps, R., Delvoux, B, Van Langendonckt, Anne, Donnez, Jacques, Husen, B, Thole, H, Dunselman, G., Groothuis, P., UCL - MD/GYPE - Département de gynécologie, d'obstétrique et de pédiatrie, UCL - (SLuc) Service de gynécologie et d'andrologie, Dassen, H, Punyadeera, C., Kamps, R., Delvoux, B, Van Langendonckt, Anne, Donnez, Jacques, Husen, B, Thole, H, Dunselman, G., and Groothuis, P.

Abstract

BACKGROUND: Estradiol (E(2)) is an important promoter of the growth of both eutopic and ectopic endometrium. The findings with regard to the expression and activity of steroidogenic enzymes in endometrium of controls, in endometrium of endometriosis patients and in endometriotic lesions are not consistent. METHODS: In this study, we have looked at the mRNA expression and protein levels of a range of steroidogenic enzymes [aromatase, 17beta-hydroxysteroid dehydrogenases (17beta-HSD) type 1, 2 and 4, estrogen sulfotransferase (EST) and steroid sulfatase (STS)] in eutopic and ectopic endometrium of patients (n = 14) with deep-infiltrative endometriosis as well as in disease-free endometrium (n = 48) using real-time PCR and immunocytochemistry. In addition, we evaluated their menstrual cycle-related expression patterns, and investigated their steroid responsiveness in explant cultures. RESULTS: Aromatase and 17beta-HSD type 1 mRNA levels were extremely low in normal human endometrium, while mRNAs for types 2 and 4 17beta-HSD, EST and STS were readily detectable. Only 17beta-HSD type 2 and EST genes showed sensitivity to progesterone in normal endometrium. Types 1 and 2 17beta-HSD and STS protein was detected in normal endometrium using new polyclonal antibodies. CONCLUSIONS: In endometriosis lesions, the balance is tilted in favor of enzymes producing E(2). This is due to a suppression of types 2 and 4 17beta-HSD, and an increased expression of aromatase and type 1 17beta-HSD in ectopic endometrium.

Published
2007

35. Expression and regulation of vascular endothelial growth factor ligands and receptors during menstruation and post-menstrual repair of human endometrium

Author

Punyadeera, Chamindie, Thijssen, V., Tchaikovski, S., Kamps, R., Delvoux, B., Dunselman, G., de Goeij, A., Griffioen, A., Groothuis, P., Punyadeera, Chamindie, Thijssen, V., Tchaikovski, S., Kamps, R., Delvoux, B., Dunselman, G., de Goeij, A., Griffioen, A., and Groothuis, P.

Abstract

*This article is free to read on the publisher's website* Regeneration and growth of the human endometrium after shedding of the functional layer during menstruation depends on an adequate angiogenic response. We analysed the mRNA expression levels of all known vascular endothelial growth factor (VEGF) ligands and receptors in human endometrium collected in the menstrual and proliferative phases of the menstrual cycle. In addition, we evaluated the expression of VEGF-A, VEGF-R2 and NRP-1 at the protein level. Two periods of elevated mRNA expression of ligands and receptors were observed, separated by a distinct drop at cycle days (CDs) 9 and 10. Immunohistochemical staining showed that VEGF and VEGF-R2 were expressed in epithelial, stromal and endothelial cells. NRP-1 was mainly confined to stroma and blood vessels; only in late-proliferative endometrium, epithelial staining was also observed. Except for endothelial VEGF-R2 expression in CDs 6-8, there were no significant differences in the expression of VEGF, VEGF-R2 or NRP-1 in any of the cell compartments. In contrast, VEGF release by cultured human endometrium explants decreased during the proliferative phase. This output was significantly reduced in menstrual and early-proliferative endometrium by estradiol (E2) treatment. Western blot analysis indicated that part of the VEGF-A was trapped in the extracellular matrix (ECM). Changes in VEGF ligands and receptors were associated with elevated expression of the hypoxia markers HIF1 alpha and CA-IX in the menstrual and early proliferative phases. HIF1 alpha was also detected in late-proliferative phase endometrium. Our findings indicate that VEGF-A exerts its actions mostly during the first half of the proliferative phase. Furthermore, VEGF-A production appears to be triggered by hypoxia in the menstrual phase and subsequently suppressed toy estrogen during the late proliferative phase.

