Your search keyword '"Danielle de Jong"' showing total 75 results

1. Rapid test for Mycobacterium leprae infection: a practical tool for leprosy

Author

Louise Pierneef, Anouk van Hooij, Danielle de Jong, Gaby Wassenaar, Els Verhard, Elisa Tjon Kon Fat, Nadine Engel, Marufa Khatun, Santosh Soren, Abu Sufian Chowdhury, Colette van Hees, Paul Corstjens, and Annemieke Geluk

Subjects

Mycobacterium leprae, Diagnosis, Lateral flow, Leprosy, IgM, Quantitative UCP-based rapid test, Infectious and parasitic diseases, RC109-216, Public aspects of medicine, RA1-1270

Abstract

Abstract Background Detection of infection with Mycobacterium leprae allows timely prophylactic treatment, thereby reducing transmission as well as the risk of permanent, leprosy-associated nerve damage. However, since there is no worldwide-implemented standard test for M. leprae infection, detection of infection in asymptomatic individuals remains a major challenge for control programs in endemic areas. In previous studies, we developed and field-tested a lateral flow assay (LFA) quantitatively detecting human IgM against M. leprae-specific phenolic glycolipid I (anti-PGL-I), a marker for both active and past infection. This rapid test utilizes luminescent, background-free, up-converting reporter particles (UCP) and immunochromatography (i.e. the UCP-LF test platform) for accurate quantitation of anti-PGL-I IgM without operator bias. The aim of this study was to evaluate the final version of this quantitative UCP-based rapid test (i.e. PGL-I QURapid), using serum and fingerstick blood (FSB). Methods The test comprises a lateral flow strip, in a standard plastic or biodegradable cassette. It can be provided with a humanized, recombinant control to monitor test performance and calculate accurate anti-PGL-I IgM levels. The performance of this QUR-test was assessed using serum and FSB from patients with leprosy (n = 214), tuberculosis (n = 20), buruli ulcer (n = 19), leishmaniasis (n = 14), non-tuberculous mycobacterial (n = 35) infections, as well as healthy Dutch individuals (n = 710) and humanized, recombinant anti-PGL-I IgM antibodies. Plot receiver operating characteristic curves were created and sensitivity (Sn), specificity (Sp) and the area under the curve were calculated to evaluate test performance. Results Test results classified multibacillary leprosy patients with 95.0% Sn and 100% Sp using serum and 91.5% Sn and 99.8% Sp using FSB. Qualitative test results could be read after 2 min flow time, with accurate quantitation from 10 min onwards. The new anti-PGL-I IgM control supports production of batches with predetermined seropositivity thresholds and monitoring of the PGL-I QUR-test in various settings. Conclusion The operational version of the PGL-I QURapid with point-of-care applicability, meets the WHO target product profile criteria. Thus, this QUR-test is ready for public health implementations. Graphical Abstract

Published

2024

2. Field-friendly anti-PGL-I serosurvey in children to monitor Mycobacterium leprae transmission in Bihar, India

Author

Louise Pierneef, Paritosh Malaviya, Anouk van Hooij, Shyam Sundar, Abhishek Kumar Singh, Rajiv Kumar, Danielle de Jong, Maaike Meuldijk, Awnish Kumar, Zijie Zhou, Kristien Cloots, Paul Corstjens, Epco Hasker, and Annemieke Geluk

Subjects

children, leprosy, anti-M. leprae PGL-I antibodies, infection, diagnostics, serosurvey, Medicine (General), R5-920

Abstract

BackgroundIt has been amply described that levels of IgM antibodies against Mycobacterium leprae (M. leprae) phenolic glycolipid I (PGL-I) correlate strongly with the bacterial load in an infected individual. These findings have generated the concept of using seropositivity for antibodies against M. leprae PGL-I as an indicator of the proportion of the population that has been infected. Although anti-PGL-I IgM levels provide information on whether an individual has ever been infected, their presence cannot discriminate between recent and past infections. Since infection in (young) children by definition indicates recent transmission, we piloted the feasibility of assessment of anti-PGL-I IgM seroprevalence among children in a leprosy endemic area in India as a proxy for recent M. leprae transmission.Material and methodsA serosurvey for anti-PGL-I IgM antibodies among children in highly leprosy endemic villages in Bihar, India, was performed, applying the quantitative anti-PGL-I UCP-LFA cassette combined with low-invasive, small-volume fingerstick blood (FSB).ResultsLocal staff obtained FSB of 1,857 children (age 3–11 years) living in 12 leprosy endemic villages in Bihar; of these, 215 children (11.58%) were seropositive for anti-PGL-I IgM.ConclusionThe anti-PGL-I seroprevalence level of 11.58% among children corresponds with the seroprevalence levels described in studies in other leprosy endemic areas over the past decades where no prophylactic interventions have taken place. The anti-PGL-I UCP-LFA was found to be a low-complexity tool that could be practically combined with serosurveys and was well-accepted by both healthcare staff and the population. On route to leprosy elimination, quantitative anti-PGL-I serology in young children holds promise as a strategy to monitor recent M. leprae transmission in an area.

Published

2023

3. Development of lateral flow assays to detect host proteins in cattle for improved diagnosis of bovine tuberculosis

Author

Hamza Khalid, Louise Pierneef, Anouk van Hooij, Zijie Zhou, Danielle de Jong, Elisa Tjon Kon Fat, Timothy K. Connelley, Jayne C. Hope, Paul L. A. M. Corstjens, and Annemieke Geluk

Subjects

biomarkers, bovine tuberculosis, chemokines, cytokines, diagnostics, DIVA, Veterinary medicine, SF600-1100

Abstract

Bovine tuberculosis (bTB), caused by Mycobacterium bovis (M. bovis) infection in cattle, is an economically devastating chronic disease for livestock worldwide. Efficient disease control measures rely on early and accurate diagnosis using the tuberculin skin test (TST) and interferon-gamma release assays (IGRAs), followed by culling of positive animals. Compromised performance of TST and IGRA, due to BCG vaccination or co-infections with non-tuberculous mycobacteria (NTM), urges improved diagnostics. Lateral flow assays (LFAs) utilizing luminescent upconverting reporter particles (UCP) for quantitative measurement of host biomarkers present an accurate but less equipment- and labor-demanding diagnostic test platform. UCP-LFAs have proven applications for human infectious diseases. Here, we report the development of UCP-LFAs for the detection of six bovine proteins (IFN-γ, IL-2, IL-6, CCL4, CXCL9, and CXCL10), which have been described by ELISA as potential biomarkers to discriminate M. bovis infected from naïve and BCG-vaccinated cattle. We show that, in line with the ELISA data, the combined PPDb-induced levels of IFN-γ, IL-2, IL-6, CCL4, and CXCL9 determined by UCP-LFAs can discriminate M. bovis challenged animals from naïve (AUC range: 0.87–1.00) and BCG-vaccinated animals (AUC range: 0.97–1.00) in this cohort. These initial findings can be used to develop a robust and user-friendly multi-biomarker test (MBT) for bTB diagnosis.

Published

2023

4. Host biomarker-based quantitative rapid tests for detection and treatment monitoring of tuberculosis and COVID-19

Author

Louise Pierneef, Anouk van Hooij, Danielle de Jong, Elisa M. Tjon Kon Fat, Krista E. van Meijgaarden, Elisa Petruccioli, Valentina Vanini, Anna H.E. Roukens, Delia Goletti, Paul L.A.M. Corstjens, Simone A. Joosten, Annemieke Geluk, M.S. Arbous, B.M. van den Berg, S. Cannegieter, C.M. Cobbaert, A. van der Does, J.J.M. van Dongen, J. Eikenboom, M.C.M. Feltkamp, A. Geluk, J.J. Goeman, M. Giera, T. Hankemeier, M.H.M. Heemskerk, P.S. Hiemstra, C.H. Hokke, J.J. Janse, S.P. Jochems, S.A. Joosten, M. Kikkert, L. Lamont, J. Manniën, T.H.M. Ottenhoff, M.R. del Prado, N. Queralt Rosinach, M. Roestenberg, M. Roos, A.H.E. Roukens, H.H. Smits, E.J. Snijder, F.J.T. Staal, L.A. Trouw, R. Tsonaka, A. Verhoeven, L.G. Visser, J.J.C. de Vries, D.J. van Westerloo, J. Wigbers, H.J. van der Wijk, R.C. van Wissen, M. Wuhrer, M. Yazdanbakhsh, and M. Zlei

Subjects

Virology, Bacteriology, Science

Abstract

Summary: Diagnostic services for tuberculosis (TB) are not sufficiently accessible in low-resource settings, where most cases occur, which was aggravated by the COVID-19 pandemic. Early diagnosis of pulmonary TB can reduce transmission. Current TB-diagnostics rely on detection of Mycobacterium tuberculosis (Mtb) in sputum requiring costly, time-consuming methods, and trained staff. In this study, quantitative lateral flow (LF) assays were used to measure levels of seven host proteins in sera from pre-COVID-19 TB patients diagnosed in Europe and latently Mtb-infected individuals (LTBI), and from COVID-19 patients and healthy controls. Analysis of host proteins showed significantly lower levels in LTBI versus TB (AUC:0 · 94) and discriminated healthy individuals from COVID-19 patients (0 · 99) and severe COVID-19 from TB. Importantly, these host proteins allowed treatment monitoring of both respiratory diseases. This study demonstrates the potential of non-sputum LF assays as adjunct diagnostics and treatment monitoring for COVID-19 and TB based on quantitative detection of multiple host biomarkers.

Published

2023

5. GNL3 is an evolutionarily conserved stem cell gene influencing cell proliferation, animal growth and regeneration in the hydrozoan Hydractinia

Author

Gonzalo Quiroga-Artigas, Danielle de Jong, and Christine E. Schnitzler

Subjects

cnidarian, stem cell, nucleostemin, GNL3, GNL3L, CRISPR/Cas9, Biology (General), QH301-705.5

Abstract

Nucleostemin (NS) is a vertebrate gene preferentially expressed in stem and cancer cells, which acts to regulate cell cycle progression, genome stability and ribosome biogenesis. NS and its paralogous gene, GNL3-like (GNL3L), arose in the vertebrate clade after a duplication event from their orthologous gene, G protein Nucleolar 3 (GNL3). Research on invertebrate GNL3, however, has been limited. To gain a greater understanding of the evolution and functions of the GNL3 gene, we have performed studies in the hydrozoan cnidarian Hydractinia symbiolongicarpus, a colonial hydroid that continuously generates pluripotent stem cells throughout its life cycle and presents impressive regenerative abilities. We show that Hydractinia GNL3 is expressed in stem and germline cells. The knockdown of GNL3 reduces the number of mitotic and S-phase cells in Hydractinia larvae of different ages. Genome editing of Hydractinia GNL3 via CRISPR/Cas9 resulted in colonies with reduced growth rates, polyps with impaired regeneration capabilities, gonadal morphological defects, and low sperm motility. Collectively, our study shows that GNL3 is an evolutionarily conserved stem cell and germline gene involved in cell proliferation, animal growth, regeneration and sexual reproduction in Hydractinia, and sheds new light into the evolution of GNL3 and of stem cell systems.

Published

2022

6. Higher cMET dependence of sacral compared to clival chordoma cells: contributing to a better understanding of cMET in chordoma

Author

Birgit Lohberger, Susanne Scheipl, Ellen Heitzer, Franz Quehenberger, Danielle de Jong, Karoly Szuhai, Bernadette Liegl-Atzwanger, and Beate Rinner

Subjects

Medicine, Science

Abstract

Abstract Chordomas are rare slow growing, malignant bone tumors of the axial skeleton with no approved medical treatment. As the majority of chordomas express cMET and its ligand, HGF, and crosstalks between EGFR and MET-signaling exist, we aimed to explore cMET activity in chordoma cell lines and clinical samples. We investigated nine chordoma patients and four chordoma cell lines for cMET expression. Two clival and two sacral chordoma cell lines were tested for chromosomal abnormalities of the MET gene locus; we studied the influence of HGF on the autocrine secretion and migration behavior, as well as protein expression and phosphorylation. Two MET/ALK inhibitors were investigated for their effects on cell viability, cell cycle, cyclin alterations, apoptosis, and downstream signaling pathways. Moderate and strong expression of membrane and cytoplasmic cMET in chordoma patients and cell lines used, as well as concentration-dependent increase in phospho cMET expression after HGF stimulation in all four chordoma cell lines was shown. U-CH2, MUG-Chor1, and UM-Chor1 are polysomic for MET. Chordoma cell lines secreted EGF, VEGF, IL-6, and MMP9 upon HGF-stimulation. Sacral cell lines showed a distinct HGF-induced migration. Both inhibitors dose-dependently inhibited cell growth, induce apoptosis and cell-cycle arrest, and suppress downstream pathways. Heterogeneous responses obtained in our in vitro setting indicate that cMET inhibitors alone or in combination with other drugs might particularly benefit patients with sacral chordomas.

