Your search keyword '"Willemse, Marieke"' showing total 34 results

1. Ameliorated cellular hallmarks of myotonic dystrophy in hybrid myotubes from patient and unaffected donor cells

Author

Raaijmakers, Renée H.L., Ausems, C. Rosanne M., Willemse, Marieke, Cumming, Sarah A., van Engelen, Baziel G.M., Monckton, Darren G., van Bokhoven, Hans, and Wansink, Derick G.

Published

2024

2. Block or degrade? Balancing on- and off-target effects of antisense strategies against transcripts with expanded triplet repeats in DM1

Author

El Boujnouni, Najoua, van der Bent, M. Leontien, Willemse, Marieke, ’t Hoen, Peter A.C., Brock, Roland, and Wansink, Derick G.

Published

2023

3. Bosutinib in Resistant and Intolerant Pediatric Patients With Chronic Phase Chronic Myeloid Leukemia: Results From the Phase I Part of Study ITCC054/COG AAML1921.

Author

Brivio, Erica, Pennesi, Edoardo, Willemse, Marieke E., Huitema, Alwin D.R., Jiang, Yilin, van Tinteren, Harm D.R., van der Velden, Vincent H.J., Beverloo, Berna H., den Boer, Monique L., Rammeloo, Lukas A.J., Hudson, Chad, Heerema, Nyla, Kowalski, Karey, Zhao, Huadong, Kuttschreuter, Luke, Bautista Sirvent, Francisco J., Bukowinski, Andrew, Rizzari, Carmelo, Pollard, Jessica, and Murillo-Sanjuán, Laura

Published

2024

4. The PedAL/EuPAL Project: A Global Initiative to Address the Unmet Medical Needs of Pediatric Patients with Relapsed or Refractory Acute Myeloid Leukemia.

Author

Ceolin, Valeria, Ishimaru, Sae, Karol, Seth E., Bautista, Francisco, Goemans, Bianca Frederika, Gueguen, Gwenaëlle, Willemse, Marieke, Di Laurenzio, Laura, Lukin, Jennifer, van Tinteren, Harm, Locatelli, Franco, Petit, Arnaud, Tomizawa, Daisuke, Norton, Alice, Kaspers, Gertjan, Reinhardt, Dirk, Tasian, Sarah K., Nichols, Gwen, Kolb, Edward Anders, and Zwaan, Christian Michel

Subjects

BIOMARKERS, REPORTING of diseases, DRUG efficacy, CLINICAL trials, PEDIATRICS, PROGNOSIS, DISEASE relapse, LYMPHOMAS, NEEDS assessment, MEDICAL needs assessment, PATIENT safety

Abstract

Simple Summary: The prognosis of children with relapsed/refractory (R/R) acute myeloid leukemia (AML) remains poor, and innovative treatments are needed. Most drugs approved for adults with AML over the last decade are not available or not licensed for use in children. Clinical trials in pediatric AML to assess the safety and/or efficacy of new drugs may take a long time to recruit given smaller patient numbers. The overarching aim of the Pediatric Acute Leukemia (PedAL) program, supported by the Leukemia and Lymphoma Society as part of its Dare to Dream Project, is to establish new standards of care for children with R/R AML via international collaboration in Europe, North America, and Asia-Pacific to accelerate clinical trial conduction, increase access to promising new therapies, and create a registry of uniformly-collected data. These efforts will facilitate biomarker-driven approaches of targeted therapies, of which an overview is provided in this manuscript, with the intent to obtain regulatory approvals. The prognosis of children with acute myeloid leukemia (AML) has improved incrementally over the last few decades. However, at relapse, overall survival (OS) is approximately 40–50% and is even lower for patients with chemo-refractory disease. Effective and less toxic therapies are urgently needed for these children. The Pediatric Acute Leukemia (PedAL) program is a strategic global initiative that aims to overcome the obstacles in treating children with relapsed/refractory acute leukemia and is supported by the Leukemia and Lymphoma Society in collaboration with the Children's Oncology Group, the Innovative Therapies for Children with Cancer consortium, and the European Pediatric Acute Leukemia (EuPAL) foundation, amongst others. In Europe, the study is set up as a complex clinical trial with a stratification approach to allocate patients to sub-trials of targeted inhibitors at relapse and employing harmonized response and safety definitions across sub-trials. The PedAL/EuPAL international collaboration aims to determine new standards of care for AML in a first and second relapse, using biology-based selection markers for treatment stratification, and deliver essential data to move drugs to front-line pediatric AML studies. An overview of potential treatment targets in pediatric AML, focused on drugs that are planned to be included in the PedAL/EuPAL project, is provided in this manuscript. [ABSTRACT FROM AUTHOR]

Published

2024

5. Independent prognostic value of BCR-ABL1-like signature and IKZF1 deletion, but not high CRLF2 expression, in children with B-cell precursor ALL

Author

van der Veer, Arian, Waanders, Esmé, Pieters, Rob, Willemse, Marieke E., Van Reijmersdal, Simon V., Russell, Lisa J., Harrison, Christine J., Evans, William E., van der Velden, Vincent H.J., Hoogerbrugge, Peter M., Van Leeuwen, Frank, Escherich, Gabriele, Horstmann, Martin A., Mohammadi Khankahdani, Leila, Rizopoulos, Dimitris, De Groot-Kruseman, Hester A., Sonneveld, Edwin, Kuiper, Roland P., and Den Boer, Monique L.

Published

2013

6. Intracellular NAD(H) levels control motility and invasion of glioma cells

Author

van Horssen, Remco, Willemse, Marieke, Haeger, Anna, Attanasio, Francesca, Güneri, Tuba, Schwab, Albrecht, Stock, Christian M., Buccione, Roberto, Fransen, Jack A. M., and Wieringa, Bé

Published

2013

7. Disturbed CXCR4/CXCL12 axis in paediatric precursor B-cell acute lymphoblastic leukaemia

Author

van den Berk, Lieke C. J., van der Veer, Arian, Willemse, Marieke E., Theeuwes, Myrte J. G. A., Luijendijk, Mirjam W., Tong, Wing H., van der Sluis, Inge M., Pieters, Rob, and den Boer, Monique L.