Published
2006

36. Oestrogen-modulated gene expression in the human endometrium

Author

Punyadeera, Chamindie, Dassen, H., Klomp, J., Dunselman, G., Kamps, R., Dijcks, F., Ederveen, A., de Goeij, A., Groothuis, P., Punyadeera, Chamindie, Dassen, H., Klomp, J., Dunselman, G., Kamps, R., Dijcks, F., Ederveen, A., de Goeij, A., and Groothuis, P.

Abstract

To identify key regulatory mechanisms in the growth and development of the human endometrium, microarray analysis was performed on uncultured human endometrium collected during menstruation (M) and the late-proliferative (LATE-P)-phase of the menstrual cycle, as well as after 24 h incubation in the presence of oestradiol (17beta-E2). We demonstrate the expression of novel gene transcripts in the human endometrium. i.e. mucin-9, novel oestrogen-responsive gene transcripts, i.e. gelsolin and flotillin-1, and genes known to be expressed in human endometrium but not yet shown to be oestrogen responsive, i.e. connexin-37 and TFF1/pS2. Genes reported to be expressed during the implantation window and implicated in progesterone action, i.e. secretoglobin family 2A, member 2 (mammaglobin) and homeobox-containing proteins, were up-regulated in uncultured LATE-P-phase endometrium compared to M-phase endometrium. Some gene transcripts are regulated directly by 17beta-E2 alone, others are influenced by the in vivo environment as well. These observations emphasise that the regulation of endometrium maturation by oestrogen entails more then just stimulation of cell proliferation.

Published
2005

37. Monitoring van oevers Hollandsche IJssel, saneren natuurlijk?

Author

Kerkum, F., Oosterbaan, J., Kamps, R., Doze, J., Kerkum, F., Oosterbaan, J., Kamps, R., and Doze, J.

Abstract

Om de Hollandsche IJssel weer schoner en natuurlijker te krijgen heeft in 1996 de Stuurgroep Hollandsche IJssel besloten tot de uitvoering van een integrale aanpak van de rivier. Deze aanpak houdt onder andere in dat de vervuiling wordt weggehaald en de oevers opnieuw worden ingericht. Om meer inzicht te krijgen in wat de effecten van deze combinatie van sanering en herinrichting zijn op fauna en flora van waterbodem en oever, is tegelijkertijd op drie locaties een zevenjarig monitoringsonderzoek gestart. Hiermee kan in de toekomst met verbeterde inzichten nieuwe gecombineerde saneringen effectiever worden uitgevoerd. In het voorjaar van 2004 zijn de laatste bemonsteringen in het kader van het monitoringsonderzoek uitgevoerd. Het eindrapport van het onderzoek wordt medio dit jaar verwacht

Published
2005

42. TESLA: The superconducting electron positron linear collider with an integrated X-ray laser laboratory. Technical design report. Pt. 2: The accelerator