Published

2021

7. Detection and Monitoring of Mycobacterium leprae Infection in Nine Banded Armadillos (Dasypus novemcinctus) Using a Quantitative Rapid Test

Author

Zijie Zhou, Maria Pena, Anouk van Hooij, Louise Pierneef, Danielle de Jong, Roena Stevenson, Rachel Walley, Paul L. A. M. Corstjens, Richard Truman, Linda Adams, and Annemieke Geluk

Subjects

antibodies, armadillo, diagnosis, lateral flow assay, leprosy, M. leprae, Microbiology, QR1-502

Abstract

Leprosy is an infectious disease caused by Mycobacterium leprae with tropism for skin and peripheral nerves. Incessant transmission in endemic areas is still impeding elimination of leprosy. Although detection of M. leprae infection remains a challenge in asymptomatic individuals, the presence of antibodies specific for phenolglycolipid-I (PGL-I) correlate with bacterial load. Therefore, serosurveillance utilizing field-friendly tests detecting anti-PGL-I antibodies, can be applied to identify those who may transmit bacteria and to study (reduction of) M. leprae transmission. However, serology based on antibody detection cannot discriminate between past and present M. leprae infection in humans, nor can it detect individuals carrying low bacillary loads. In humans, anti-PGL-I IgM levels are long-lasting and usually detected in more individuals than anti-PGL-I IgG levels. Inherent to the characteristically long incubation time of leprosy, IgM/IgG relations (antibody kinetics) in leprosy patients and infected individuals are not completely clear. To investigate the antibody response directly after infection, we have measured antibody levels by ELISA, in longitudinal samples of experimentally M. leprae infected, susceptible nine-banded armadillos (Dasypus novemcinctus). In addition, we assessed the user- and field-friendly, low-cost lateral flow assay (LFA) utilizing upconverting reporter particles (UCP), developed for quantitative detection of human anti-PGL-I IgM (UCP-LFA), to detect treatment- or vaccination-induced changes in viable bacterial load. Our results show that serum levels of anti-PGL-I IgM, and to a lesser extent IgG, significantly increase soon after experimental M. leprae infection in armadillos. In view of leprosy phenotypes in armadillos, this animal model can provide useful insight into antibody kinetics in early infection in the various spectral forms of human leprosy. The UCP-LFA for quantitative detection of anti-PGL-I IgM allows monitoring the efficacy of vaccination and rifampin-treatment in the armadillo leprosy model, thereby providing a convenient tool to evaluate the effects of drugs and vaccines and new diagnostics.

Published

2021

8. Prototype multi-biomarker test for point-of-care leprosy diagnostics

Author

Anouk van Hooij, Elisa M. Tjon Kon Fat, Danielle de Jong, Marufa Khatun, Santosh Soren, Abu Sufian Chowdhury, Johan Chandra Roy, Khorshed Alam, Jong-Pill Kim, Jan Hendrik Richardus, Annemieke Geluk, and Paul L.A.M. Corstjens

Subjects

Diagnostic Technique in Health Technology, Applied Microbiology, Biotechnology, Science

Abstract

Summary: To end the decade-long, obstinately stagnant number of new leprosy cases, there is an urgent need for field-applicable diagnostic tools that detect infection with Mycobacterium leprae, leprosy's etiologic agent. Since immunity against M. leprae is characterized by humoral and cellular markers, we developed a lateral flow test measuring multiple host proteins based on six previously identified biomarkers for various leprosy phenotypes. This multi-biomarker test (MBT) demonstrated feasibility of quantitative detection of six host serum proteins simultaneously, jointly allowing discrimination of patients with multibacillary and paucibacillary leprosy from control individuals in high and low leprosy endemic areas. Pilot testing of fingerstick blood showed similar MBT performance in point-of-care (POC) settings as observed for plasma and serum. Thus, this newly developed prototype MBT measures six biomarkers covering immunity against M. leprae across the leprosy spectrum. The MBT thereby provides the basis for immunodiagnostic POC tests for leprosy with potential for other (infectious) diseases as well.

Published

2021

9. Household Contacts of Leprosy Patients in Endemic Areas Display a Specific Innate Immunity Profile

Author

Anouk van Hooij, Maria Tió-Coma, Els M. Verhard, Marufa Khatun, Khorshed Alam, Elisa Tjon Kon Fat, Danielle de Jong, Abu Sufian Chowdhury, Paul Corstjens, Jan Hendrik Richardus, and Annemieke Geluk

Subjects

innate immunity, lateral flow test, diagnostics, M. leprae, UCP-LFA, leprosy, Immunologic diseases. Allergy, RC581-607

Abstract

Leprosy is a chronic infectious disease, caused by Mycobacterium leprae, that can lead to severe life-long disabilities. The transmission of M. leprae is continuously ongoing as witnessed by the stable new case detection rate. The majority of exposed individuals does, however, not develop leprosy and is protected from infection by innate immune mechanisms. In this study the relation between innate immune markers and M. leprae infection as well as the occurrence of leprosy was studied in household contacts (HCs) of leprosy patients with high bacillary loads. Serum proteins associated with innate immunity (ApoA1, CCL4, CRP, IL-1Ra, IL-6, IP-10, and S100A12) were determined by lateral flow assays (LFAs) in conjunction with the presence of M. leprae DNA in nasal swabs (NS) and/or slit-skin smears (SSS). The HCs displayed ApoA1 and S100A12 levels similar to paucibacillary patients and could be differentiated from endemic controls based on the levels of these markers. In the 31 households included the number (percentage) of HCs that were concomitantly diagnosed with leprosy, or tested positive for M. leprae DNA in NS and SSS, was not equally divided. Specifically, households where M. leprae infection and leprosy disease was not observed amongst members of the household were characterized by higher S100A12 and lower CCL4 levels in whole blood assays of HCs in response to M. leprae. Lateral flow assays provide a convenient diagnostic tool to quantitatively measure markers of the innate immune response and thereby detect individuals which are likely infected with M. leprae and at risk of developing disease or transmitting bacteria. Low complexity diagnostic tests measuring innate immunity markers can therefore be applied to help identify who should be targeted for prophylactic treatment.

Published

2020

10. p120-catenin prevents multinucleation through control of MKLP1-dependent RhoA activity during cytokinesis

Author

Robert A.H. van de Ven, Jolien S. de Groot, Danielle Park, Robert van Domselaar, Danielle de Jong, Karoly Szuhai, Elsken van der Wall, Oscar M. Rueda, H. Raza Ali, Carlos Caldas, Paul J. van Diest, Martin W. Hetzer, Erik Sahai, and Patrick W.B. Derksen

Subjects

Science

Abstract

The tumour suppressor p120-catenin (p120) controls cadherin-based adhesion. Here, the authors demonstrate that p120 regulates cytokinesis through binding to the centralspindlin component MKLP1 and controls RhoA activity. Loss of p120 in cancer induces multinucleation and chromosomal instability, independent of cell-cell adhesion.

Published

2016

11. Human Extravillous Trophoblasts Penetrate Decidual Veins and Lymphatics before Remodeling Spiral Arteries during Early Pregnancy.

Author

Nannan He, Liesbeth van Iperen, Danielle de Jong, Karoly Szuhai, Frans M Helmerhorst, Lucette A J van der Westerlaken, and Susana M Chuva de Sousa Lopes

Subjects

Medicine, Science

Abstract

In humans, the defective invasion of the maternal endometrium by fetal extravillous trophoblasts (EVTs) can lead to insufficient perfusion of the placenta, resulting in pregnancy complications that can put both mother and baby at risk. To study the invasion of maternal endometrium between (W)5.5-12 weeks of gestation by EVTs, we combined fluorescence in situ hybridization, immunofluorescence and immunohistochemistry to determine the presence of (male) EVTs in the vasculature of the maternal decidua. We observed that interstitial mononuclear EVTs directly entered decidual veins and lymphatics from W5.5. This invasion of decidual veins and lymphatics occurred long before endovascular EVTs remodelled decidual spiral arteries. This unexpected early entrance of interstitial mononuclear EVTs in the maternal circulation does not seem to contribute to the materno-placental vascular connection directly, but rather to establish (and expand) the materno-fetal interface through an alternative vascular route.

Published

2017

12. NKX2-5 mutations causative for congenital heart disease retain functionality and are directed to hundreds of targets

Author

Romaric Bouveret, Ashley J Waardenberg, Nicole Schonrock, Mirana Ramialison, Tram Doan, Danielle de Jong, Antoine Bondue, Gurpreet Kaur, Stephanie Mohamed, Hananeh Fonoudi, Chiann-mun Chen, Merridee A Wouters, Shoumo Bhattacharya, Nicolas Plachta, Sally L Dunwoodie, Gavin Chapman, Cédric Blanpain, and Richard P Harvey

Subjects

cardiogenesis, transcription factor, genetic disease, Medicine, Science, Biology (General), QH301-705.5

Abstract

We take a functional genomics approach to congenital heart disease mechanism. We used DamID to establish a robust set of target genes for NKX2-5 wild type and disease associated NKX2-5 mutations to model loss-of-function in gene regulatory networks. NKX2-5 mutants, including those with a crippled homeodomain, bound hundreds of targets including NKX2-5 wild type targets and a unique set of "off-targets", and retained partial functionality. NKXΔHD, which lacks the homeodomain completely, could heterodimerize with NKX2-5 wild type and its cofactors, including E26 transformation-specific (ETS) family members, through a tyrosine-rich homophilic interaction domain (YRD). Off-targets of NKX2-5 mutants, but not those of an NKX2-5 YRD mutant, showed overrepresentation of ETS binding sites and were occupied by ETS proteins, as determined by DamID. Analysis of kernel transcription factor and ETS targets show that ETS proteins are highly embedded within the cardiac gene regulatory network. Our study reveals binding and activities of NKX2-5 mutations on WT target and off-targets, guided by interactions with their normal cardiac and general cofactors, and suggest a novel type of gain-of-function in congenital heart disease.

Published

2015

13. Correction: Corrigendum: p120-catenin prevents multinucleation through control of MKLP1-dependent RhoA activity during cytokinesis

Author

Robert A. H. van de Ven, Jolien S. de Groot, Danielle Park, Robert van Domselaar, Danielle de Jong, Karoly Szuhai, Elsken van der Wall, Oscar M. Rueda, H. Raza Ali, Carlos Caldas, Paul J. van Diest, Martin W. Hetzer, Erik Sahai, and Patrick W. B. Derksen

Subjects

Science

Abstract

Nature Communications 7: Article number: 13874 (2016); Published 22 December 2016; Updated 6 September 2017 The financial support for this Article was not fully acknowledged. The Acknowledgements should have included the National Institutes of Health grants R01GM098749 and National Institutes of Health Transformative Research Award R01NS096786.

Published

2017

14. Dendritic morphology of hippocampal and amygdalar neurons in adolescent mice is resilient to genetic differences in stress reactivity.

Author

Anup G Pillai, Danielle de Jong, Sofia Kanatsou, Harm Krugers, Alana Knapman, Jan-Michael Heinzmann, Florian Holsboer, Rainer Landgraf, Marian Joëls, and Chadi Touma

Subjects

Medicine, Science

Abstract

Many studies have shown that chronic stress or corticosterone over-exposure in rodents leads to extensive dendritic remodeling, particularly of principal neurons in the CA3 hippocampal area and the basolateral amygdala. We here investigated to what extent genetic predisposition of mice to high versus low stress reactivity, achieved through selective breeding of CD-1 mice, is also associated with structural plasticity in Golgi-stained neurons. Earlier, it was shown that the highly stress reactive (HR) compared to the intermediate (IR) and low (LR) stress reactive mice line presents a phenotype, with respect to neuroendocrine parameters, sleep architecture, emotional behavior and cognition, that recapitulates some of the features observed in patients suffering from major depression. In late adolescent males of the HR, IR, and LR mouse lines, we observed no significant differences in total dendritic length, number of branch points and branch tips, summated tip order, number of primary dendrites or dendritic complexity of either CA3 pyramidal neurons (apical as well as basal dendrites) or principal neurons in the basolateral amygdala. Apical dendrites of CA1 pyramidal neurons were also unaffected by the differences in stress reactivity of the animals; marginally higher length and complexity of the basal dendrites were found in LR compared to IR but not HR mice. In the same CA1 pyramidal neurons, spine density of distal apical tertiary dendrites was significantly higher in LR compared to IR or HR animals. We tentatively conclude that the dendritic complexity of principal hippocampal and amygdala neurons is remarkably stable in the light of a genetic predisposition to high versus low stress reactivity, while spine density seems more plastic. The latter possibly contributes to the behavioral phenotype of LR versus HR animals.