Published

2014

8. Increased OXPHOS activity precedes rise in glycolytic rate in H-RasV12/E1A transformed fibroblasts that develop a Warburg phenotype

Author

Pluk Helma, Oerlemans Frank, Smift Amy L, Winer Mike, Wu Min, Willemse Marieke, van Dommelen Michiel MT, te Lindert Mariska M, de Groof Ad JC, Fransen Jack AM, and Wieringa Bé

Subjects

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

Abstract

Abstract Background The Warburg phenotype in cancer cells has been long recognized, but there is still limited insight in the consecutive metabolic alterations that characterize its establishment. We obtained better understanding of the coupling between metabolism and malignant transformation by studying mouse embryonic fibroblast-derived cells with loss-of-senescence or H-RasV12/E1A-transformed phenotypes at different stages of oncogenic progression. Results Spontaneous immortalization or induction of senescence-bypass had only marginal effects on metabolic profiles and viability. In contrast, H-RasV12/E1A transformation initially caused a steep increase in oxygen consumption and superoxide production, accompanied by massive cell death. During prolonged culture in vitro, cell growth rate increased gradually, along with tumor forming potential in in vitro anchorage-independent growth assays and in vivo tumor formation assays in immuno-deficient mice. Notably, glucose-to-lactic acid flux increased with passage number, while cellular oxygen consumption decreased. This conversion in metabolic properties was associated with a change in mitochondrial NAD+/NADH redox, indicative of decreased mitochondrial tricarboxic acid cycle and OXPHOS activity. Conclusion The high rate of oxidative metabolism in newly transformed cells is in marked contrast with the high glycolytic rate in cells in the later tumor stage. In our experimental system, with cells growing under ambient oxygen conditions in nutrient-rich media, the shift towards this Warburg phenotype occurred as a step-wise adaptation process associated with augmented tumorigenic capacity and improved survival characteristics of the transformed cells. We hypothesize that early-transformed cells, which potentially serve as founders for new tumor masses may escape therapies aimed at metabolic inhibition of tumors with a fully developed Warburg phenotype.

Published

2009

9. P676: UPDATED RESULTS FROM THE TRIAL ITCC‐054/COG‐AAML1921: BOSUTINIB IN NEWLY DIAGNOSED AND RESISTANT/INTOLERANT PEDIATRIC PATIENTS WITH CHRONIC MYELOID LEUKEMIA.

Author

Brivio, Erica, Pennesi, Edoardo, Willemse, Marieke, Jiang, Yilin, van der Velden, Vincent, Beverloo, Berna, Hudson, Chad, Kuttschreuter, Luke, van der Sluis, Inge, Brethon, Benoît, Bautista, Francisco, J. Burke, Michael, Heerema, Nyla, Bukowinski, Andrew, Cooper, Stacy, Pollard, Jessica, Nagasubramani, Ramamoorthy, Redell, Michele, Bourquin, Jean‐Pierre, and Pais, Ray

Published

2023

10. (CTG)n repeat-mediated dysregulation of MBNL1 and MBNL2 expression during myogenesis in DM1 occurs already at the myoblast stage.

Author

André, Laurène M., van Cruchten, Remco T. P., Willemse, Marieke, and Wansink, Derick G.

Subjects

MYOBLASTS, RNA metabolism, PROGENITOR cells, MUSCLE cells, CELL nuclei, DEVELOPMENTAL biology

Abstract

Myotonic dystrophy type 1 (DM1) is a severe neuromuscular disorder caused by the expression of trinucleotide repeat-containing DMPK transcripts. Abnormally expanded (CUG)n repeats in these transcripts form hairpin-like structures that cause the RNA to accumulate in the cell nucleus by sequestering isoforms of the Muscleblind (MBNL) family, tissue-specific regulators of developmentally programmed, post-transcriptional processes in RNA metabolism. Through this mechanism, the function of MBNL in RNA processing becomes dominantly perturbed, which eventually leads to aberrant alternative splicing and the expression of foetal splice variants of a wide variety of proteins, including the MBNL isoforms themselves. Here, we employ a patient-derived muscle cell model for DM1 to examine in detail the expression of MBNL RNA and protein variants during myogenic differentiation. This DM1 model consists of a panel of isogenic myoblast cell lines that either contain a pathogenic DMPK allele with a congenital mutation of 2600 triplets, or lack this expanded repeat through CRISPR/Cas9-mediated gene editing. We found that the temporal expression levels of MBNL1, MBNL2 and MBNL3 RNAs are not influenced by presence of the (CTG)2600 repeat during myogenesis in vitro. However, throughout myoblast proliferation and differentiation to myotubes a disproportionate inclusion of MBNL1 exon 5 and MBNL2 exons 5 and 8 occurs in cells with the (CTG)2600 repeat. As a consequence, a reduced quantity and imbalanced collection of splice variants of MBNL1 and MBNL2 accumulates in both the cytoplasm and the nucleus of DM1 myoblasts and myotubes. We thus propose that both the quantitative and qualitative changes in the intracellular partitioning of MBNL proteins are a pivotal cause of skeletal muscle problems in DM1, starting already in muscle progenitor cells. [ABSTRACT FROM AUTHOR]

Published

2019

11. Super-Resolution Correlative Light and Electron Microscopy (SR-CLEM) Reveals Novel Ultrastructural Insights Into Dendritic Cell Podosomes.

Author

Joosten, Ben, Cambi, Alessandra, van den Dries, Koen, Willemse, Marieke, and Fransen, Jack

Subjects

CYTOSKELETAL proteins, TISSUES, DENDRITIC cells, ADAPTOR proteins, VINCULIN, ZYXIN, MICROSCOPY, CELL membranes

Abstract

Podosomes are multimolecular cytoskeletal structures that coordinate the migration of tissue-resident dendritic cells (DCs). They consist of a protrusive actin-rich core and an adhesive integrin-rich ring that contains adaptor proteins such as vinculin and zyxin. Individual podosomes are typically interconnected by a dense network of actin filaments giving rise to large podosome clusters. The actin density in podosome clusters complicates the analysis of podosomes by light microscopy alone. Here, we present an optimized procedure for performing super-resolution correlative light and electron microscopy (SR-CLEM) to study the organization of multiple proteins with respect to actin in podosome clusters at the ventral plasma membrane of DCs. We demonstrate that our procedure is suited to correlate at least three colors in super-resolution Airyscan microscopy with scanning electron microscopy (SEM). Using this procedure, we first reveal an intriguing complexity in the organization of ventral and radiating actin filaments in clusters formed by DCs which was not properly detected before by light microscopy alone. Next, we demonstrate a differential organization of vinculin and zyxin with respect to the actin filaments at podosomes. While vinculin mostly resides at sites where the actin filaments connect to the cell membrane, zyxin is primarily associated with filaments close to and on top of the core. Finally, we reveal a novel actin-based structure with SEM that connects closely associated podosome cores and which may be important for podosome topography sensing. Interestingly, these interpodosomal connections, in contrast to the radiating and ventral actin filaments appear to be insensitive to inhibition of actin polymerization suggesting that these pools of actin are not dynamically coupled. Together, our work demonstrates the power of correlating different imaging modalities for studying multimolecular cellular structures and could potentially be further exploited to study processes at the ventral plasma membrane of immune cells such as clathrin-mediated endocytosis or immune synapse formation. [ABSTRACT FROM AUTHOR]

Published

2018

12. Preliminary results from the first-in-child phase II trial (ITCC-054/COG-AAML1921) of bosutinib in pediatric patients with newly diagnosed (ND) chronic myeloid leukemia (CML).