Author

Andruszkow, J., Agababyan, A., Ageyev, A., Antoine, C., Aseev, V., Aune, B., Ayvazyan, V., Baboi, N., Bacher, R., Bahrdt, J., Bakker, R., Balakin, V., Balandin, V., Bandelmann, R., Barni, D., Bazhan, A., Bernard, M., Bialowons, W., Blair, G., Bloess, D., Bohnet, I., Bondarchuk, E., Bonezzi, M., Boni, R., Borzemski, P., Bosotti, A., Bourdon, J., Bousson, S., Brefeld, W., Brenger, A., Brinkmann, R., Brokmeier, H. G., Bruinsma, P. J. T., Bruck, H. D., Buhler, S., Burmeister, H., Burnton, C., Bockmann, T., Carneiro, J. P., Castellano, M., Castro, P., Catani, L., Celik, S., Champion, M., Chel, S., Chen, H., Cheng, J., Chernousko, Y., Cho, Y., Choroba, S., Cianchi, A., Clausen, M., Clozza, A., Colby, E. R., Crawford, C., Curtoni, A., Decking, W., Den Hartog, P., Derbenev, Y., Desmons, M., Devred, A., Di Pirro, G., Dietzel, W., Dinter, H., Dohlus, M., Doinikov, N., Drozhdin, A., Duhme, H. T., Dwersteg, B., Ebert, M., Eckoldt, H. J., Edwards, D., Edwards, H. T., Emma, P., Engelke, U., Englisch, U., Escherich, K., Faatz, B., Fartoukh, S., Fateev, A. A., Feikes, J., Feldhaus, J., Ferrario, M., Fitch, M. J., Flottmann, K., Follath, R., Fouaidy, M., Frentrup, W., Gadwinkel, E., Gall, P. D., Gamp, A., Garcia-Tabares, L., Garvey, T., Gassot, H., Gaupp, A., Gehring, R., Geitz, M., Gensch, U., Giove, D., Glock, H. W., Gluskin, E., Goddard, B., Goloborodko, S., Golubeva, N., Gonin, I., Gorbunov, V., Gourdin, C., Grabosch, H., Graef, D., Graeff, W., Grandsire, L., Gretchko, V., Grevsmuhl, T., Grigoryan, B., Grygiel, G., Gubarev, V., Guiducci, S., Gossel, A., Gunther, B., Habermann, T., Haebel, E., Hahn, U., Hartrott, M., Hartung, W. H., Hecht, D., Heidbrook, N., Henke, H., Henschel, H., Hensler, O., Hensler, R., Herb, S., Hessler, C., Hoffmann, G., Hoffstaetter, G., Horlitz, G., Huang, W., Hubert, D., Hulsmann, P., Huning, M., Ischebeck, R., Ivanov, I., Jablonka, M., Jaeschke, E., Janata, E., Jelezov, I., Jensch, K., Jensen, J. P., Joly, J. M., Juillard, M., Junquera, T., Jurkiewicz, P., Jostingmeier, A., Jungst, K. P., Kabel, A., Kahl, J., Kaiser, F. R., Kaiser, H., Kako, E., Kamps, R., Kamps, T., Katelev, V. V., Kauschke, M., Khabiboulline, T., Kircher, F., Kirchgessner, J. L., Klein, H., Kneisel, P., Knobloch, J., Knopf, U., Kocharyan, V., Komarek, P., Kong, D., Kostin, D., Kouptsidis, J., Kovalishin, A., Kovar, J., Kraemer, D., Krassilnikov, M., Kravchuk, L., Krebs, O., Kreps, G., Kriens, W., Krzywinski, J., Kuperman, G., Korfer, M., Lalaian, M., Lange, R., Leblond, B., Leenen, M., Lepercq, P., Lesrel, J., Leuschner, A., Liepe, M., Lierl, H., Liero, A., Lilje, L., Limberg, T., Lin, Q., Loginov, A., Lokajczyk, T., Loos, H., Lorenz, R., Lorkiewicz, J., Lottin, J. P., Loulergue, A., Lu, F., Lu, Hui-Hua, Luong, M., Loffler, F., Magne, C., Mahner, E., Marini, J., Maschmann, W., Maslov, M., Materlik, G., Matheisen, A., Menzel, J., Merker, E., Michelato, P., Minty, M., Moiseev, V., Montag, C., Mosnier, A., Muratov, V., Moller, G., Moller, W. D., Muller, G., Muller, U. C., Napoly, O., Neugebauer, F., Nicol, T., Nielsen, U., Novikov-Borodin, A., Novokhatski, A., Omeich, M., Padamsee, H. S., Pagani, C., Palmieri, V., Panvier, R., Paramonov, V., Payet, J., Pekeler, M., Peregud, V., Peters, F., Peters, H. B., Peters, O., Petersen, B., Peterson, T., Petrosyan, A., Petrosyan, G., Petrosyan, L., Petrov, A., Petrov, V. A., Pfluger, J., Phung Ngoc, B., Pieczora, K., Piel, H., Pierini, P., Pillat, P., Piot, P., Plawski, T., Plucinski, L., Polkovnikov, K., Popov, A., Prenting, J., Proch, D., Pupeter, N., Poplau, G., Qiao, J., Quack, H., Rehlich, K., Reiche, S., Rejngardt-Nikulin, P., Renken, D., Reschke, D., Reyzl, I., Richter, A., Riekehr, S., Rienen, U., Riesch, H., Riet, J. M., Rode, C., Rosenzweig, J., Rossbach, J., Roth, S., Rothemund, K., Rummler, J., Sachwitz, M., Safa, H., Saito, K., Saldin, E. L., Sandner, W., Sandvo, H., Sanelli, C., Sanok, Z., Sarvas, J., Schlarb, H., Schmidt, G., Schmitt, H., Schmitz, M., Schmuser, P., Schneider, J. R., Schneidmiller, E. A., Schnieber, R., Schoeneburg, B., Schreiber, H. J., Schreiber, S., Schulte, D., Schwarz, W., Schutt, P., Sedykh, S. N., Seidel, M., Sekutowicz, J., Sellmann, D., Serafini, L., Serio, M., Sertore, D., Setzer, S., Sgamma, F., Simrock, S., Singer, W., Singer, X., Sinram, K., Skasyrskaia, A., Sobenin, N., Sobierajski, R., Sokolov, I., Somersalo, E., Sparr, B., Spelt, J. B., Stecchi, A., Steinbrecher, R., Stephan, F., Stivanello, F., Stolper, M., Stoye, T., Swiderski, A., Sytchev, K. P., Sytchev, V. A., Sytin, A., Tang, C., Tazzari, S., Tazzioli, F., Valery Telnov, Tesch, K., Tesch, N., Thom, H., Tigner, M., Timm, H., Timm, M., Tischer, M., Tonisch, F., Tonutti, M., Toral, F., Trakhtenberg, E., Travier, C., Treusch, R., Trines, D., Tsakanov, V., Tschentscher, T., Twarowski, K., Ukkola, M., Ullrich, F. R., Varisco, G., Verzilov, V., Vielitz, T., Visentin, B., Vogel, V., Walker, N., Walter, G., Wanzenberg, R., Wedekind, H. P., Weichert, G., Weiland, T., Weise, H., Weisend, J. G., Wendt, M., Wenninger, H., Werner, M., White, M. M., Will, I., Wittenburg, K., Wojtkiewicz, J., Wolff, S., Wolski, A., Wu, Y., Wulf, F., Wobke, G., Wustefeld, G., Xiang, Y., Yazynin, I., Yi, H., Yla-Oijala, P., Yurkov, M. V., Zapfe, K., Zavadtsev, A., Zeng, X., Zhao, Q., Zhogolev, P., Zhou, F., Zimmermann, B., Zintchenko, S., Zobjack, U., and Zolotov, A.