Published

2012

15. MDMX regulates transcriptional activity of p53 and FOXO proteins to stimulate proliferation of melanoma cells

Author

Renier C. Heijkants, Amina F. A. S. Teunisse, Danielle de Jong, Kseniya Glinkina, Hailiang Mei, Szymon M. Kielbasa, Karoly Szuhai, and Aart G. Jochemsen

Subjects

p53, MDMX, FOXO, MDM2, RFX7, uveal melanoma, cutaneous melanoma, RNA-seq, Cancer Research, Oncology

Abstract

The tumor suppressor protein p53 has an important role in cell-fate determination. In cancer cells, the activity of p53 is frequently repressed by high levels of MDMX and/or MDM2. MDM2 is a ubiquitin ligase whose activity results in ubiquitin- and proteasome-dependent p53 degradation, while MDMX inhibits p53-activated transcription by shielding the p53 transactivation domain. Interestingly, the oncogenic functions of MDMX appear to be more wide-spread than inhibition of p53. The present study aimed to elucidate the MDMX-controlled transcriptome. Therefore, we depleted MDMX with four distinct shRNAs from a high MDMX expressing uveal melanoma cell line and determined the effect on the transcriptome by RNAseq. Biological function analyses indicate the inhibition of the cell cycle regulatory genes and stimulation of cell death activating genes upon MDMX depletion. Although the inhibition of p53 activity clearly contributes to the transcription regulation controlled by MDMX, it appeared that the transcriptional regulation of multiple genes did not only rely on p53 expression. Analysis of gene regulatory networks indicated a role for Forkhead box (FOX) transcription factors. Depletion of FOXO proteins partly prevented the transcriptional changes upon MDMX depletion. Furthermore, depletion of FOXO proteins relatively diminished the growth inhibition upon MDMX knockdown, although the knockdown of the FOXO transcription factors also reduces cell growth. In conclusion, the p53-independent oncogenic functions of MDMX could be partially explained by its regulation of FOXO activity.

Published

2022

16. Host biomarker-based quantitative rapid tests for detection and treatment monitoring of tuberculosis and COVID-19

Author

Louise Pierneef, Anouk van Hooij, Danielle de Jong, Elisa M. Tjon Kon Fat, Krista E. van Meijgaarden, Elisa Petruccioli, Valentina Vanini, Anna H.E. Roukens, Delia Goletti, Paul L.A.M. Corstjens, Simone A. Joosten, Annemieke Geluk, M.S. Arbous, B.M. van den Berg, S. Cannegieter, C.M. Cobbaert, A. van der Does, J.J.M. van Dongen, J. Eikenboom, M.C.M. Feltkamp, A. Geluk, J.J. Goeman, M. Giera, T. Hankemeier, M.H.M. Heemskerk, P.S. Hiemstra, C.H. Hokke, J.J. Janse, S.P. Jochems, S.A. Joosten, M. Kikkert, L. Lamont, J. Manniën, T.H.M. Ottenhoff, M.R. del Prado, N. Queralt Rosinach, M. Roestenberg, M. Roos, A.H.E. Roukens, H.H. Smits, E.J. Snijder, F.J.T. Staal, L.A. Trouw, R. Tsonaka, A. Verhoeven, L.G. Visser, J.J.C. de Vries, D.J. van Westerloo, J. Wigbers, H.J. van der Wijk, R.C. van Wissen, M. Wuhrer, M. Yazdanbakhsh, and M. Zlei

Subjects

Multidisciplinary

Abstract

Diagnostic services for tuberculosis (TB) are not sufficiently accessible in low-resource settings, where most cases occur, which was aggravated by the COVID-19 pandemic. Early diagnosis of pulmonary TB can reduce transmission. Current TB-diagnostics rely on detection of

Published

2022

17. Author response for 'GNL3 is an evolutionarily conserved stem cell gene influencing cell proliferation, animal growth and regeneration in the hydrozoan Hydractinia'

Author

null Gonzalo Quiroga-Artigas, null Danielle de Jong, and null Christine E. Schnitzler

Published

2022

18. P-Glycoprotein (ABCB1/MDR1) Controls Brain Penetration and Intestinal Disposition of the PARP1/2 Inhibitor Niraparib

Author

Nancy H.C. Loos, Hilde Rosing, Margarida L. F. Martins, Maria C. Lebre, Danielle de Jong, Alfred H. Schinkel, Jos H. Beijnen, Matthijs M. Tibben, and Sümeyra Mucuk

Subjects

Genetically modified mouse, Indazoles, Abcg2, CYP3A, Metabolite, Pharmaceutical Science, Pharmacology, Poly(ADP-ribose) Polymerase Inhibitors, Madin Darby Canine Kidney Cells, chemistry.chemical_compound, Mice, Dogs, Pharmacokinetics, Piperidines, Tetrahydroisoquinolines, Drug Discovery, Distribution (pharmacology), Animals, Cytochrome P-450 CYP3A, Tissue Distribution, ATP Binding Cassette Transporter, Subfamily B, Member 1, CYP3A4, biology, Chemistry, Brain, Biological Transport, In vitro, Intestines, biology.protein, Molecular Medicine, Acridines

Abstract

Niraparib (Zejula), a selective oral PARP1/2 inhibitor registered for ovarian, fallopian tube, and primary peritoneal cancer treatment, is under investigation for other malignancies, including brain tumors. We explored the impact of the ABCB1 and ABCG2 multidrug efflux transporters, the OATP1A/1B uptake transporters, and the CYP3A drug-metabolizing complex on oral niraparib pharmacokinetics, using wild-type and genetically modified mouse and cell line models. In vitro, human ABCB1 and mouse Abcg2 transported niraparib moderately. Compared to wild-type mice, niraparib brain-to-plasma ratios were 6- to 7-fold increased in Abcb1a/1b-/- and Abcb1a/1b;Abcg2-/- but not in single Abcg2-/- mice, while niraparib plasma exposure at later time points was ∼2-fold increased. Niraparib recovery in the small intestinal content was markedly reduced in the Abcb1a/1b-deficient strains. Pretreatment of wild-type mice with oral elacridar, an ABCB1/ABCG2 inhibitor, increased niraparib brain concentration and reduced small intestinal content recovery to levels observed in Abcb1a/1b;Abcg2-/- mice. Oatp1a/1b deletion did not significantly affect niraparib oral bioavailability or liver distribution but decreased metabolite M1 liver uptake. No significant effects of mouse Cyp3a ablation were observed, but overexpression of transgenic human CYP3A4 unexpectedly increased niraparib plasma exposure. Thus, Abcb1 deficiency markedly increased niraparib brain distribution and reduced its small intestinal content recovery, presumably through reduced biliary excretion and/or decreased direct intestinal excretion. Elacridar pretreatment inhibited both processes completely. Clinically, the negligible role of OATP1 and CYP3A could be advantageous for niraparib, diminishing drug-drug interaction or interindividual variation risks involving these proteins. These findings may support the further clinical development and application of niraparib.

Published

2021

19. Higher cMET dependence of sacral compared to clival chordoma cells

Author

Birgit Lohberger, Bernadette Liegl-Atzwanger, Ellen Heitzer, Danielle de Jong, Susanne Scheipl, Beate Rinner, Franz Quehenberger, and Karoly Szuhai

Subjects

musculoskeletal diseases, Sacrum, Cell biology, DNA Copy Number Variations, Cell Survival, Pyridines, Science, Apoptosis, Biology, Skull Base Neoplasms, Article, Medical research, Crizotinib, Cell Line, Tumor, Chordoma, medicine, Humans, Anaplastic Lymphoma Kinase, Anilides, Autocrine signalling, Protein Kinase Inhibitors, Cell Proliferation, Cancer, Multidisciplinary, Hepatocyte Growth Factor, Cell growth, Proto-Oncogene Proteins c-met, Cell cycle, medicine.disease, Gene Expression Regulation, Neoplastic, Cranial Fossa, Posterior, Cell culture, Cancer research, Medicine, Sacral Chordoma, Signal Transduction

Abstract

Chordomas are rare slow growing, malignant bone tumors of the axial skeleton with no approved medical treatment. As the majority of chordomas express cMET and its ligand, HGF, and crosstalks between EGFR and MET-signaling exist, we aimed to explore cMET activity in chordoma cell lines and clinical samples. We investigated nine chordoma patients and four chordoma cell lines for cMET expression. Two clival and two sacral chordoma cell lines were tested for chromosomal abnormalities of the MET gene locus; we studied the influence of HGF on the autocrine secretion and migration behavior, as well as protein expression and phosphorylation. Two MET/ALK inhibitors were investigated for their effects on cell viability, cell cycle, cyclin alterations, apoptosis, and downstream signaling pathways. Moderate and strong expression of membrane and cytoplasmic cMET in chordoma patients and cell lines used, as well as concentration-dependent increase in phospho cMET expression after HGF stimulation in all four chordoma cell lines was shown. U-CH2, MUG-Chor1, and UM-Chor1 are polysomic for MET. Chordoma cell lines secreted EGF, VEGF, IL-6, and MMP9 upon HGF-stimulation. Sacral cell lines showed a distinct HGF-induced migration. Both inhibitors dose-dependently inhibited cell growth, induce apoptosis and cell-cycle arrest, and suppress downstream pathways. Heterogeneous responses obtained in our in vitro setting indicate that cMET inhibitors alone or in combination with other drugs might particularly benefit patients with sacral chordomas.

Published

2021

20. Prototype multi-biomarker test for point-of-care leprosy diagnostics

Author

Abu Sufian Chowdhury, Khorshed Alam, Anouk van Hooij, Annemieke Geluk, Paul L. A. M. Corstjens, Elisa M. Tjon Kon Fat, Jong-Pill Kim, Marufa Khatun, Jan Hendrik Richardus, Danielle de Jong, Johan Chandra Roy, Santosh Soren, and Public Health

Subjects

0301 basic medicine, Fingerstick, Applied Microbiology, Paucibacillary Leprosy, 02 engineering and technology, Article, Lateral flow test, 03 medical and health sciences, SDG 3 - Good Health and Well-being, medicine, lcsh:Science, Mycobacterium leprae, Host protein, Point of care, Multidisciplinary, Diagnostic Technique in Health Technology, biology, business.industry, 021001 nanoscience & nanotechnology, medicine.disease, biology.organism_classification, 030104 developmental biology, Immunology, Biomarker (medicine), lcsh:Q, Leprosy, 0210 nano-technology, business, Biotechnology

Abstract

Summary To end the decade-long, obstinately stagnant number of new leprosy cases, there is an urgent need for field-applicable diagnostic tools that detect infection with Mycobacterium leprae, leprosy's etiologic agent. Since immunity against M. leprae is characterized by humoral and cellular markers, we developed a lateral flow test measuring multiple host proteins based on six previously identified biomarkers for various leprosy phenotypes. This multi-biomarker test (MBT) demonstrated feasibility of quantitative detection of six host serum proteins simultaneously, jointly allowing discrimination of patients with multibacillary and paucibacillary leprosy from control individuals in high and low leprosy endemic areas. Pilot testing of fingerstick blood showed similar MBT performance in point-of-care (POC) settings as observed for plasma and serum. Thus, this newly developed prototype MBT measures six biomarkers covering immunity against M. leprae across the leprosy spectrum. The MBT thereby provides the basis for immunodiagnostic POC tests for leprosy with potential for other (infectious) diseases as well., Graphical Abstract, Highlights • Prototype MBT that quantitatively detects six host-derived biomarkers is developed • The immunopathological spectrum of leprosy is ideally suited to evaluate the MBT • MBT discriminated patients with leprosy from controls in a high and non-endemic area • Application of the MBT using low invasive fingerstick blood is technically feasible, Diagnostic Technique in Health Technology; Applied Microbiology; Biotechnology

Published

2021

21. Vascular tumor recapitulated in endothelial cells from hiPSCs engineered to express the SERPINE1-FOSB translocation

Author

Daniela C.F. Salvatori, Xu Cao, Christine L. Mummery, Karoly Szuhai, Francijna E. van den Hil, Inge H. Briaire-de Bruijn, Hailiang Mei, Valeria V. Orlova, Danielle de Jong, Judith V.M.G. Bovée, and David G.P. van IJzendoorn