Author

Pennesi, Edoardo, Brivio, Erica, Willemse, Marieke E, Jiang, Yilin, van der Velden, Vincent HJ, Beverloo, H Berna, Hudson, Chad, Heerema, Nyla A, Kuttschreuter, Luke, Frediani, Jamie, Spiller, Susan, Batra, Sandeep, Redell, Michele, Bertorello, Nicoletta, Locatelli, Franco, van der Sluis, Inge M, Roth, Michael, Hijiya, Nobuko, and Zwaan, C Michel

Published

2023

13. Disturbed CXCR4/ CXCL12 axis in paediatric precursor B-cell acute lymphoblastic leukaemia.

Author

Berk, Lieke C. J., Veer, Arian, Willemse, Marieke E., Theeuwes, Myrte J. G. A., Luijendijk, Mirjam W., Tong, Wing H., Sluis, Inge M., Pieters, Rob, and Boer, Monique L.

Subjects

LYMPHOBLASTIC leukemia in children, BONE marrow, CXCR4 receptors, B cell lymphoma, HEMATOPOIETIC stem cells, LEUKEMIA treatment

Abstract

Malignant cells infiltrating the bone marrow ( BM) interfere with normal cellular behaviour of supporting cells, thereby creating a malignant niche. We found that CXCR4-receptor expression was increased in paediatric precursor B-cell acute lymphoblastic leukaemia ( BCP- ALL) cells compared with normal mononuclear haematopoietic cells ( P < 0·0001). Furthermore, high CXCR4-expression correlated with an unfavourable outcome in BCP- ALL (5-year cumulative incidence of relapse ± standard error: 38·4% ± 6·9% in CXCR4-high versus 12% ± 4·6% in CXCR4-low expressing cases, P < 0·0001). Interestingly, BM levels of the CXCR4-ligand ( CXCL12) were 2·7-fold lower ( P = 0·005) in diagnostic BCP- ALL samples compared with non-leukaemic controls. Induction chemotherapy restored CXCL12 levels to normal. Blocking the CXCR4-receptor with Plerixafor showed that the lower CXCL12 serum levels at diagnosis could not be explained by consumption by the leukaemic cells, nor did we observe an altered CXCL12-production capacity of BM-mesenchymal stromal cells ( BM- MSC) at this time-point. We rather observed that a very high density of leukaemic cells negatively affected CXCL12-production by the BM- MSC while stimulating the secretion levels of granulocyte colony-stimulating factor (G- CSF). These results suggest that highly proliferative leukaemic cells are able to down-regulate secretion of cytokines involved in homing ( CXCL12), while simultaneously up-regulating those involved in haematopoietic mobilization (G- CSF). Therefore, interference with the CXCR4/ CXCL12 axis may be an effective way to mobilize BCP- ALL cells. [ABSTRACT FROM AUTHOR]

Published

2014

14. NAMPT-Mediated Salvage Synthesis of NAD+ Controls Morphofunctional Changes of Macrophages.

Author

Venter, Gerda, Oerlemans, Frank T. J. J., Willemse, Marieke, Wijers, Mietske, Fransen, Jack A. M., and Wieringa, Bé

Subjects

MACROPHAGES, CYTOSKELETON, NICOTINAMIDE adenine dinucleotide phosphate, PHOSPHORIBOSYLTRANSFERASES, CYTOKINES, ENZYME regulation

Abstract

Functional morphodynamic behavior of differentiated macrophages is strongly controlled by actin cytoskeleton rearrangements, a process in which also metabolic cofactors ATP and NAD(H) (i.e. NAD+ and NADH) and NADP(H) (i.e. NADP+ and NADPH) play an essential role. Whereas the link to intracellular ATP availability has been studied extensively, much less is known about the relationship between actin cytoskeleton dynamics and intracellular redox state and NAD+-supply. Here, we focus on the role of nicotinamide phosphoribosyltransferase (NAMPT), found in extracellular form as a cytokine and growth factor, and in intracellular form as one of the key enzymes for the production of NAD+ in macrophages. Inhibition of NAD+ salvage synthesis by the NAMPT-specific drug FK866 caused a decrease in cytosolic NAD+ levels in RAW 264.7 and Maf-DKO macrophages and led to significant downregulation of the glycolytic flux without directly affecting cell viability, proliferation, ATP production capacity or mitochondrial respiratory activity. Concomitant with these differential metabolic changes, the capacity for phagocytic ingestion of particles and also substrate adhesion of macrophages were altered. Depletion of cytoplasmic NAD+ induced cell-morphological changes and impaired early adhesion in phagocytosis of zymosan particles as well as spreading performance. Restoration of NAD+ levels by NAD+, NMN, or NADP+ supplementation reversed the inhibitory effects of FK866. We conclude that direct coupling to local, actin-based, cytoskeletal dynamics is an important aspect of NAD+’s cytosolic role in the regulation of morphofunctional characteristics of macrophages. [ABSTRACT FROM AUTHOR]

Published

2014

15. Glucose Controls Morphodynamics of LPS-Stimulated Macrophages.

Author

Venter, Gerda, Oerlemans, Frank T. J. J., Wijers, Mietske, Willemse, Marieke, Fransen, Jack A. M., and Wieringa, Bé

Subjects

ZYMOSAN, MACROPHAGES, OXIDATIVE phosphorylation, POST-translational modification, ACTIN, GLYCOLYSIS