44. LNC-ing Genetics in Mitochondrial Disease.

Author

Kamps R and Robinson EL

Abstract

Primary mitochondrial disease (MD) is a group of rare genetic diseases reported to have a prevalence of 1:5000 and is currently without a cure. This group of diseases includes mitochondrial encephalopathy, lactic acidosis, and stroke-like episodes (MELAS), maternally inherited diabetes and deafness (MIDD), Leber's hereditary optic neuropathy (LHON), Leigh syndrome (LS), Kearns-Sayre syndrome (KSS), and myoclonic epilepsy and ragged-red fiber disease (MERRF). Additionally, secondary mitochondrial dysfunction has been implicated in the most common current causes of mortality and morbidity, including cardiovascular disease (CVD) and cancer. Identifying key genetic contributors to both MD and secondary mitochondrial dysfunction may guide clinicians to assess the most effective treatment course and prognosis, as well as informing family members of any hereditary risk of disease transmission. Identifying underlying genetic causes of primary and secondary MD involves either genome sequencing (GS) or small targeted panel analysis of known disease-causing nuclear- or mitochondrial genes coding for mitochondria-related proteins. Due to advances in GS, the importance of long non-coding RNA (lncRNA) as functional contributors to the pathophysiology of MD is being unveiled. A limited number of studies have thus far reported the importance of lncRNAs in relation to MD causation and progression, and we are entering a new area of attention for clinical geneticists in specific rare malignancies. This commentary provides an overview of what is known about the role of lncRNAs as genetic and molecular contributors to disease pathophysiology and highlights an unmet need for a deeper understanding of mitochondrial dysfunction in serious human disease burdens., Competing Interests: Dr. Emma Robinson is a member of CardioLINC and prior Working Group Leader and Science Communication Manager of EU-CardioRNA (CA17129&mdash;Catalysing transcriptomics research in cardiovascular disease). She is currently a full-time employee of Edwards Lifesciences (Irvine, California).