Subjects

PHE, pseudomyogenic hemangioendothelioma, Induced Pluripotent Stem Cells, endothelial cell differentiation, Soft Tissue Neoplasms, Chromosomal translocation, Biology, tumor model, Endothelial cell differentiation, Article, Translocation, Genetic, General Biochemistry, Genetics and Molecular Biology, chromosomal translocation, Fusion gene, Plasminogen Activator Inhibitor 1, Humans, t(7, 19)(q22, q13) SERPINE1-FOSB chromosomal translocation, Tube formation, hiPSCs, CRISPR/Cas9-mediated gene targeting, hiPSC-ECs, gene fusion, Endothelial Cells, Cell Differentiation, hiPSC-derived ECs, Vascular Neoplasms, Cell biology, human induced pluripotent stem cells, Transplantation, Endothelial stem cell, Cell culture, vascular tumor, Neoplasms, Vascular Tissue, Proto-Oncogene Proteins c-fos, FOSB

Abstract

Summary Chromosomal translocations are prevalent among soft tissue tumors, including those of the vasculature such as pseudomyogenic hemangioendothelioma (PHE). PHE shows endothelial cell (EC) features and has a tumor-specific t(7;19)(q22;q13) SERPINE1-FOSB translocation, but is difficult to study as no primary tumor cell lines have yet been derived. Here, we engineer the PHE chromosomal translocation into human induced pluripotent stem cells (hiPSCs) using CRISPR/Cas9 and differentiate these into ECs (hiPSC-ECs) to address this. Comparison of parental with PHE hiPSC-ECs shows (1) elevated expression of FOSB, (2) higher proliferation and more tube formation but lower endothelial barrier function, (3) invasive growth and abnormal vessel formation in mice after transplantation, and (4) specific transcriptome alterations reflecting PHE and indicating PI3K-Akt and MAPK signaling pathways as possible therapeutic targets. The modified hiPSC-ECs thus recapitulate functional features of PHE and demonstrate how these translocation models can be used to understand tumorigenic mechanisms and identify therapeutic targets., Graphical Abstract, Highlights SERPINE1-FOSB translocation in hiPSC to model the vascular tumor PHE CRISPR/Cas9-mediated gene targeting to engineer hiPSCSERPINE1-FOSB hiPSC-ECsSERPINE1-FOSB show increased FOSB expression Functional features of PHE recapitulated by hiPSC-ECsSERPINE1-FOSB, van IJzendoorn et al. introduce a t(7;19)(q22;q13) SERPINE1-FOSB chromosomal translocation into hiPSCs to model the vascular tumor pseudomyogenic hemangioendothelioma (PHE). hiPSC-endothelial cells carrying the translocation recapitulate functional features of PHE in vitro and in vivo. SERPINE1-FOSB translocated hiPSCs can thus be used to understand tumorigenic mechanisms and identify therapeutic targets.

Published

2020

22. Synthetic Phenolic Glycolipids for application in diagnostic tests for leprosy

Author

Paul L. A. M. Corstjens, Rosita Moretti, L Melanie Groot, J. Hessel M. van Dijk, Annemieke Geluk, Jolijn Geboers, Els Verhard-Seymonsbergen, Anouk van Hooij, Gijs A. van der Marel, Jeroen D. C. Codée, and Danielle de Jong

Subjects

Glycan, Glycoconjugate, diagnosis, Molecular Conformation, carbohydrates, 010402 general chemistry, 01 natural sciences, Biochemistry, Microbiology, Glycolipid, medicine, Humans, Molecular Biology, Pathogen, Mycobacterium leprae, chemistry.chemical_classification, Antigens, Bacterial, Full Paper, biology, Diagnostic Tests, Routine, 010405 organic chemistry, Organic Chemistry, lateral flow assay, Full Papers, medicine.disease, biology.organism_classification, glycoconjugates, 0104 chemical sciences, chemistry, Infectious disease (medical specialty), biology.protein, Molecular Medicine, Leprosy, Glycolipids, Antibody, leprosy

Abstract

Point‐of‐care (POC) diagnostic tests for the rapid detection of individuals infected with Mycobacterium leprae, the causative pathogen of leprosy, represent efficient tools to guide therapeutic and prophylactic treatment strategies in leprosy control programs, thus positively contributing to clinical outcome and reducing transmission of this infectious disease. Levels of antibodies directed against the M. leprae‐specific phenolic glycolipid I (PGL−I) closely correlate with an individual's bacterial load and a higher risk of developing leprosy. We describe herein the assembly of a set of PGL glycans carrying the characteristic phenol aglycon and featuring different methylation patterns. The PGL trisaccharides were applied to construct neoglycoproteins that were used to detect anti‐PGL IgM antibodies in leprosy patients. ELISAs and quantitative lateral‐flow assays based on up‐converting nanoparticles (UCP‐LFAs) showed that the generated PGL−I and PGL‐II trisaccharide neoglycoconjugates can be applied for the detection of anti M. leprae IgM antibodies in POC tests., Getting to the point of care: Trisaccharides of phenolic glycolipids (PGL) originating from M. leprae were evaluated for their diagnostic potential as neoglycoproteins in ELISA and an up‐converting particle lateral flow assay (UCP‐LFA). Two naturally occurring trisaccharides were found to be suitable for this purpose and can thus be used for future field studies in leprosy endemic areas.

Published

2020

23. Household Contacts of Leprosy Patients in Endemic Areas Display a Specific Innate Immunity Profile

Author

Annemieke Geluk, Abu Sufian Chowdhury, Khorshed Alam, Paul L. A. M. Corstjens, Marufa Khatun, Anouk van Hooij, Els M. Verhard, Elisa M. Tjon Kon Fat, Danielle de Jong, Jan Hendrik Richardus, Maria Tió-Coma, and Public Health

Subjects

0301 basic medicine, lcsh:Immunologic diseases. Allergy, Adult, Male, Adolescent, Endemic Diseases, Immunology, UCP-LFA, Disease, leprae, lateral flow test, Lateral flow test, 03 medical and health sciences, Young Adult, 0302 clinical medicine, Leprosy, medicine, diagnostics, Immunology and Allergy, Humans, Child, Mycobacterium leprae, innate immunity, Asymptomatic Infections, Original Research, Whole blood, M. leprae, Innate immune system, biology, Transmission (medicine), business.industry, Middle Aged, medicine.disease, biology.organism_classification, Blood proteins, Immunity, Innate, 030104 developmental biology, Female, business, lcsh:RC581-607, Biomarkers, 030215 immunology

Abstract

Leprosy is a chronic infectious disease, caused by Mycobacterium leprae, that can lead to severe life-long disabilities. The transmission of M. leprae is continuously ongoing as witnessed by the stable new case detection rate. The majority of exposed individuals does, however, not develop leprosy and is protected from infection by innate immune mechanisms. In this study the relation between innate immune markers and M. leprae infection as well as the occurrence of leprosy was studied in household contacts (HCs) of leprosy patients with high bacillary loads. Serum proteins associated with innate immunity (ApoA1, CCL4, CRP, IL-1Ra, IL-6, IP-10, and S100A12) were determined by lateral flow assays (LFAs) in conjunction with the presence of M. leprae DNA in nasal swabs (NS) and/or slit-skin smears (SSS). The HCs displayed ApoA1 and S100A12 levels similar to paucibacillary patients and could be differentiated from endemic controls based on the levels of these markers. In the 31 households included the number (percentage) of HCs that were concomitantly diagnosed with leprosy, or tested positive for M. leprae DNA in NS and SSS, was not equally divided. Specifically, households where M. leprae infection and leprosy disease was not observed amongst members of the household were characterized by higher S100A12 and lower CCL4 levels in whole blood assays of HCs in response to M. leprae. Lateral flow assays provide a convenient diagnostic tool to quantitatively measure markers of the innate immune response and thereby detect individuals which are likely infected with M. leprae and at risk of developing disease or transmitting bacteria. Low complexity diagnostic tests measuring innate immunity markers can therefore be applied to help identify who should be targeted for prophylactic treatment.

Published

2020

24. Coronaviruses and arteriviruses display striking differences in their cyclophilin A-dependence during replication in cell culture

Author

Karoly Szuhai, Philippe Gallay, Udayan Chatterji, Eric J. Snijder, Danielle de Jong, Adriaan H. de Wilde, Jessika C. Zevenhoven-Dobbe, Clara C. Posthuma, and Corrine Beugeling

Subjects

0301 basic medicine, Human coronavirus 229E, CypA, Virus Cultivation, Arterivirus, viruses, Knockout, Cypa, Biology, Virus Replication, Alphacoronavirus, Article, Cell Line, 03 medical and health sciences, Cyclophilin A, MERS-coronavirus, Virology, Cricetinae, Animals, Humans, CRISPR/Cas9, Cyclophilin, Host factor, virus diseases, biology.organism_classification, Coronavirus, 030104 developmental biology, EAV, Betacoronavirus, human coronavirus-229E

Abstract

Cyclophilin A (CypA) is an important host factor in the replication of a variety of RNA viruses. Also the replication of several nidoviruses was reported to depend on CypA, although possibly not to the same extent. These prior studies are difficult to compare, since different nidoviruses, cell lines and experimental set-ups were used. Here, we investigated the CypA dependence of three distantly related nidoviruses that can all replicate in Huh7 cells: the arterivirus equine arteritis virus (EAV), the alphacoronavirus human coronavirus 229E (HCoV-229E), and the betacoronavirus Middle East respiratory syndrome coronavirus (MERS-CoV). The replication of these viruses was compared in the same parental Huh7 cells and in CypA-knockout Huh7 cells generated using CRISPR/Cas9-technology. CypA depletion reduced EAV yields by ~ 3-log, whereas MERS-CoV progeny titers were modestly reduced (3-fold) and HCoV-229E replication was unchanged. This study reveals that the replication of nidoviruses can differ strikingly in its dependence on cellular CypA., Highlights • Nidoviruses display differences in sensitivity towards cyclophilin A depletion. • Replication of MERS-coronavirus is reduced modestly in cyclophilin A-knockout cells. • Equine arteritis virus replication is strongly inhibited by cyclophilin A depletion. • Chromosomal anomalies complicate CRISPR/Cas9-mediated gene editing in Huh7 cells.

Published

2017

25. Generation of Fibrodysplasia ossificans progressiva and control integration free iPSC lines from periodontal ligament fibroblasts

Author

Jan Coen Netelenbos, Elisabeth M.W. Eekhoff, T. J. de Vries, Christian Freund, Karoly Szuhai, Danielle de Jong, Gonzalo Sanchez-Duffhues, Harald Mikkers, Marie-José Goumans, P. ten Dijke, R. van Es, Nathalie Bravenboer, Internal medicine, ACS - Diabetes & metabolism, AGEM - Endocrinology, metabolism and nutrition, Amsterdam Movement Sciences - Rehabilitation & Development, Parodontologie (OII, ACTA), and Periodontology

Subjects

0301 basic medicine, Adult, Periodontal Ligament, Induced Pluripotent Stem Cells, Cell Culture Techniques, Bone morphogenetic protein, Cell Line, 03 medical and health sciences, Young Adult, 0302 clinical medicine, SDG 3 - Good Health and Well-being, medicine, Periodontal fiber, Humans, Fibroblast, Induced pluripotent stem cell, lcsh:QH301-705.5, biology, Base Sequence, Point mutation, Reproducibility of Results, General Medicine, Cell Biology, Fibroblasts, biology.organism_classification, medicine.disease, Sendai virus, 030104 developmental biology, medicine.anatomical_structure, lcsh:Biology (General), Fibrodysplasia ossificans progressiva, Cancer research, Heterotopic ossification, Female, 030217 neurology & neurosurgery, Developmental Biology

Abstract

Fibrodysplasia ossificans progressiva (FOP) is a very rare devastating heterotopic ossification disorder, classically caused by a heterozygous single point mutation (c.617G>A) in the ACVR1gene, encoding the Bone morphogenetic protein (BMP) type I receptor, also termed activin receptor-like kinase (ALK)2. FOP patients develop heterotopic ossification episodically in response to inflammatory insults, thereby compromising tissue sampling and the development of in vitro surrogate models for FOP. Here we describe the generation and characterization of a control and a classical FOP induced pluripotent stem cell (iPSC) line derived from periodontal ligament fibroblast cells using Sendai virus vectors.