Abstract

Macrophages constantly undergo morphological changes when quiescently surveying the tissue milieu for signs of microbial infection or damage, or after activation when they are phagocytosing cellular debris or foreign material. These morphofunctional alterations require active actin cytoskeleton remodeling and metabolic adaptation. Here we analyzed RAW 264.7 and Maf-DKO macrophages as models to study whether there is a specific association between aspects of carbohydrate metabolism and actin-based processes in LPS-stimulated macrophages. We demonstrate that the capacity to undergo LPS-induced cell shape changes and to phagocytose complement-opsonized zymosan (COZ) particles does not depend on oxidative phosphorylation activity but is fueled by glycolysis. Different macrophage activities like spreading, formation of cell protrusions, as well as phagocytosis of COZ, were thereby strongly reliant on the presence of low levels of extracellular glucose. Since global ATP production was not affected by rewiring of glucose catabolism and inhibition of glycolysis by 2-deoxy-D-glucose and glucose deprivation had differential effects, our observations suggest a non-metabolic role for glucose in actin cytoskeletal remodeling in macrophages, e.g. via posttranslational modification of receptors or signaling molecules, or other effects on the machinery that drives actin cytoskeletal changes. Our findings impute a decisive role for the nutrient state of the tissue microenvironment in macrophage morphodynamics. [ABSTRACT FROM AUTHOR]

Published

2014

16. Disturbed CXCR4/CXCL12 Axis In Pediatric Precursor B-Cell Acute Lymphoblastic Leukemia

Author

van den Berk, Lieke C.J., Veer, Arian van der, Willemse, Marieke E., Theeuwes, Myrte J.G.A., Luijendijk, Mirjam W., Tong, Wing H., van der Sluis, Inge M., Pieters, Rob, and den Boer, Monique L.

Published

2013

17. Intracellular NAD(H) levels control motility and invasion of glioma cells.

Author

Horssen, Remco, Willemse, Marieke, Haeger, Anna, Attanasio, Francesca, Güneri, Tuba, Schwab, Albrecht, Stock, Christian, Buccione, Roberto, Fransen, Jack, and Wieringa, Bé

Subjects

*INTRACELLULAR membranes, *GLIOMAS, *NICOTINAMIDE, *PHOSPHORIBOSYLTRANSFERASES, *PHARMACOLOGY, *NEOPLASTIC cell transformation

Abstract

Oncogenic transformation involves reprogramming of cell metabolism, whereby steady-state levels of intracellular NAD and NADH can undergo dramatic changes while ATP concentration is generally well maintained. Altered expression of nicotinamide phosphoribosyltransferase (NAMPT), the rate-limiting enzyme of NAD-salvage, accompanies the changes in NAD(H) during tumorigenesis. Here, we show by genetic and pharmacological inhibition of NAMPT in glioma cells that fluctuation in intracellular [NAD(H)] differentially affects cell growth and morphodynamics, with motility/invasion capacity showing the highest sensitivity to [NAD(H)] decrease. Extracellular supplementation of NAD or re-expression of NAMPT abolished the effects. The effects of NAD(H) decrease on cell motility appeared parallel coupled with diminished pyruvate-lactate conversion by lactate dehydrogenase (LDH) and with changes in intracellular and extracellular pH. The addition of lactic acid rescued and knockdown of LDH-A replicated the effects of [NAD(H)] on motility. Combined, our observations demonstrate that [NAD(H)] is an important metabolic component of cancer cell motility. Nutrient or drug-mediated modulation of NAD(H) levels may therefore represent a new option for blocking the invasive behavior of tumors. [ABSTRACT FROM AUTHOR]

Published

2013

18. APT Changes the Fluorescence Lifetime of Cyan Fluorescent Protein via an Interaction with His148.

Author

Borst, Jan Willem, Willemse, Marieke, Slijkhuis, Rik, van der Krogt, Gerard, Laptenok, Sergey P., Jalink, Kees, Wieringa, Be, and Fransen, Jack A. M.

Subjects

*ADENOSINE triphosphate, *FLUORIMETRY, *FLUORESCENCE, *FLUORESCENCE spectroscopy, *PROTEIN-protein interactions, *CERULEAN warbler, *ELECTROSTATIC adhesion, *HISTIDINE, *ASPARTIC acid

Abstract

Recently, we described that ATP induces changes in YFP/CFP fluorescence intensities of Fluorescence Resonance Energy Transfer (FRET) sensors based on CFP-YFP. To get insight into this phenomenon, we employed fluorescence lifetime spectroscopy to analyze the influence of ATP on these fluorescent proteins in more detail. Using different donor and acceptor pairs we found that ATP only affected the CFP-YFP based versions. Subsequent analysis of purified monomers of the used proteins showed that ATP has a direct effect on the fluorescence lifetime properties of CFP. Since the fluorescence lifetime analysis of CFP is rather complicated by the existence of different lifetimes, we tested a variant of CFP, i.e. Cerulean, as a monomer and in our FRET constructs. Surprisingly, this CFP variant shows no ATP concentration dependent changes in the fluorescence lifetime. The most important difference between CFP and Cerulean is a histidine residue at position 148. Indeed, changing this histidine in CFP into an aspartic acid results in identical fluorescence properties as observed for the Cerulean fluorescent based FRET sensor. We therefore conclude that the changes in fluorescence lifetime of CFP are affected specifically by possible electrostatic interactions of the negative charge of ATP with the positively charged histidine at position 148. Clearly, further physicochemical characterization is needed to explain the sensitivity of CFP fluorescence properties to changes in environmental (i.e. ATP concentrations) conditions. [ABSTRACT FROM AUTHOR]

Published

2010

19. Leukemia Cells with a BCR-ABL1-Like signature and/or IKZF1 deletions, but Not High CRLF2 Expression, Are Predictive of an Unfavorable Prognosis in Childhood B Cell Precursor Acute Lymphoblastic Leukemia

Author

Van Der Veer, Arian, Waanders, Esmee, Pieters, Rob, Willemse, Marieke E., Reijmersdaal, Simon, Russell, Lisa J, Harrison, Christine J, Evans, William E., van der Velden, Vincent H.J., Hoogerbrugge, Peter M., van Leeuwen, Frank N., Escherich, G., Horstman, Martin, Khankahdani, Leila mohammadi, Rizopoulos, Dimitris, de Groot-Kruseman, Hester A., Sonneveld, Edwin, Kuiper, Roland P., and Den Boer, Monique L.

Published

2012

20. Unfavorable Prognostic Value of IKAROS but Not CRLF2 in Children with BCRABL1-positive Acute Lymphoblastic Leukemia,

Author

Veer, Arian Van Der, Willemse, Marieke E., De Haas, Valerie, Veerman, Anjo J.P., Kamps, Willem A., Pieters, Rob, and Boer, Monique L. Den

Published

2011

21. ATP and FRET—a cautionary note.

Author

Willemse, Marieke, Janssen, Edwin, de Lange, Frank, Wieringa, Bé, and Fransen, Jack

Subjects

*LETTERS to the editor, *ADENOSINE triphosphatase

Abstract

A letter to the editor is presented on several articles on adenosine triphosphate (ATP) and the use of biosensors based on fluorescence resonance energy transfer (FRET) that were published in the previous issues.