Published
2024
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45. Impact of benzo[a]pyrene, PCB153 and sex hormones on human ESC-Derived thyroid follicles using single cell transcriptomics.

Author

Nazzari M, Romitti M, Kip AM, Kamps R, Costagliola S, van de Beucken T, Moroni L, and Caiment F

Subjects
Humans, Female, Male, Single-Cell Analysis, Human Embryonic Stem Cells drug effects, Human Embryonic Stem Cells metabolism, Benzo(a)pyrene toxicity, Polychlorinated Biphenyls toxicity, Endocrine Disruptors toxicity, Transcriptome drug effects, Gonadal Steroid Hormones, Thyroid Gland drug effects
Abstract

Introduction: Endocrine disruptors are compounds of manmade origin able to interfere with the endocrine system and constitute an important environmental concern. Indeed, detrimental effects on thyroid physiology and functioning have been described. Differences exist in the susceptibility of human sexes to the incidence of thyroid disorders, like autoimmune diseases or cancer., Methods: To study how different hormonal environments impact the thyroid response to endocrine disruptors, we exposed human embryonic stem cell-derived thyroid organoids to physiological concentrations of sex hormones resembling the serum levels of human females post-ovulation or males of reproductive age for three days. Afterwards, we added 10 µM benzo[a]pyrene or PCB153 for 24 h and analyzed the transcriptome changes via single-cell RNA sequencing with differential gene expression and gene ontology analysis., Results: The sex hormones receptors genes AR, ESR1, ESR2 and PGR were expressed at low levels. Among the thyroid markers, only TG resulted downregulated by benzo[a]pyrene or benzo[a]pyrene with the "male" hormones mix. Both hormone mixtures and benzo[a]pyrene alone upregulated ribosomal genes and genes involved in oxidative phosphorylation, while their combination decreased the expression compared to benzo[a]pyrene alone. The "male" mix and benzo[a]pyrene, alone or in combination, upregulated genes involved in lipid transport and metabolism (APOA1, APOC3, APOA4, FABP1, FABP2, FABP6). The combination of "male" hormones and benzo[a]pyrene induced also genes involved in inflammation and NFkB targets. Benzo[a]pyrene upregulated CYP1A1, CYP1B1 and NQO1 irrespective of the hormonal context. The induction was stronger in the "female" mix. Benzo[a]pyrene alone upregulated genes involved in cell cycle regulation, response to reactive oxygen species and apoptosis. PCB153 had a modest effect in presence of "male" hormones, while we did not observe any changes with the "female" mix., Conclusion: This work shows how single cell transcriptomics can be applied to selectively study the in vitro effects of endocrine disrupters and their interaction with different hormonal contexts., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 The Authors. Published by Elsevier Ltd.. All rights reserved.)

Published
2024
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46. Mitochondrial DNA D-loop variants correlate with a primary open-angle glaucoma subgroup.

Author

Vallbona-Garcia A, Lindsey PJ, Kamps R, Stassen APM, Nguyen N, van Tienen FHJ, Hamers IHJ, Hardij R, van Gisbergen MW, Benedikter BJ, de Coo IFM, Webers CAB, Gorgels TGMF, and Smeets HJM