Published

2019

26. Pseudomyogenic Hemangioendothelioma Recapitulated in Endothelial Cells from Human Induced Pluripotent Stem Cells Engineered to Express the SERPINE1-FOSB Translocation

Author

Christine L. Mummery, Valeria V. Orlova, Inge H. Briaire-de Bruijn, Danielle de Jong, Francijna E. van den Hil, Karoly Szuhai, Judith V.M.G. Bovée, David G.P. van IJzendoorn, and Daniela C.F. Salvatori

Subjects

Tube formation, Transcriptome, Transplantation, Fusion gene, Cell culture, Chromosomal translocation, Biology, Pseudomyogenic Hemangioendothelioma, Cell biology, FOSB

Abstract

Chromosomal translocations are prevalent among soft tissue tumors including those of the vasculature. Pseudomyogenic hemangioendothelioma (PHE) is one such tumor. It has features of endothelial cells (ECs) and a tumor-specific t(7;19)(q22;q13) SERPINE1-FOSB translocation, but has been difficult to study since to date no cell lines have been derived from the tumor. To address this, we engineered the PHE chromosomal translocation into human induced pluripotent stem cells (hiPSCs) using CRISPR/Cas9 and differentiated these into ECs (hiPSC-ECs). Comparison of parental and modified (PHE) lines with the t(7;19)(q22;q13) SERPINE1-FOSB translocation showed (i) elevated expression of FOSB specifically in hiPSC-ECs in vitro and in vivo (ii) increased proliferation and tube formation but decreased endothelial barrier function (iii) transcriptome alterations specific for hiPSC-ECs that reflect typical PHE histopathological features (iv) invasive growth and abnormal vessel formation in mouse after transplantation of the mutated cells. hiPSC-ECs carrying the SERPINE1-FOSB translocation thus recapitulated functional features of PHE and demonstrated that this approach can yield models of translocation-driven tumors for identification of therapeutic targets and deeper understanding of underlying tumorigenic mechanisms.

Published

2019

27. Fusion events lead to truncation ofFOSin epithelioid hemangioma of bone

Author

Karoly Szuhai, Judith V.M.G. Bovée, Piero Picci, Cleofe Romagosa, David G.P. van IJzendoorn, Maria Serena Benassi, Marco Gambarotti, Danielle de Jong, Soeren Daugaard, and Michiel A. J. van de Sande

Subjects

Genetics, Cancer Research, Translocation Breakpoint, Chromosomal translocation, Biology, medicine.disease, Stop codon, Fusion gene, Transactivation, Exon, medicine, Cancer research, Epithelioid hemangioendothelioma, Epithelioid Hemangioma

Abstract

Epithelioid hemangioma of bone is a locally aggressive vascular neoplasm. It can be challenging to diagnose because of the wide histological spectrum, which can make it difficult to differentiate from other vascular neoplasms such as epithelioid hemangioendothelioma or epithelioid angiosarcoma. COBRA-FISH karyotyping identified a balanced t(3;14) translocation. Transcriptome sequencing of the index case and two other epithelioid hemangiomas revealed a recurrent translocation breakpoint involving the FOS gene, which was fused to different partners in all three cases. The break was observed in exon 4 of the FOS gene and the fusion event led to the introduction of a stop codon. In all instances, the truncation of the FOS gene would result in the loss of the transactivation domain (TAD). Using FISH probes we found a break in the FOS gene in two additional cases, in none of these cases a recurrent fusion partner could be identified. In total, FOS was split in 5/7 evaluable samples. We did not observe point mutations leading to early stop codons in any of the 10 cases where RNA was available. Detection of FOS rearrangement may be a useful diagnostic tool to assist in the often difficult differential diagnosis of vascular tumors of bone. Our data suggest that the translocation causes truncation of the FOS protein, with loss of the TAD, which is thereby a novel mechanism involved in tumorigenesis.

Published

2015

28. Flow-S: A Field-Deployable Device with Minimal Hands-On Effort to Concentrate and Quantify Schistosoma Circulating Anodic Antigen (CAA) from Large Urine Volumes

Author

Daniëlle de Jong, Cody Carrell, Jane K. Maganga, Loyce Mhango, Peter S. Shigella, Maddy Gill, Ryan Shogren, Brianna Mullins, Jay W. Warrick, John M. Changalucha, Govert J. van Dam, Khanh Pham, Jennifer A. Downs, and Paul L. A. M. Corstjens

Subjects

circulating anodic antigen, CAA, equipment-free, field-deployable, lateral flow, LF, Medicine (General), R5-920

Abstract

A laboratory-based lateral flow (LF) test that utilizes up-converting reporter particles (UCP) for ultrasensitive quantification of Schistosoma circulating anodic antigen (CAA) in urine is a well-accepted test to identify active infection. However, this UCP-LF CAA test requires sample pre-treatment steps not compatible with field applications. Flow, a new low-cost disposable, allows integration of large-volume pre-concentration of urine analytes and LF detection into a single field-deployable device. We assessed a prototype Flow-Schistosoma (Flow-S) device with an integrated UCP-LF CAA test strip, omitting all laboratory-based steps, to enable diagnosis of active Schistosoma infection in the field using urine. Flow-S is designed for large-volume (5–20 mL) urine, applying passive paper-based filtration and antibody-based CAA concentration. Samples tested for schistosome infection were collected from women of reproductive age living in a Tanzania region where S. haematobium infection is endemic. Fifteen negative and fifteen positive urine samples, selected based on CAA levels quantified in paired serum, were analyzed with the prototype Flow-S. The current Flow-S prototype, with an analytical lower detection limit of 1 pg CAA/mL, produced results correlated with the laboratory-based UCP-LF CAA test. Urine precipitates occurred in frozen banked samples and affected accurate quantification; however, this should not occur in fresh urine. Based on the findings of this study, Flow-S appears suitable to replace the urine pre-treatment required for the laboratory-based UCP-LF CAA test, thus allowing true field-based applications with fresh urine samples. The urine precipitates observed with frozen samples, though less important given the goal of testing fresh urines, warrant additional investigation to evaluate methods for mitigation. Flow-S devices permit testing of pooled urine samples with applications for population stratified testing. A field test with fresh urine samples, a further optimized Flow-S device, and larger statistical power has been scheduled.

Published

2024

29. Protein nanobarcodes enable single-step multiplexed fluorescence imaging.

Author

Daniëlle de Jong-Bolm, Mohsen Sadeghi, Cristian A Bogaciu, Guobin Bao, Gabriele Klaehn, Merle Hoff, Lucas Mittelmeier, F Buket Basmanav, Felipe Opazo, Frank Noé, and Silvio O Rizzoli

Subjects

Biology (General), QH301-705.5

Abstract

Multiplexed cellular imaging typically relies on the sequential application of detection probes, as antibodies or DNA barcodes, which is complex and time-consuming. To address this, we developed here protein nanobarcodes, composed of combinations of epitopes recognized by specific sets of nanobodies. The nanobarcodes are read in a single imaging step, relying on nanobodies conjugated to distinct fluorophores, which enables a precise analysis of large numbers of protein combinations. Fluorescence images from nanobarcodes were used as input images for a deep neural network, which was able to identify proteins with high precision. We thus present an efficient and straightforward protein identification method, which is applicable to relatively complex biological assays. We demonstrate this by a multicell competition assay, in which we successfully used our nanobarcoded proteins together with neurexin and neuroligin isoforms, thereby testing the preferred binding combinations of multiple isoforms, in parallel.

Published

2023

30. Human Extravillous Trophoblasts Penetrate Decidual Veins and Lymphatics before Remodeling Spiral Arteries during Early Pregnancy

Author

Frans M. Helmerhorst, Karoly Szuhai, Susana M. Chuva de Sousa Lopes, Lucette A. J. van der Westerlaken, Liesbeth van Iperen, Danielle de Jong, and Nannan He

Subjects

0301 basic medicine, Embryology, Pathology, Maternal Health, Immunofluorescence, lcsh:Medicine, Endometrium, 0302 clinical medicine, Pregnancy, Medicine and Health Sciences, lcsh:Science, 030219 obstetrics & reproductive medicine, Multidisciplinary, medicine.diagnostic_test, Decidua, Obstetrics and Gynecology, Arteries, Anatomy, Trophoblasts, medicine.anatomical_structure, Lymphatic system, Immunohistochemistry, Female, Research Article, medicine.medical_specialty, Histology, Vascular Remodeling, Research and Analysis Methods, Veins, 03 medical and health sciences, Placenta, medicine, Humans, Immunoassays, Fetus, business.industry, lcsh:R, Uterus, Reproductive System, Biology and Life Sciences, medicine.disease, 030104 developmental biology, Cardiovascular Anatomy, Immunologic Techniques, Blood Vessels, Women's Health, lcsh:Q, Blastocysts, business, Developmental Biology

Abstract

In humans, the defective invasion of the maternal endometrium by fetal extravillous trophoblasts (EVTs) can lead to insufficient perfusion of the placenta, resulting in pregnancy complications that can put both mother and baby at risk. To study the invasion of maternal endometrium between (W)5.5-12 weeks of gestation by EVTs, we combined fluorescence in situ hybridization, immunofluorescence and immunohistochemistry to determine the presence of (male) EVTs in the vasculature of the maternal decidua. We observed that interstitial mononuclear EVTs directly entered decidual veins and lymphatics from W5.5. This invasion of decidual veins and lymphatics occurred long before endovascular EVTs remodelled decidual spiral arteries. This unexpected early entrance of interstitial mononuclear EVTs in the maternal circulation does not seem to contribute to the materno-placental vascular connection directly, but rather to establish (and expand) the materno-fetal interface through an alternative vascular route.

Published

2017

31. Array CGH analysis identifies two distinct subgroups of primary angiosarcoma of bone

Author

Sofie L. J. Verbeke, Karoly Szuhai, Raf Sciot, Danielle de Jong, Judith V.M.G. Bovée, Cristina R. Antonescu, and Franco Bertoni

Subjects

Cancer Research, Candidate gene, Pathology, medicine.medical_specialty, medicine.diagnostic_test, Chromosome, Soft tissue, Primary Angiosarcoma, Biology, Molecular biology, Genetics, medicine, Immunohistochemistry, Angiosarcoma, neoplasms, Comparative genomic hybridization, Fluorescence in situ hybridization

Abstract

Molecular genetic studies on vascular tumors are rare. Recently, possible involvement of MYC and KDR has been documented in a subset of angiosarcomas of soft tissue. We performed a cytogenetic analysis of primary angiosarcomas of bone (n = 13) and soft tissue (n = 5) using high density array-comparative genomic hybridization (array-CGH). Regions of interest were validated by fluorescence in situ hybridization (FISH). Antibodies for candidate genes (SKI, MYC, KDR, and MAPK9) were selected and immunohistochemistry was performed. Six angiosarcomas of bone and four angiosarcomas of soft tissue showed chromosomal losses, gains, and high level amplifications. Cluster analysis identified two groups: a group with a complex genetic profile and a group with only few genetic aberrations. Five regions of interest were selected, which were located at chromosome bands 1p36.23, 2q32-34, 5q35, 8q24, and 17q21.32-24.2. Interphase FISH confirmed the high-level amplifications. Immunohistochemical analysis showed high expression of MYC (16/60), MAPK9 (63/69), and SKI (52/62). There were no differences between the two groups with regards to location, immunohistochemical expression nor survival. In summary, we identified two subgroups of angiosarcoma: those with few or no gross aberrations and those which show numerous genetic aberrations consisting of chromosomal losses, gains and high level amplifications or complex aberrations. The most common finding was amplification of 2q and 17q in both angiosarcoma of bone and soft tissue, suggesting overlap in tumorigenesis irrespective of their location. We show MYC amplification in primary angiosarcoma indicating this is not entirely specific for radiation-induced angiosarcoma. © 2014 Wiley Periodicals, Inc.

Published

2014

32. Transactivating mutation of theMYOD1gene is a frequent event in adult spindle cell rhabdomyosarcoma

Author

Wai Yi Leung, Danielle de Jong, Karoly Szuhai, Christopher D.M. Fletcher, and Pancras C.W. Hogendoorn

Subjects

Genetics, Somatic cell, Sclerosing rhabdomyosarcoma, Biology, medicine.disease, Molecular biology, Pathology and Forensic Medicine, Conserved sequence, medicine, MYF6, MYF5, Embryonal rhabdomyosarcoma, Rhabdomyosarcoma, Spindle cell rhabdomyosarcoma

Abstract

Rhabdomyosarcoma (RMS) is the most common soft-tissue sarcoma in children and adolescents, being characterized by expression of genes and morphological and ultrastructural features of sarcomeric differentiation. The spindle cell variant of rhabdomyosarcoma (spindle cell RMS) in adults has been defined as an entity, separated from embryonal rhabdomyosarcoma (ERMS), with unfavourable clinical outcome. So far, no recurrent genetic alteration has been identified in the adult form of spindle cell RMS. We studied a case of adult spindle cell RMS using next-generation sequencing (NGS) after exome capture. Using this approach, we identified 31 tumour-specific somatic alterations and selected four genes with predicted functional relevance to muscle differentiation and growth. MYOD1, KIF18A, NOTCH1, and EML5 were further tested for mutations using Sanger sequencing on DNA from FFPE samples from 16 additional, adult spindle cell RMS samples. The highly conserved sequence homology of MYOD1 with other myogenic transcription factors prompted us to screen the basic DNA-binding domains of MYF5, MYF6 and MYOG for mutations. From the investigated 17 samples, seven (41%) showed homozygous mutation of MYOD1, indicating a critical role in this rare subtype of adult spindle cell RMS, while no mutations were found in any of the other genes involved in myogenic differentiation. The p.L122R mutation occurs in the conserved DNA binding domain in MYOD1 and leads to transactivation and MYC-like functions. MYOD1 homozygous mutations are frequent, recurrent and pathognomonic events in adult-type spindle cell RMS.