Published

2007

22. Recovery in the Myogenic Program of Congenital Myotonic Dystrophy Myoblasts after Excision of the Expanded (CTG)n Repeat.

Author

André, Laurène M., van Cruchten, Remco T.P., Willemse, Marieke, Bezstarosti, Karel, Demmers, Jeroen A.A., van Agtmaal, Ellen L., Wansink, Derick G., and Wieringa, Bé

Subjects

MYOTONIA atrophica, MYOBLASTS, GENOME editing, GENE therapy, PROTEOMICS, IN vitro studies

Abstract

The congenital form of myotonic dystrophy type 1 (cDM) is caused by the large-scale expansion of a (CTG•CAG)n repeat in DMPK and DM1-AS. The production of toxic transcripts with long trinucleotide tracts from these genes results in impairment of the myogenic differentiation capacity as cDM's most prominent morpho-phenotypic hallmark. In the current in vitro study, we compared the early differentiation programs of isogenic cDM myoblasts with and without a (CTG)2600 repeat obtained by gene editing. We found that excision of the repeat restored the ability of cDM myoblasts to engage in myogenic fusion, preventing the ensuing myotubes from remaining immature. Although the cDM-typical epigenetic status of the DM1 locus and the expression of genes therein were not altered upon removal of the repeat, analyses at the transcriptome and proteome level revealed that early abnormalities in the temporal expression of differentiation regulators, myogenic progression markers, and alternative splicing patterns before and immediately after the onset of differentiation became normalized. Our observation that molecular and cellular features of cDM are reversible in vitro and can be corrected by repeat-directed genome editing in muscle progenitors, when already committed and poised for myogenic differentiation, is important information for the future development of gene therapy for different forms of myotonic dystrophy type 1 (DM1). [ABSTRACT FROM AUTHOR]

Published

2019

23. The nuclear concentration required for antisense oligonucleotide activity in myotonic dystrophy cells.

Author

van der Bent, M. Leontien, da Silva Filho, Omar Paulino, Willemse, Marieke, Hällbrink, Mattias, Wansink, Derick G., and Brock, Roland

Published

2019

24. Cancer cell metabolism regulates extracellular matrix degradation by invadopodia

Author

van Horssen, Remco, Buccione, Roberto, Willemse, Marieke, Cingir, Sahika, Wieringa, Bé, and Attanasio, Francesca

Subjects

*CANCER cells, *CELL metabolism, *EXTRACELLULAR matrix, *CELL membrane abnormalities, *CELL transformation, *GLYCOLYSIS, *PHENOTYPES

Abstract

Abstract: Transformed cancer cells have an altered metabolism, characterized by a shift towards aerobic glycolysis, referred to as ‘the Warburg phenotype’. A change in flux through mitochondrial OXPHOS and cytosolic pathways for ATP production and a gain of capacity for biomass production in order to sustain the needs for altered growth and morphodynamics are typically involved in this global rewiring of cancer cell metabolism. Characteristically, these changes in metabolism are accompanied by enhanced uptake of nutrients like glucose and glutamine. Here we focus on the relationship between cell metabolism and cell dynamics, in particular the formation and function of invadopodia, specialized structures for focal degradation of the extracellular matrix. Since we recently found presence of enzymes that are active in glycolysis and associated pathways in invadopodia, we hypothesize that metabolic adaptation and invadopodia formation are linked processes. We give an overview on the background for this idea and show for the first time that extracellular matrix degradation by invadopodia can be differentially manipulated, without effects on cell proliferation, by use of metabolic inhibitors or changes in nutrient composition of cell culture media. We conclude that cell metabolism and carbohydrate availability, especially pyruvate, are involved in fuelling of invadopodia formation and activity. [Copyright &y& Elsevier]

Published

2013

25. Submembranous recruitment of creatine kinase B supports formation of dynamic actin-based protrusions of macrophages and relies on its C-terminal flexible loop.

Author

Venter, Gerda, Polling, Saskia, Pluk, Helma, Venselaar, Hanka, Wijers, Mietske, Willemse, Marieke, Fransen, Jack A.M., and Wieringa, Bé

Subjects

*CREATINE kinase, *ACTIN, *MACROPHAGES, *C-terminal residues, *ADENOSINE triphosphate, *CATALYTIC activity, *BIOINFORMATICS

Abstract

Subcellular partitioning of creatine kinase contributes to the formation of patterns in intracellular ATP distribution and the fuelling of cellular processes with a high and sudden energy demand. We have previously shown that brain-type creatine kinase (CK-B) accumulates at the phagocytic cup in macrophages where it is involved in the compartmentalized generation of ATP for actin remodeling. Here, we report that CK-B catalytic activity also helps in the formation of protrusive ruffle structures which are actin-dependent and abundant on the surface of both unstimulated and LPS-activated macrophages. Recruitment of CK-B to these structures occurred transiently and inhibition of the enzyme's catalytic activity with cyclocreatine led to a general smoothening of surface morphology as visualized by scanning electron microscopy. Comparison of the dynamics of distribution of YFP-tagged CK-mutants and isoforms by live imaging revealed that amino acid residues in the C-terminal segment (aa positions 323–330) that forms one of the protein's two mobile loops are involved in partitioning over inner regions of the cytosol and nearby sites where membrane protrusions occur during induction of phagocytic cup formation. Although wt CK-B, muscle-type CK (CK-M), and a catalytically dead CK-B-E232Q mutant with intact loop region were normally recruited from the cytosolic pool, no dynamic transition to the phagocytic cup area was seen for the CK-homologue arginine kinase and a CK-B-D326A mutant protein. Bioinformatics analysis helped us to predict that conformational flexibility of the C-terminal loop, independent of conformational changes induced by substrate binding or catalytic activity, is likely involved in exposing the enzyme for binding at or near the sites of membrane protrusion formation. [ABSTRACT FROM AUTHOR]

Published

2015

26. Detection of 2-O-Sulfated Iduronate and N-Acetylglucosamine Units in Heparan Sulfate by an Antibody Selected against Acharan Sulfate (IdoA2S-GlcNAc)n.

Author

ten Dam, Gerdy B., van de Westerlo, Els M.A., Smetsers, Toon F.C.M., Willemse, Marieke, van Muijen, Goos N.P., Merry, Catherine L.R., Gallagher, John T., Kim, Yeong S., and van Kuppevelt, Tom H.