Abstract

Introduction: Primary open-angle glaucoma (POAG) is a characteristic optic neuropathy, caused by degeneration of the optic nerve-forming neurons, the retinal ganglion cells (RGCs). High intraocular pressure (IOP) and aging have been identified as major risk factors; yet the POAG pathophysiology is not fully understood. Since RGCs have high energy requirements, mitochondrial dysfunction may put the survivability of RGCs at risk. We explored in buffy coat DNA whether mtDNA variants and their distribution throughout the mtDNA could be risk factors for POAG., Methods: The mtDNA was sequenced from age- and sex-matched study groups, being high tension glaucoma (HTG, n=71), normal tension glaucoma patients (NTG, n=33), ocular hypertensive subjects (OH, n=7), and cataract controls (without glaucoma; n=30), all without remarkable comorbidities., Results: No association was found between the number of mtDNA variants in genes encoding proteins, tRNAs, rRNAs, and in non-coding regions in the different study groups. Next, variants that controls shared with the other groups were discarded. A significantly higher number of exclusive variants was observed in the D-loop region for the HTG group (~1.23 variants/subject), in contrast to controls (~0.35 variants/subject). In the D-loop, specifically in the 7S DNA sub-region within the Hypervariable region 1 (HV1), we found that 42% of the HTG and 27% of the NTG subjects presented variants, while this was only 14% for the controls and OH subjects. As we have previously reported a reduction in mtDNA copy number in HTG, we analysed if specific D-loop variants could explain this. While the majority of glaucoma patients with the exclusive D-loop variants m.72T>C, m.16163 A>G, m.16186C>T, m.16298T>C, and m.16390G>A presented a mtDNA copy number below controls median, no significant association between these variants and low copy number was found and their possible negative role in mtDNA replication remains uncertain. Approximately 38% of the HTG patients with reduced copy number did not carry any exclusive D-loop or other mtDNA variants, which indicates that variants in nuclear-encoded mitochondrial genes, environmental factors, or aging might be involved in those cases., Conclusion: In conclusion, we found that variants in the D-loop region may be a risk factor in a subgroup of POAG, possibly by affecting mtDNA replication., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2024 Vallbona-Garcia, Lindsey, Kamps, Stassen, Nguyen, van Tienen, Hamers, Hardij, van Gisbergen, Benedikter, de Coo, Webers, Gorgels and Smeets.)

Published
2024
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47. Socio-Sexual Experiences and Access to Healthcare Among Informal PrEP Users in the Netherlands.

Author

van Dijk M, de Wit JBF, Kamps R, Guadamuz TE, Martinez JE, and Jonas KJ

Subjects
Delivery of Health Care, Homosexuality, Male, Humans, Male, Netherlands, Sexual Behavior, HIV Infections prevention & control, Pre-Exposure Prophylaxis, Sexual and Gender Minorities
Abstract

The aim of this qualitative study was to explore the experiences of informal PrEP users regarding access to PrEP and PrEP-related healthcare, community responses, sexual behavior and well-being. We interviewed 30 men who have sex with men (MSM) in semi-structured online interviews between March and August 2018. Interviews were analyzed using interpretive description. Informal PrEP users were well informed about the use of PrEP, but sometimes did not make use of renal testing. Participants reported a lack of PrEP knowledge among healthcare providers, which limited their access to PrEP and put them at risk, as they received incorrect information. Although some participants reported negative reactions from potential sex partners, most received positive reactions and were sometimes seen as more desirable sex partners. PrEP healthcare services should not only be accessible to formal PrEP users, but also to PrEP users who procure PrEP informally.

Published
2021
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48. Tfam Knockdown Results in Reduction of mtDNA Copy Number, OXPHOS Deficiency and Abnormalities in Zebrafish Embryos.

Author

Otten ABC, Kamps R, Lindsey P, Gerards M, Pendeville-Samain H, Muller M, van Tienen FHJ, and Smeets HJM

Abstract

High mitochondrial DNA (mtDNA) copy numbers are essential for oogenesis and embryogenesis and correlate with fertility of oocytes and viability of embryos. To understand the pathology and mechanisms associated with low mtDNA copy numbers, we knocked down mitochondrial transcription factor A ( tfam ), a regulator of mtDNA replication, during early zebrafish development. Reduction of tfam using a splice-modifying morpholino (MO) resulted in a 42 ± 17% decrease in mtDNA copy number in embryos at 4 days post fertilization. Morphant embryos displayed abnormal development of the eye, brain, heart, and muscle, as well as a 50 ± 22% decrease in ATP production. Transcriptome analysis revealed a decrease in protein-encoding transcripts from the heavy strand of the mtDNA, and down-regulation of genes involved in haem production and the metabolism of metabolites, which appear to trigger increased rRNA and tRNA synthesis in the nucleoli. However, this stress or compensatory response appears to fall short as pathology emerges and expression of genes related to eye development are severely down-regulated. Taken together, this study highlights the importance of sufficient mtDNA copies for early zebrafish development. Zebrafish is an excellent model to manipulate the mtDNA bottleneck and study its effect on embryogenesis rapidly and in large numbers of offspring., (Copyright © 2020 Otten, Kamps, Lindsey, Gerards, Pendeville-Samain, Muller, van Tienen and Smeets.)