Published

2014

33. Multiplex ligation-dependent probe amplification and fluorescence in situ hybridization are complementary techniques to detect cytogenetic abnormalities in multiple myeloma

Author

Karoly Szuhai, Suvi Savola, Marianna Dávid, Szabolcs Kosztolányi, László Kereskai, Donát Alpár, Béla Kajtár, Zsofia Holczer-Nagy, László Pajor, Pál Jáksó, and Danielle de Jong

Subjects

Cancer Research, Monosomy, medicine.diagnostic_test, Genetic heterogeneity, Biology, medicine.disease, Molecular biology, Multiplex polymerase chain reaction, Genetics, medicine, Multiplex, Multiplex ligation-dependent probe amplification, Hyperdiploidy, Fluorescence in situ hybridization, Chromosome 13

Abstract

Multiple myeloma (MM) is a genetically heterogeneous disease with diverse clinical outcomes. Interphase fluorescence in situ hybridization (i-FISH) is the most commonly used approach to detect recurrent cytogenetic abnormalities in this malignancy. We aimed to assess the performance of multiplex ligation-dependent probe amplification (MLPA) to reveal copy number abnormalities (CNAs) in MM. Diagnostic bone marrow samples from 81 patients were analyzed using 42 MLPA probes for the following regions: 1p32-31, 1p21, 1q21.3, 1q23.3, 5q31.3, 12p13.31, 13q14, 16q12, 16q23, and 17p13. All samples were also screened by i-FISH for the presence of hyperdiploidy, deletion/monosomy of chromosome 13, deletion of TP53, disruption of the immunoglobulin heavy-chain gene, t(4;14), t(11;14), t(14;16), t(8;14), gain of 5q and abnormalities of chromosome 1. A total of 245 alterations were detected in 79 cases (98%). Investigating the same aberrations, the two methods showed a congruency of higher than 90%. A low proportion of cells with the relevant abnormality, focal CNAs and unmatched probes were responsible for the discrepancies. MLPA revealed 95 CNAs not detected by i-FISH providing additional information in 53 cases (65%). Scrutiny of CNAs on chromosome 1, using more than 20 probes, revealed significant heterogeneity in size and location, and variable intra-chromosomal and intra-clonal rates of loss or gain. Our results suggest that MLPA is a reliable high-throughput technique to detect CNAs in MM. Since balanced aberrations are key to prognostic classification of this disease, MLPA and i-FISH should be applied as complementary techniques in diagnostic pathology.

Published

2013

34. p120-catenin prevents multinucleation through control of MKLP1-dependent RhoA activity during cytokinesis

Author

Jolien S. de Groot, Paul J. van Diest, Danielle de Jong, Robert A. H. van de Ven, Erik Sahai, Carlos Caldas, Martin W. Hetzer, Karoly Szuhai, Patrick W. B. Derksen, H. Raza Ali, Oscar M. Rueda, Danielle Park, Elsken van der Wall, Robert van Domselaar, Szuhai, Karoly [0000-0002-1228-4245], and Apollo - University of Cambridge Repository

Subjects

0301 basic medicine, Delta Catenin, RHOA, animal structures, Science, General Physics and Astronomy, Breast Neoplasms, Kaplan-Meier Estimate, Biology, General Biochemistry, Genetics and Molecular Biology, Article, 03 medical and health sciences, Cell Line, Tumor, Journal Article, Cell Adhesion, Animals, Humans, Cleavage furrow, Cell adhesion, Anaphase, Cytokinesis, Mice, Knockout, Multidisciplinary, Cadherin, Catenins, General Chemistry, 3. Good health, Cell biology, 030104 developmental biology, Centralspindlin, Catenin, embryonic structures, biology.protein, Female, rhoA GTP-Binding Protein, Microtubule-Associated Proteins, HeLa Cells, Protein Binding

Abstract

Spatiotemporal activation of RhoA and actomyosin contraction underpins cellular adhesion and division. Loss of cell–cell adhesion and chromosomal instability are cardinal events that drive tumour progression. Here, we show that p120-catenin (p120) not only controls cell–cell adhesion, but also acts as a critical regulator of cytokinesis. We find that p120 regulates actomyosin contractility through concomitant binding to RhoA and the centralspindlin component MKLP1, independent of cadherin association. In anaphase, p120 is enriched at the cleavage furrow where it binds MKLP1 to spatially control RhoA GTPase cycling. Binding of p120 to MKLP1 during cytokinesis depends on the N-terminal coiled-coil domain of p120 isoform 1A. Importantly, clinical data show that loss of p120 expression is a common event in breast cancer that strongly correlates with multinucleation and adverse patient survival. In summary, our study identifies p120 loss as a driver event of chromosomal instability in cancer., The tumour suppressor p120-catenin (p120) controls cadherin-based adhesion. Here, the authors demonstrate that p120 regulates cytokinesis through binding to the centralspindlin component MKLP1 and controls RhoA activity. Loss of p120 in cancer induces multinucleation and chromosomal instability, independent of cell-cell adhesion.

Published

2016

35. Analysis of steric effects in DamID profiling of transcription factor target genes

Author

Mirana Ramialison, Nicole Schonrock, Ashley J. Waardenberg, Richard P. Harvey, Tram Doan, Danielle de Jong, and Romaric Bouveret

Subjects

0301 basic medicine, Heart Defects, Congenital, Serum Response Factor, Site-Specific DNA-Methyltransferase (Adenine-Specific), Methyltransferase, Mutant, Biology, 03 medical and health sciences, chemistry.chemical_compound, Mice, Serum response factor, Genetics, Animals, Humans, ets-Domain Protein Elk-4, Transcription factor, Gene, ets-Domain Protein Elk-1, Wild type, DNA, Molecular biology, Chromatin, Cell biology, 030104 developmental biology, chemistry, Gene Expression Regulation, Genetic Techniques, Homeobox Protein Nkx-2.5

Abstract

DNA adenine methyltransferase identification (DamID) is an enzymatic technology for detecting DNA regions targeted by chromatin-associated proteins. Proteins are fused to bacterial DNA adenine methyltransferase (Dam) and expressed in cultured cells or whole organisms. Here, we used DamID to detect DNA regions bound by the cardiac-restricted transcription factors (TFs) NKX2-5 and SRF, and ubiquitously-expressed co-factors ELK1 and ELK4. We compared targets bound by these TFs as N- and C-terminal fusions with Dam, for both wild type (WT) NKX2-5 and mutant proteins mimicking those found in congenital heart disease. Overall, DamID is highly robust: while the orientation of WT Dam fusions can affect the size of the target sets, their signatures remained largely reproducible. Furthermore, a severe NKX2-5 mutant lacking the homeodomain showed strong steric effects negatively impacting target discovery. The extent of steric effect is likely to be dependent on the protein in question and the orientation of Dam fusion.

Published

2016

36. Inhibition of Bcl-2 family members sensitizes mesenchymal chondrosarcoma to conventional chemotherapy: report on a novel mesenchymal chondrosarcoma cell line

Author

Hans Gelderblom, Alwine B. Kruisselbrink, Yvonne de Jong, Jonathan A. Fletcher, Annemiek M. van Maldegem, Adrián Mariño-Enríquez, Judith V.M.G. Bovée, Karoly Szuhai, Inge H. Briaire-de Bruijn, Anne-Marie Cleton-Jansen, Johnny Suijker, and Danielle de Jong

Subjects

0301 basic medicine, Adult, Male, Pathology, medicine.medical_specialty, Antineoplastic Agents, Piperazines, Pathology and Forensic Medicine, Nitrophenols, 03 medical and health sciences, 0302 clinical medicine, Cell Line, Tumor, medicine, Humans, Doxorubicin, Viability assay, Molecular Biology, Cisplatin, Sulfonamides, business.industry, Mesenchymal stem cell, Bcl-2 family, Biphenyl Compounds, Cell Biology, medicine.disease, Mesenchymal chondrosarcoma, 030104 developmental biology, Proto-Oncogene Proteins c-bcl-2, Cell culture, Drug Resistance, Neoplasm, 030220 oncology & carcinogenesis, Cancer research, Chondrosarcoma, Mesenchymal, Chondrosarcoma, business, medicine.drug

Abstract

Mesenchymal chondrosarcomas are rare and highly aggressive sarcomas occurring in bone and soft tissue, with poor overall survival. Bcl-2 expression was previously shown to be upregulated in mesenchymal chondrosarcomas. We here report on a newly derived mesenchymal chondrosarcoma cell line, MCS170, in which we investigated treatment with the BH3 mimetic ABT-737 alone or in combination with conventional chemotherapy as a possible new therapeutic strategy. The presence of the characteristic HEY1-NCOA2 fusion was confirmed in the MCS170 cell line using FISH, RT-PCR, and sequencing. The MCS170 cell line was treated with ABT-737 alone or in combination with doxorubicin or cisplatin. Cell viability and proliferation was determined using WST-1 viability assays and the xCELLigence system. Expression of Bcl-2 family members was studied using immunohistochemistry. Apoptosis was determined using the caspase-glo 3/7 assay and western blot for PARP cleavage. The MCS170 cell line was sensitive to doxorubicin treatment with an IC50 of 0.09 μM after 72 h, but more resistant to cisplatin treatment with an IC50 of 4.5 μM after 72 h. Cells showed little sensitivity toward ABT-737 with an IC50 of 1.8 μM after 72 h. Combination treatments demonstrated ABT-737 synergism with cisplatin as well as doxorubicin as shown by induction of apoptosis and reduction in cell proliferation. Restoration of the apoptotic machinery by inhibition of Bcl-2 family members sensitizes MCS170 mesenchymal chondrosarcoma cells to conventional chemotherapy. This indicates that combining the inhibition of Bcl-2 family members with conventional chemotherapy can be a possible therapeutic strategy for patients with mesenchymal chondrosarcoma.

Published

2016

37. Characterization of a New Human Cell Line (CH-3573) Derived from a Grade II Chondrosarcoma with Matrix Production

Author

Danielle de Jong, José Antonio López-Guerrero, Silvia Calabuig-Fariñas, Amando Peydró, Antonio Pellín, Rosario Gil Benso, Lara Navarro, Karoly Szuhai, Isidro Machado, Antonio Llombart-Bosch, and Teresa San Miguel

Subjects

Adult, Male, Cancer Research, Pathology, medicine.medical_specialty, Karyotype, Transplantation, Heterologous, Chondrosarcoma, Mice, Nude, Bone Neoplasms, Biology, Pathology and Forensic Medicine, Mice, Grade II, In vivo, Cell Line, Tumor, medicine, Animals, Humans, Bone tumor, In Situ Hybridization, Fluorescence, Matrix, General Medicine, medicine.disease, Immunohistochemistry, Primary tumor, In vitro, Neoplasm Proteins, Oncology, Cell culture, Tumor progression, Grade II Chondrosarcoma, Neoplasm Grading, Cell line

Abstract

Chondrosarcomas are malignant cartilage-forming tumors that represent the third most common malignant solid tumor of bone. In patients with grades II and III, local recurrence, increasing tumor size and dedifferentiation have been associated with lower survival rates. These biologically poorly-understood neoplasms vary considerably in clinical presentation and biological behavior. Cytogenetic studies have shown that heterogeneity is related to karyotypic complexity; moreover, alterations in the 9p21 locus and TP53 gene are related to disease progression. Despite the relatively high frequency of chondrosarcoma only a limited number of cell lines exist in the scientific community, limiting the possibility to study hypothesis-derived research or primary drug interaction necessary for pre-clinical studies. We report a chondrosarcoma cell line, CH-3573, derived from a primary tumor that may serve as a useful tool for both in vitro and in vivo models to study the molecular pathogenesis. In addition, xenograft passages in nude mice were studied to characterize the genetic stability over the course of tumor progression. In contrary to other reported cell lines, an important feature of our established cell line was the retained matrix production, a characteristic feature of a conventional grade II chondrosarcoma. The cell line (CH-3573) was characterized by pathological, immunohistochemical and molecular genetic methods.