Subjects

*GLUCOSAMINE, *OLIGOSACCHARIDES, *AMINO acids, *ORGANIC acids, *AMINO acid sequence, *PROTEIN analysis, *ANTICOAGULANTS, *NEUROENDOCRINE tumors

Abstract

The snail glycosaminoglycan acharan sulfate (AS) is structurally related to heparan sulfates (HS) and has a repeating disaccharide structure of α-D-N-acetylglucosaminyl-2-O-sulfo-α-L-iduronic acid (GlcNAc-IdoA2S) residues. Using the phage display technology, a unique antibody (MW3G3) was selected against AS with a VH3, DP 47, and a CDR3 amino acid sequence of QKKRPRF. Antibody MW3G3 did not react with desulfated, N-deacetylated or N-sulfated AS, indicating that reactivity depends on N-acetyl and 2-O-sulfate groups. Antibody MW3G3 also had a high preference for (modified) heparin oligosaccharides containing N-acetylated glucosamine and 2-O-sulfated iduronic acid residues. In tissues, antibody MW3G3 identified a HS oligosaccharide epitope containing N-acetylated glucosamine and 2-O-sulfated iduronic acid residues as enzymatic N-deacetylation of HS in situ prevented staining, and 2-O-sulfotransferase-deficient Chinese hamster ovary cells were not reactive. An immunohistochemical survey using various rat organs revealed a distinct distribution of the MW3G3 epitope, which was primarily present in the basal laminae of most (but not all) blood vessels and of some epithelia, including human skin. No staining was observed in the glycosaminoglycan-rich tumor matrix of metastatic melanoma. In conclusion, we have selected an antibody that identifies HS oligosaccharides containing N-acetylated glucosamine and 2-O-sulfated iduronic acid residues. This antibody may be instrumental in identifying structural alterations in HS in health and disease. [ABSTRACT FROM AUTHOR]

Published

2004

27. The PedAL/EuPAL Project: A Global Initiative to Address the Unmet Medical Needs of Pediatric Patients with Relapsed or Refractory Acute Myeloid Leukemia.

Author

Ceolin V, Ishimaru S, Karol SE, Bautista F, Goemans BF, Gueguen G, Willemse M, Di Laurenzio L, Lukin J, van Tinteren H, Locatelli F, Petit A, Tomizawa D, Norton A, Kaspers G, Reinhardt D, Tasian SK, Nichols G, Kolb EA, Zwaan CM, and Cooper TM

Abstract

The prognosis of children with acute myeloid leukemia (AML) has improved incrementally over the last few decades. However, at relapse, overall survival (OS) is approximately 40-50% and is even lower for patients with chemo-refractory disease. Effective and less toxic therapies are urgently needed for these children. The Pediatric Acute Leukemia (PedAL) program is a strategic global initiative that aims to overcome the obstacles in treating children with relapsed/refractory acute leukemia and is supported by the Leukemia and Lymphoma Society in collaboration with the Children's Oncology Group, the Innovative Therapies for Children with Cancer consortium, and the European Pediatric Acute Leukemia (EuPAL) foundation, amongst others. In Europe, the study is set up as a complex clinical trial with a stratification approach to allocate patients to sub-trials of targeted inhibitors at relapse and employing harmonized response and safety definitions across sub-trials. The PedAL/EuPAL international collaboration aims to determine new standards of care for AML in a first and second relapse, using biology-based selection markers for treatment stratification, and deliver essential data to move drugs to front-line pediatric AML studies. An overview of potential treatment targets in pediatric AML, focused on drugs that are planned to be included in the PedAL/EuPAL project, is provided in this manuscript.

Published

2023

28. Recovery in the Myogenic Program of Congenital Myotonic Dystrophy Myoblasts after Excision of the Expanded (CTG) n Repeat.

Author

André LM, van Cruchten RTP, Willemse M, Bezstarosti K, Demmers JAA, van Agtmaal EL, Wansink DG, and Wieringa B

Subjects

Cell Line, Epigenesis, Genetic, Gene Editing, Genetic Therapy, Humans, Muscle Development, Myoblasts cytology, Myoblasts metabolism, Myotonic Dystrophy pathology, Myotonic Dystrophy therapy, Myotonin-Protein Kinase genetics, Myoblasts pathology, Myotonic Dystrophy genetics, Trinucleotide Repeats

Abstract

The congenital form of myotonic dystrophy type 1 (cDM) is caused by the large-scale expansion of a (CTG•CAG) n repeat in DMPK and DM1-AS . The production of toxic transcripts with long trinucleotide tracts from these genes results in impairment of the myogenic differentiation capacity as cDM's most prominent morpho-phenotypic hallmark. In the current in vitro study, we compared the early differentiation programs of isogenic cDM myoblasts with and without a (CTG)2600 repeat obtained by gene editing. We found that excision of the repeat restored the ability of cDM myoblasts to engage in myogenic fusion, preventing the ensuing myotubes from remaining immature. Although the cDM-typical epigenetic status of the DM1 locus and the expression of genes therein were not altered upon removal of the repeat, analyses at the transcriptome and proteome level revealed that early abnormalities in the temporal expression of differentiation regulators, myogenic progression markers, and alternative splicing patterns before and immediately after the onset of differentiation became normalized. Our observation that molecular and cellular features of cDM are reversible in vitro and can be corrected by repeat-directed genome editing in muscle progenitors, when already committed and poised for myogenic differentiation, is important information for the future development of gene therapy for different forms of myotonic dystrophy type 1 (DM1).

Published

2019

29. Intrinsic Myogenic Potential of Skeletal Muscle-Derived Pericytes from Patients with Myotonic Dystrophy Type 1.

Author

Ausems CRM, Raaijmakers RHL, van den Broek WJAA, Willemse M, van Engelen BGM, Wansink DG, and van Bokhoven H

Abstract

Pericytes are multipotent, vessel-associated progenitors that exhibit high proliferative capacity, can cross the blood-muscle barrier, and have the ability to home to muscle tissue and contribute to myogenesis. Consequently, pericyte-based therapies hold great promise for muscular dystrophies. A complex multi-system disorder exhibiting muscular dystrophy for which pericytes might be a valuable cell source is myotonic dystrophy type 1 (DM1). DM1 is caused by an unstable (CTG)n repeat in the DMPK gene and characterized by skeletal muscle weakness, muscle wasting, and myotonia. We have successfully isolated alkaline phosphatase-positive pericytes from skeletal muscle of DM1 patients and a transgenic mouse model. Intranuclear (CUG)n RNA foci, a pathogenic DM1 hallmark, were identified in human and mouse pericytes. Notably, pericytes from DM1 patients maintained similar growth parameters and innate myogenic characteristics in vitro compared to cells from unaffected controls. Our in vitro results thus demonstrate the potential of pericytes to ameliorate muscle features in DM1 in a therapeutic setting., (© 2019 The Author(s).)