Published
2020
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49. The Missing "lnc" between Genetics and Cardiac Disease.

Author

Azodi M, Kamps R, Heymans S, and Robinson EL

Abstract

: Cardiovascular disease (CVD) is one of the biggest threats to public health worldwide. Identifying key genetic contributors to CVD enables clinicians to assess the most effective treatment course and prognosis, as well as potentially inform family members. This often involves either whole exome sequencing (WES) or targeted panel analysis of known pathogenic genes. In the future, tailored or personalized therapeutic strategies may be implemented, such as gene therapy. With the recent revolution in deep sequencing technologies, we know that up to 90% of the human genome is transcribed, despite only 2% of the 6 billion DNA bases coding for proteins. The long non-coding RNA (lncRNA) "genes" make up an important and significant fraction of this "dark matter" of the genome. We highlight how, despite lncRNA genes exceeding that of classical protein-coding genes by number, the "non-coding" human genome is neglected when looking for genetic components of disease. WES platforms and pathogenic gene panels still do not cover even characterized lncRNA genes that are functionally involved in the pathophysiology of CVD. We suggest that the importance of lncRNAs in disease causation and progression be taken as seriously as that of pathogenic protein variants and mutations, and that this is maybe a new area of attention for clinical geneticists., Competing Interests: The authors declare no conflict of interest.

Published
2020
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50. Whole Exome Sequencing Is the Preferred Strategy to Identify the Genetic Defect in Patients With a Probable or Possible Mitochondrial Cause.

Author

Theunissen TEJ, Nguyen M, Kamps R, Hendrickx AT, Sallevelt SCEH, Gottschalk RWH, Calis CM, Stassen APM, de Koning B, Mulder-Den Hartog ENM, Schoonderwoerd K, Fuchs SA, Hilhorst-Hofstee Y, de Visser M, Vanoevelen J, Szklarczyk R, Gerards M, de Coo IFM, Hellebrekers DMEI, and Smeets HJM

Abstract

Mitochondrial disorders, characterized by clinical symptoms and/or OXPHOS deficiencies, are caused by pathogenic variants in mitochondrial genes. However, pathogenic variants in some of these genes can lead to clinical manifestations which overlap with other neuromuscular diseases, which can be caused by pathogenic variants in non-mitochondrial genes as well. Mitochondrial pathogenic variants can be found in the mitochondrial DNA (mtDNA) or in any of the 1,500 nuclear genes with a mitochondrial function. We have performed a two-step next-generation sequencing approach in a cohort of 117 patients, mostly children, in whom a mitochondrial disease-cause could likely or possibly explain the phenotype. A total of 86 patients had a mitochondrial disorder, according to established clinical and biochemical criteria. The other 31 patients had neuromuscular symptoms, where in a minority a mitochondrial genetic cause is present, but a non-mitochondrial genetic cause is more likely. All patients were screened for pathogenic variants in the mtDNA and, if excluded, analyzed by whole exome sequencing (WES). Variants were filtered for being pathogenic and compatible with an autosomal or X-linked recessive mode of inheritance in families with multiple affected siblings and/or consanguineous parents. Non-consanguineous families with a single patient were additionally screened for autosomal and X-linked dominant mutations in a predefined gene-set. We identified causative pathogenic variants in the mtDNA in 20% of the patient-cohort, and in nuclear genes in 49%, implying an overall yield of 68%. We identified pathogenic variants in mitochondrial and non-mitochondrial genes in both groups with, obviously, a higher number of mitochondrial genes affected in mitochondrial disease patients. Furthermore, we show that 31% of the disease-causing genes in the mitochondrial patient group were not included in the MitoCarta database, and therefore would have been missed with MitoCarta based gene-panels. We conclude that WES is preferable to panel-based approaches for both groups of patients, as the mitochondrial gene-list is not complete and mitochondrial symptoms can be secondary. Also, clinically and genetically heterogeneous disorders would require sequential use of multiple different gene panels. We conclude that WES is a comprehensive and unbiased approach to establish a genetic diagnosis in these patients, able to resolve multi-genic disease-causes.

Published
2018
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