Published

2012

38. Heterogeneous and Complex Rearrangements of Chromosome Arm 6q in Chondromyxoid Fibroma

Author

Salvatore Romeo, Ronald A J Duim, Pauline M. Wijers-Koster, Karoly Szuhai, Raphael Sciot, Fredrik Mertens, Danielle de Jong, Julia A. Bridge, Andrew E. Rosenberg, Maria Debiec-Rychter, Pancras C.W. Hogendoorn, and Paola Dal Cin

Subjects

Genetics, Candidate gene, medicine.diagnostic_test, Breakpoint, Chondromyxoid fibroma, In situ hybridization, Gene rearrangement, Biology, medicine.disease, Pathology and Forensic Medicine, Gene mapping, medicine, Fluorescence in situ hybridization, Comparative genomic hybridization

Abstract

Chondromyxoid fibroma (CMF) is an uncommon benign cartilaginous tumor of bone usually occurring during the second decade of life. CMF is associated with recurrent rearrangements of chromosome bands 6p23-25, 6q12-15, and 6q23-27. To delineate further the role and frequency of the involvement of three candidate regions (6q13, 6q23.3 and 6q24) in the pathogenesis of CMF, we studied a group of 43 cases using a molecular cytogenetic approach. Fluorescence in situ hybridization with probe sets bracketing the putative breakpoint regions was performed in 30 cases. The expression level of nearby candidate genes was studied by immunohistochemistry and quantitative RT-PCR in 24 and 23 cases, respectively. Whole-genome copy number screening was performed by array comparative genomic hybridization in 16 cases. Balanced and unbalanced rearrangements of 6q13 and 6q23.3 occurred in six and five cases, respectively, and a hemizygous deletion in 6q24 was found in five cases. Two known tumor suppressor genes map to the latter region: PLAGL1 and UTRN. However, neither of these two genes nor BCLAF1 and COL12A1, respectively located in 6q23.3 and 6q13, showed altered expression. Therefore, although rearrangements of chromosomal regions 6q13, 6q23.3, and 6q24 are common in CMF, the complexity of the changes precludes the use of a single fluorescence in situ hybridization probe set as an adjunct diagnostic tool. These data indicate that the genetic alterations in CMF are heterogeneous and are likely a result of a cryptic rearrangement beyond the resolution level of combined binary ratio fluorescence in situ hybridization or a point mutation.

Published

2010

39. Osteosarcoma originates from mesenchymal stem cells in consequence of aneuploidization and genomic loss of Cdkn2

Author

Alexander B. Mohseny, Inge H. Briaire-de Bruijn, Karoly Szuhai, Anne-Marie Cleton-Jansen, Pancras C.W. Hogendoorn, Emilie P. Buddingh, Melissa van Pel, Danielle de Jong, and Salvatore Romeo

Subjects

musculoskeletal diseases, Pathology, medicine.medical_specialty, Tumor suppressor gene, Mesenchymal stem cell, Biology, medicine.disease, Pathology and Forensic Medicine, Malignant transformation, Germline mutation, CDKN2A, medicine, Osteosarcoma, Sarcoma, Stem cell, neoplasms

Abstract

High-grade osteosarcoma is characterized by extensive genetic instability, thereby hampering the identification of causative gene mutations and understanding of the underlying pathological processes. It lacks a benign precursor lesion and reports on associations with hereditary predisposition or germline mutations are uncommon, despite the early age of onset. Here we demonstrate a novel comprehensive approach for the study of premalignant stages of osteosarcoma development in a murine mesenchymal stem cell (MSC) system that formed osteosarcomas upon grafting. By parallel functional and phenotypic analysis of normal MSCs, transformed MSCs and derived osteosarcoma cells, we provide substantial evidence for a MSC origin of osteosarcoma. In a stepwise approach, using COBRA-FISH karyotyping and array CGH in different passages of MSCs, we identified aneuploidization, translocations and homozygous loss of the cdkn2 region as the key mediators of MSC malignant transformation. We then identified CDKN2A/p16 protein expression in 88 osteosarcoma patients as a sensitive prognostic marker, thereby bridging the murine MSCs model to human osteosarcoma. Moreover, occasional reports in patients mention osteosarcoma formation following bone marrow transplantation for an unrelated malignancy. Our findings suggest a possible hazard for the clinical use of MSCs; however, they also offer new opportunities to study early genetic events in osteosarcoma genesis and, more importantly, to modulate these events and record the effect on tumour progression. This could be instrumental for the identification of novel therapeutic strategies, since the success of the current therapies has reached a plateau phase.

Published

2009

40. Long–term culture of primary human lymphoblastic leukemia cells in the absence of serum or hematopoietic growth factors

Author

Erik W.A. Marijt, H. M. Goselink, Marja van der Burg, Karoly Szuhai, Oliver G. Ottmann, Danielle de Jong, Bart A. Nijmeijer, J.H. Frederik Falkenburg, Roel Willemze, and Marianke L.J. van Schie

Subjects

Cancer Research, Time Factors, Cell Culture Techniques, Blastic Phase, Biology, Culture Media, Serum-Free, hemic and lymphatic diseases, Leukemia, B-Cell, Genetics, medicine, Humans, Molecular Biology, Cell Proliferation, ABL, breakpoint cluster region, Myeloid leukemia, Imatinib, Cell Biology, Hematology, Precursor Cell Lymphoblastic Leukemia-Lymphoma, medicine.disease, Leukemia, Haematopoiesis, Cell culture, Immunology, Intercellular Signaling Peptides and Proteins, medicine.drug

Abstract

Objective B–lineage acute lymphoblastic leukemia (ALL) and chronic myeloid leukemia in lymphatic blastic phase in adults have poor prognoses despite intensive chemotherapy. Novel targeted treatment modalities emerge, but their evaluation requires relevant in vitro models of lymphoblastic leukemia. Presently available cell lines do not fully represent this heterogeneous disease. Available in vitro culturing protocols do not support long–term proliferation of primary cells. We therefore aimed to develop a culture system that allows long–term proliferation of primary human B–lineage lymphoblastic leukemia. Materials and Methods Primary lymphoblastic leukemia cells were cultured in a defined serum–free medium, in the absence or presence of human hematopoietic growth factors or serum. Results In the defined serum–free medium, cells from 12 of 34 cases immediately proliferated in vitro. In the absence of hematopoietic growth factors and serum these cases proliferated for more than 1 year without signs of exhaustion. The culturing system supported different subtypes of lymphoblastic leukemia. Two chronic myeloid leukemia in lymphatic blastic phase, four bcr/abl–positive ALL, one etv6/abl–positive ALL, 2 e2a–pbx1−positive ALL, and one t(9;11)–positive ALL could be long–term expanded, as well as two ALL that displayed nontypical cytogenetics. Not all bcr/abl– or e2a–pbx1−positive ALL proliferated in vitro, demonstrating heterogeneity within these subtypes. The proliferating bcr/abl– and etv6/abl–positive cells displayed sensitivity to imatinib, demonstrating that their proliferation depended on the activity of these oncoproteins. Conclusion The serum–free culturing system may be a valuable instrument in the study of ALL cell biology, as well as in the evaluation of novel targeted therapeutics.

Published

2009

41. NKX2-5 mutations causative for congenital heart disease retain functionality and are directed to hundreds of targets

Author

Gavin Chapman, Romaric Bouveret, Nicole Schonrock, Gurpreet Kaur, Richard P. Harvey, Hananeh Fonoudi, Shoumo Bhattacharya, Tram Doan, Chiann-mun Chen, Cédric Blanpain, Antoine Bondue, Mirana Ramialison, Merridee A. Wouters, Nicolas Plachta, Ashley J. Waardenberg, Sally L. Dunwoodie, Danielle de Jong, and Stephanie Mohamed

Subjects

QH301-705.5, Science, Mutant, Gene regulatory network, Biology, medicine.disease_cause, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, 0302 clinical medicine, genetic disease, medicine, Biology (General), Gene, Transcription factor, transcription factor, 030304 developmental biology, Genetics, 0303 health sciences, Mutation, General Immunology and Microbiology, General Neuroscience, cardiogenesis, Wild type, General Medicine, 3. Good health, embryonic structures, cardiovascular system, Medicine, Homeobox, Functional genomics, 030217 neurology & neurosurgery

Abstract

We take a functional genomics approach to congenital heart disease mechanism. We used DamID to establish a robust set of target genes for NKX2-5 wild type and disease associated NKX2-5 mutations to model loss-of-function in gene regulatory networks. NKX2-5 mutants, including those with a crippled homeodomain, bound hundreds of targets including NKX2-5 wild type targets and a unique set of "off-targets", and retained partial functionality. NKXΔHD, which lacks the homeodomain completely, could heterodimerize with NKX2-5 wild type and its cofactors, including E26 transformation-specific (ETS) family members, through a tyrosine-rich homophilic interaction domain (YRD). Off-targets of NKX2-5 mutants, but not those of an NKX2-5 YRD mutant, showed overrepresentation of ETS binding sites and were occupied by ETS proteins, as determined by DamID. Analysis of kernel transcription factor and ETS targets show that ETS proteins are highly embedded within the cardiac gene regulatory network. Our study reveals binding and activities of NKX2-5 mutations on WT target and off-targets, guided by interactions with their normal cardiac and general cofactors, and suggest a novel type of gain-of-function in congenital heart disease.

Published

2015

42. Author response: NKX2-5 mutations causative for congenital heart disease retain functionality and are directed to hundreds of targets

Author

Mirana Ramialison, Gavin Chapman, Antoine Bondue, Sally L. Dunwoodie, Richard P. Harvey, Ashley J. Waardenberg, Hananeh Fonoudi, Nicole Schonrock, Merridee A. Wouters, Tram Doan, Danielle de Jong, Nicolas Plachta, Stephanie Mohamed, Romaric Bouveret, Gurpreet Kaur, Chiann-mun Chen, Cédric Blanpain, and Shoumo Bhattacharya

Subjects

Heart disease, business.industry, medicine, medicine.disease, business, Bioinformatics

Published

2015

43. A translocation t(6;14) in two cases of leiomyosarcoma: Molecular cytogenetic and array-based comparative genomic hybridization characterization

Author

Judith V.M.G. Bovée, Marieke A. de Graaff, Danielle de Jong, Pancras C.W. Hogendoorn, Karoly Szuhai, and Inge H. Briaire-de Bruijn

Subjects

Leiomyosarcoma, Cancer Research, HMGA1, Smooth muscle cell differentiation, translocation, Chromosomal translocation, Locus (genetics), Biology, Translocation, Genetic, FISH, Gene duplication, Genetics, medicine, Tumor Cells, Cultured, Humans, Actinin, HMGA1a Protein, Molecular Biology, In Situ Hybridization, Fluorescence, Chromosomes, Human, Pair 14, Comparative Genomic Hybridization, medicine.diagnostic_test, Breakpoint, Karyotype, medicine.disease, Molecular biology, body regions, Tissue Array Analysis, soft tissue sarcoma, array-CGH, Mutation, Chromosomes, Human, Pair 6, Fluorescence in situ hybridization

Abstract

Leiomyosarcomas are malignant mesenchymal tumors that recapitulate smooth muscle cell differentiation. Tumors are characterized by a genetic heterogeneity with complex karyotypes without a tumor-specific genetic aberration. Their pathobiology is still poorly understood and no specific targeted treatment is currently available for these aggressive tumors. For six leiomyosarcomas, cells were cultured and analyzed by combined binary ratio labeling fluorescence in situ hybridization (COBRA-FISH) karyotyping. A t(6;14) was identified in two cases. FISH breakpoint mapping of case L1339 reveals a breakpoint at chromosome 6p21.31 close to HMGA1 , and a small deletion was observed on the distal side of the gene. A small homozygous deletion was also found in the breakpoint region of chromosome 14q24.1 involving ACTN1 . The second case revealed a der(6)t(6;14)(p21.1;q21.3), with a duplication adjacent to the breakpoint at chromosome 6. Confirmatory FISH revealed a second leiomyosarcoma with an aberration at 14q24.1. Alterations at this locus were found in 5% (2 of 39) of the leiomyosarcomas in this study. The other identified breakpoints appeared to be non-recurrent, because they were not detected in other leiomyosarcomas, uterine leiomyomas, undifferentiated spindle cell sarcomas, or undifferentiated pleomorphic sarcomas.