Published

2019

30. CRISPR/Cas9-Induced (CTG⋅CAG) n Repeat Instability in the Myotonic Dystrophy Type 1 Locus: Implications for Therapeutic Genome Editing.

Author

van Agtmaal EL, André LM, Willemse M, Cumming SA, van Kessel IDG, van den Broek WJAA, Gourdon G, Furling D, Mouly V, Monckton DG, Wansink DG, and Wieringa B

Subjects

Animals, Bacterial Proteins genetics, Base Sequence, CRISPR-Associated Protein 9, Clustered Regularly Interspaced Short Palindromic Repeats, Codon, Disease Models, Animal, Endonucleases genetics, Fibroblasts metabolism, Gene Expression, Gene Order, Genetic Loci, Humans, Mice, RNA, Guide, CRISPR-Cas Systems, RNA, Messenger genetics, RNA, Messenger metabolism, Sequence Deletion, CRISPR-Cas Systems, Gene Editing, Genomic Instability, Myotonic Dystrophy genetics, Myotonin-Protein Kinase genetics, Trinucleotide Repeat Expansion, Trinucleotide Repeats

Abstract

Myotonic dystrophy type 1 (DM1) is caused by (CTG⋅CAG) n -repeat expansion within the DMPK gene and thought to be mediated by a toxic RNA gain of function. Current attempts to develop therapy for this disease mainly aim at destroying or blocking abnormal properties of mutant DMPK (CUG)n RNA. Here, we explored a DNA-directed strategy and demonstrate that single clustered regularly interspaced short palindromic repeats (CRISPR)/Cas9-cleavage in either its 5' or 3' unique flank promotes uncontrollable deletion of large segments from the expanded trinucleotide repeat, rather than formation of short indels usually seen after double-strand break repair. Complete and precise excision of the repeat tract from normal and large expanded DMPK alleles in myoblasts from unaffected individuals, DM1 patients, and a DM1 mouse model could be achieved at high frequency by dual CRISPR/Cas9-cleavage at either side of the (CTG⋅CAG)n sequence. Importantly, removal of the repeat appeared to have no detrimental effects on the expression of genes in the DM1 locus. Moreover, myogenic capacity, nucleocytoplasmic distribution, and abnormal RNP-binding behavior of transcripts from the edited DMPK gene were normalized. Dual sgRNA-guided excision of the (CTG⋅CAG)n tract by CRISPR/Cas9 technology is applicable for developing isogenic cell lines for research and may provide new therapeutic opportunities for patients with DM1., (Copyright © 2017 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2017

31. NAMPT-mediated salvage synthesis of NAD+ controls morphofunctional changes of macrophages.

Author

Venter G, Oerlemans FT, Willemse M, Wijers M, Fransen JA, and Wieringa B

Subjects

Blotting, Western, Cell Line, Cytokines antagonists & inhibitors, DNA Primers genetics, Fluorescence, Humans, Macrophages physiology, Microscopy, Electron, Scanning, Nicotinamide Phosphoribosyltransferase antagonists & inhibitors, Oxidation-Reduction, Oxygen Consumption physiology, Phagocytosis drug effects, Transfection, Acrylamides pharmacology, Actin Cytoskeleton physiology, Adenosine Triphosphate metabolism, Cytokines metabolism, Macrophages cytology, NAD metabolism, Nicotinamide Phosphoribosyltransferase metabolism, Piperidines pharmacology

Abstract

Functional morphodynamic behavior of differentiated macrophages is strongly controlled by actin cytoskeleton rearrangements, a process in which also metabolic cofactors ATP and NAD(H) (i.e. NAD+ and NADH) and NADP(H) (i.e. NADP+ and NADPH) play an essential role. Whereas the link to intracellular ATP availability has been studied extensively, much less is known about the relationship between actin cytoskeleton dynamics and intracellular redox state and NAD+-supply. Here, we focus on the role of nicotinamide phosphoribosyltransferase (NAMPT), found in extracellular form as a cytokine and growth factor, and in intracellular form as one of the key enzymes for the production of NAD+ in macrophages. Inhibition of NAD+ salvage synthesis by the NAMPT-specific drug FK866 caused a decrease in cytosolic NAD+ levels in RAW 264.7 and Maf-DKO macrophages and led to significant downregulation of the glycolytic flux without directly affecting cell viability, proliferation, ATP production capacity or mitochondrial respiratory activity. Concomitant with these differential metabolic changes, the capacity for phagocytic ingestion of particles and also substrate adhesion of macrophages were altered. Depletion of cytoplasmic NAD+ induced cell-morphological changes and impaired early adhesion in phagocytosis of zymosan particles as well as spreading performance. Restoration of NAD+ levels by NAD+, NMN, or NADP+ supplementation reversed the inhibitory effects of FK866. We conclude that direct coupling to local, actin-based, cytoskeletal dynamics is an important aspect of NAD+'s cytosolic role in the regulation of morphofunctional characteristics of macrophages.

Published

2014

32. Increased OXPHOS activity precedes rise in glycolytic rate in H-RasV12/E1A transformed fibroblasts that develop a Warburg phenotype.

Author

de Groof AJ, te Lindert MM, van Dommelen MM, Wu M, Willemse M, Smift AL, Winer M, Oerlemans F, Pluk H, Fransen JA, and Wieringa B

Subjects

Adenovirus E1A Proteins genetics, Adenovirus E1A Proteins physiology, Animals, Cell Line, Transformed, Cell Proliferation, Cells, Cultured, Fibroblasts cytology, Fibroblasts ultrastructure, Lactic Acid metabolism, Male, Metabolome, Mice, Mice, Inbred BALB C, Mice, Nude, Microscopy, Electron, Scanning, Mitochondria metabolism, NAD metabolism, Neoplasm Transplantation, Neoplasms, Experimental metabolism, Neoplasms, Experimental pathology, Oxygen Consumption, Retroviridae genetics, Superoxides metabolism, ras Proteins genetics, ras Proteins physiology, Cell Transformation, Neoplastic, Fibroblasts metabolism, Glycolysis, Oxidative Phosphorylation

Abstract

Background: The Warburg phenotype in cancer cells has been long recognized, but there is still limited insight in the consecutive metabolic alterations that characterize its establishment. We obtained better understanding of the coupling between metabolism and malignant transformation by studying mouse embryonic fibroblast-derived cells with loss-of-senescence or H-RasV12/E1A-transformed phenotypes at different stages of oncogenic progression., Results: Spontaneous immortalization or induction of senescence-bypass had only marginal effects on metabolic profiles and viability. In contrast, H-RasV12/E1A transformation initially caused a steep increase in oxygen consumption and superoxide production, accompanied by massive cell death. During prolonged culture in vitro, cell growth rate increased gradually, along with tumor forming potential in in vitro anchorage-independent growth assays and in vivo tumor formation assays in immuno-deficient mice. Notably, glucose-to-lactic acid flux increased with passage number, while cellular oxygen consumption decreased. This conversion in metabolic properties was associated with a change in mitochondrial NAD+/NADH redox, indicative of decreased mitochondrial tricarboxic acid cycle and OXPHOS activity., Conclusion: The high rate of oxidative metabolism in newly transformed cells is in marked contrast with the high glycolytic rate in cells in the later tumor stage. In our experimental system, with cells growing under ambient oxygen conditions in nutrient-rich media, the shift towards this Warburg phenotype occurred as a step-wise adaptation process associated with augmented tumorigenic capacity and improved survival characteristics of the transformed cells. We hypothesize that early-transformed cells, which potentially serve as founders for new tumor masses may escape therapies aimed at metabolic inhibition of tumors with a fully developed Warburg phenotype.

Published

2009

33. The synovial-sarcoma-associated SS18-SSX2 fusion protein induces epigenetic gene (de)regulation.

Author

de Bruijn DR, Allander SV, van Dijk AH, Willemse MP, Thijssen J, van Groningen JJ, Meltzer PS, and van Kessel AG

Subjects

Cholesterol metabolism, DNA Methylation, Gene Expression Profiling, Histones metabolism, Humans, Insulin-Like Growth Factor II genetics, Neoplasm Proteins biosynthesis, Oligonucleotide Array Sequence Analysis, Oncogene Proteins, Fusion chemistry, Protein Structure, Tertiary, Repressor Proteins genetics, Repressor Proteins physiology, Sarcoma, Synovial metabolism, Somatomedins physiology, Transcriptional Activation genetics, Epigenesis, Genetic physiology, Gene Expression Regulation, Neoplastic physiology, Neoplasm Proteins genetics, Oncogene Proteins, Fusion physiology, Sarcoma, Synovial genetics, Transcription, Genetic genetics

Abstract

Fusion of the SS18 and either one of the SSX genes is a hallmark of human synovial sarcoma. The SS18 and SSX genes encode nuclear proteins that exhibit opposite transcriptional activities. The SS18 protein functions as a transcriptional coactivator and is associated with the SWI/SNF complex, whereas the SSX proteins function as transcriptional corepressors and are associated with the polycomb complex. The domains involved in these opposite transcriptional activities are retained in the SS18-SSX fusion proteins. Here, we set out to determine the direct transcriptional consequences of conditional SS18-SSX2 fusion protein expression using complementary DNA microarray-based profiling. By doing so, we identified several clusters of SS18-SSX2-responsive genes, including a group of genes involved in cholesterol synthesis, which is a general characteristic of malignancy. In addition, we identified a group of SS18-SSX2-responsive genes known to be specifically deregulated in primary synovial sarcomas, including IGF2 and CD44. Furthermore, we observed an uncoupling of EGR1, JUNB, and WNT signaling in response to SS18-SSX2 expression, suggesting that the SWI/SNF-associated coactivation functions of the SS18 moiety are impaired. Finally, we found that SS18-SSX2 expression affects histone modifications in the CD44 and IGF2 promoters and DNA methylation levels in the IGF2 imprinting control region. Together, we conclude that the SS18-SSX2 fusion protein may act as a so-called transcriptional "activator-repressor," which induces downstream target gene deregulation through epigenetic mechanisms. Our results may have implications for both the development and clinical management of synovial sarcomas.

Published

2006

34. Detection of 2-O-sulfated iduronate and N-acetylglucosamine units in heparan sulfate by an antibody selected against acharan sulfate (IdoA2S-GlcNAc)n.

Author

ten Dam GB, van de Westerlo EM, Smetsers TF, Willemse M, van Muijen GN, Merry CL, Gallagher JT, Kim YS, and van Kuppevelt TH

Subjects

Animals, Antibodies chemistry, CHO Cells, Cricetinae, Disaccharides chemistry, Electrophoresis, Agar Gel, Enzyme-Linked Immunosorbent Assay, Epitopes chemistry, Humans, Immunohistochemistry, Kidney metabolism, Male, Melanoma metabolism, Oligosaccharides chemistry, Precipitin Tests, Rats, Rats, Wistar, Sensitivity and Specificity, Snails, Acetylglucosamine chemistry, Glycosaminoglycans chemistry, Heparitin Sulfate chemistry, Iduronic Acid chemistry

Abstract

The snail glycosaminoglycan acharan sulfate (AS) is structurally related to heparan sulfates (HS) and has a repeating disaccharide structure of alpha-d-N-acetylglucosaminyl-2-O-sulfo-alpha-l-iduronic acid (GlcNAc-IdoA2S) residues. Using the phage display technology, a unique antibody (MW3G3) was selected against AS with a V(H)3, DP 47, and a CDR3 amino acid sequence of QKKRPRF. Antibody MW3G3 did not react with desulfated, N-deacetylated or N-sulfated AS, indicating that reactivity depends on N-acetyl and 2-O-sulfate groups. Antibody MW3G3 also had a high preference for (modified) heparin oligosaccharides containing N-acetylated glucosamine and 2-O-sulfated iduronic acid residues. In tissues, antibody MW3G3 identified a HS oligosaccharide epitope containing N-acetylated glucosamine and 2-O-sulfated iduronic acid residues as enzymatic N-deacetylation of HS in situ prevented staining, and 2-O-sulfotransferase-deficient Chinese hamster ovary cells were not reactive. An immunohistochemical survey using various rat organs revealed a distinct distribution of the MW3G3 epitope, which was primarily present in the basal laminae of most (but not all) blood vessels and of some epithelia, including human skin. No staining was observed in the glycosaminoglycan-rich tumor matrix of metastatic melanoma. In conclusion, we have selected an antibody that identifies HS oligosaccharides containing N-acetylated glucosamine and 2-O-sulfated iduronic acid residues. This antibody may be instrumental in identifying structural alterations in HS in health and disease.

Published

2004