Published

2015

44. Fusion events lead to truncation of FOS in epithelioid hemangioma of bone

Author

David G P, van IJzendoorn, Danielle, de Jong, Cleofe, Romagosa, Piero, Picci, Maria Serena, Benassi, Marco, Gambarotti, Soeren, Daugaard, Michiel, van de Sande, Karoly, Szuhai, and Judith V M G, Bovée

Subjects

Adult, Aged, 80 and over, Male, RNA-Binding Proteins, Bone Neoplasms, Exons, Middle Aged, Translocation, Genetic, Oncogene Proteins v-fos, Karyotyping, Humans, Female, Gene Fusion, Hemangioma, Transcriptome

Abstract

Epithelioid hemangioma of bone is a locally aggressive vascular neoplasm. It can be challenging to diagnose because of the wide histological spectrum, which can make it difficult to differentiate from other vascular neoplasms such as epithelioid hemangioendothelioma or epithelioid angiosarcoma. COBRA-FISH karyotyping identified a balanced t(3;14) translocation. Transcriptome sequencing of the index case and two other epithelioid hemangiomas revealed a recurrent translocation breakpoint involving the FOS gene, which was fused to different partners in all three cases. The break was observed in exon 4 of the FOS gene and the fusion event led to the introduction of a stop codon. In all instances, the truncation of the FOS gene would result in the loss of the transactivation domain (TAD). Using FISH probes we found a break in the FOS gene in two additional cases, in none of these cases a recurrent fusion partner could be identified. In total, FOS was split in 5/7 evaluable samples. We did not observe point mutations leading to early stop codons in any of the 10 cases where RNA was available. Detection of FOS rearrangement may be a useful diagnostic tool to assist in the often difficult differential diagnosis of vascular tumors of bone. Our data suggest that the translocation causes truncation of the FOS protein, with loss of the TAD, which is thereby a novel mechanism involved in tumorigenesis.

Published

2015

45. GRM1 is upregulated through gene fusion and promoter swapping in chondromyxoid fibroma

Author

Judith V.M.G. Bovée, Jenny Nilsson, Danielle de Jong, Karoly Szuhai, Johnbosco Tayebwa, Karolin Hansén Nord, Henrik Lilljebjörn, Linda Magnusson, Francesco Vezzi, and Pancras C.W. Hogendoorn

Subjects

DNA Copy Number Variations, Molecular Sequence Data, Bone Neoplasms, In situ hybridization, Fibroma, Biology, Real-Time Polymerase Chain Reaction, Receptors, Metabotropic Glutamate, Fusion gene, Genetics, medicine, Coding region, Humans, Receptor, Promoter Regions, Genetic, Gene, In Situ Hybridization, Fluorescence, Netherlands, Regulation of gene expression, Base Sequence, Reverse Transcriptase Polymerase Chain Reaction, Sequence Analysis, RNA, Chondromyxoid fibroma, Glutamate receptor, medicine.disease, Cell biology, Chromosome Banding, Gene Expression Regulation, Neoplastic, Gene Fusion, Signal Transduction

Abstract

Glutamate receptors are well-known actors in the central and peripheral nervous systems, and altered glutamate signaling is implicated in several neurological and psychiatric disorders. It is increasingly recognized that such receptors may also have a role in tumor growth. Here we provide direct evidence of aberrant glutamate signaling in the development of a locally aggressive bone tumor, chondromyxoid fibroma (CMF). We subjected a series of CMFs to whole-genome mate-pair sequencing and RNA sequencing and found that the glutamate receptor gene GRM1 recombines with several partner genes through promoter swapping and gene fusion events. The GRM1 coding region remains intact, and 18 of 20 CMFs (90%) showed a more than 100-fold and up to 1,400-fold increase in GRM1 expression levels compared to control tissues. Our findings unequivocally demonstrate that direct targeting of GRM1 is a necessary and highly specific driver event for CMF development.

Published

2014

46. Generation of induced pluripotent stem cells from human foetal fibroblasts using the Sleeping Beauty transposon gene delivery system

Author

Eszter Varga, Karoly Szuhai, Konstantinos Gkatzis, Georgios Kosmidis, Csilla Nemes, Christian Freund, Christine L. Mummery, Andras Dinnyes, Richard P. Davis, and Danielle de Jong

Subjects

Transposable element, Cancer Research, Induced Pluripotent Stem Cells, Context (language use), Gene delivery, Biology, Insertional mutagenesis, 03 medical and health sciences, 0302 clinical medicine, Nuclear reprogramming, Humans, Human Induced pluripotent stem cell, Induced pluripotent stem cell, Molecular Biology, Transposase, Cells, Cultured, Embryonic Stem Cells, 030304 developmental biology, Genetics, 0303 health sciences, Gene Transfer Techniques, Cell Differentiation, Cell Biology, Fibroblasts, Sleeping Beauty transposon system, Cellular Reprogramming, Cell biology, Differentiation, Transfection methods, DNA Transposable Elements, Sleeping Beauty transposon, Reprogramming, 030217 neurology & neurosurgery, Developmental Biology

Abstract

Transposon gene delivery systems offer an alternative, non-viral-based approach to generate induced pluripotent stem cells (iPSCs). Here we used the Sleeping Beauty (SB) transposon to generate four human iPSC lines from foetal fibroblasts. In contrast to other gene delivery systems, the SB transposon does not exhibit an integration bias towards particular genetic elements, thereby reducing the risk of insertional mutagenesis. Furthermore, unlike the alternative transposon piggyBac, SB has no SB-like elements within the human genome, minimising the possibility of mobilising endogenous transposon elements. All iPSC lines exhibited the expected characteristics of pluripotent human cells, including the ability to differentiate to derivatives of all three germ layers in vitro. Re-expression of the SB transposase in the iPSCs after reprogramming resulted in the mobilisation of some of the transposons. These results indicate that the SB transposon system is a useful addition to methods for generating human iPSCs, both for basic and applied biomedical research, and in the context of future therapeutic application.

Published

2013

47. Intronic deletion and duplication proximal of the EXT1 gene: A novel causative mechanism for multiple osteochondromas

Author

Judith V.M.G. Bovée, Marcel G. T. Winter, Danielle de Jong, Cathelijn J. F. Waaijer, Christianne M. A. Reijnders, Karoly Szuhai, and S. John Ham

Subjects

Male, Cancer Research, Multiple osteochondroma, DNA Mutational Analysis, Locus (genetics), Biology, N-Acetylglucosaminyltransferases, Germline, Gene Duplication, Gene duplication, Genetics, Humans, Genetic Predisposition to Disease, Gene, Family Health, Base Sequence, Breakpoint, Intron, Molecular biology, Introns, Pedigree, Female, Exostoses, Multiple Hereditary, Gene Deletion

Abstract

Multiple osteochondromas (MO) is a syndrome in which benign cartilage-capped neoplasms develop at the surface of the long bones. Most cases are caused by exonic changes in EXT1 or EXT2, but 15% are negative for these changes. Here we report for the first time a family of MO patients with germline genomic alterations at the EXT1 locus without detectable mutations or copy number alterations of EXT exonic sequences. Array-CGH showed an 80.7 kb deletion of Intron 1 of EXT1 and a 68.9 kb duplication proximal of EXT1. We identified a breakpoint between the distal end of the duplicated region and a sequence distal of the deleted region in the first intron. This breakpoint was absent in non-affected family members. The configuration of the breakpoint indicates a direct insertion of the duplicated region into the deletion. However, no other breakpoint was found, which suggests a more complex genomic rearrangement has occurred within the duplicated region. Our results reveal intronic deletion and duplication as a new causative mechanism for MO not detected by conventional diagnostic methods.

Published

2013

48. Do injection drug users have more adverse events during procedural sedation and analgesia for incision and drainage of cutaneous abscesses?

Author

Eric Grafstein, Danielle de Jong, Gary Andolfatto, Lisa Lange, Frank X. Scheuermeyer, and Hong Qian

Subjects

Adult, Male, medicine.medical_specialty, medicine.medical_treatment, Sedation, Vital signs, Conscious Sedation, Drug Users, Postoperative Complications, Interquartile range, mental disorders, Incision and drainage, Medicine, Humans, Hypnotics and Sedatives, Adverse effect, Abscess, Retrospective Studies, British Columbia, business.industry, Incidence, Emergency department, medicine.disease, Surgery, Anesthesia, Procedural sedation and analgesia, Emergency Medicine, Drainage, Female, medicine.symptom, Analgesia, business, Follow-Up Studies

Abstract

Objective:Injection drug users (IDUs) often undergo procedural sedation and analgesia (PSA) in the emergency department (ED). We compared adverse events (AEs) for IDUs to those for non-IDUs receiving PSA for incision and drainage of cutaneous abscesses.Methods:This was a retrospective analysis of a PSA safety audit. IDU status was prospectively documented among consecutive patients undergoing PSA at two urban EDs. Structured data describing comorbidities, vital signs, sedation regimens, and adverse events were collected. Primary outcome was the proportion of patients in each group experiencing an AE, whereas the secondary outcomes included recovery times.Results:Of 525 consecutive patients receiving PSA for incision and drainage of an abscess, 244 were deemed IDUs and 281 non-IDUs. IDUs received higher doses of sedatives and analgesics, and 14 experienced AEs (5.7%), whereas 10 non-IDUs had AEs (3.6%), for a risk difference of 2.1% (95% CI -1.8, 6.5). Median recovery times were 18 minutes (interquartile range [IQR] 10-36) for IDUs and 12 minutes (IQR 7-19) for non-IDUs, for a difference of 6 minutes (95% CI 2-9 minutes). Median sedation times were also longer in IDUs, for a difference of 6 minutes (95% CI 5-10 minutes). Of 20 IDU patients and 1 non-IDU patient admitted to hospital, none had experienced an AE related to PSA.Conclusions:For ED patients requiring PSA for incision and drainage, IDUs had an AE rate similar to that of non-IDUs but longer sedation and recovery times. In experienced hands, PSA may be as safe in IDUs as in patients who do not use injection drugs.

Published

2013

49. Multiplex ligation-dependent probe amplification and fluorescence in situ hybridization are complementary techniques to detect cytogenetic abnormalities in multiple myeloma

Author

Donat, Alpar, Danielle, de Jong, Zsofia, Holczer-Nagy, Bela, Kajtar, Suvi, Savola, Pal, Jakso, Marianna, David, Szabolcs, Kosztolanyi, Laszlo, Kereskai, Laszlo, Pajor, and Karoly, Szuhai

Subjects

Chromosome Aberrations, DNA Copy Number Variations, Chromosomes, Human, Pair 1, Cytogenetic Analysis, Humans, Multiple Myeloma, Multiplex Polymerase Chain Reaction, In Situ Hybridization, Fluorescence

Abstract

Multiple myeloma (MM) is a genetically heterogeneous disease with diverse clinical outcomes. Interphase fluorescence in situ hybridization (i-FISH) is the most commonly used approach to detect recurrent cytogenetic abnormalities in this malignancy. We aimed to assess the performance of multiplex ligation-dependent probe amplification (MLPA) to reveal copy number abnormalities (CNAs) in MM. Diagnostic bone marrow samples from 81 patients were analyzed using 42 MLPA probes for the following regions: 1p32-31, 1p21, 1q21.3, 1q23.3, 5q31.3, 12p13.31, 13q14, 16q12, 16q23, and 17p13. All samples were also screened by i-FISH for the presence of hyperdiploidy, deletion/monosomy of chromosome 13, deletion of TP53, disruption of the immunoglobulin heavy-chain gene, t(4;14), t(11;14), t(14;16), t(8;14), gain of 5q and abnormalities of chromosome 1. A total of 245 alterations were detected in 79 cases (98%). Investigating the same aberrations, the two methods showed a congruency of higher than 90%. A low proportion of cells with the relevant abnormality, focal CNAs and unmatched probes were responsible for the discrepancies. MLPA revealed 95 CNAs not detected by i-FISH providing additional information in 53 cases (65%). Scrutiny of CNAs on chromosome 1, using more than 20 probes, revealed significant heterogeneity in size and location, and variable intra-chromosomal and intra-clonal rates of loss or gain. Our results suggest that MLPA is a reliable high-throughput technique to detect CNAs in MM. Since balanced aberrations are key to prognostic classification of this disease, MLPA and i-FISH should be applied as complementary techniques in diagnostic pathology.

Published

2013

50. Resolving different presynaptic activity patterns within single olfactory glomeruli of Xenopus laevis larvae

Author

Rodi Topci, Mihai Alevra, Erik H. U. Rauf, and Daniëlle de Jong-Bolm

Subjects

Medicine, Science

Abstract

Abstract Olfactory sensing is generally organized into groups of similarly sensing olfactory receptor neurons converging into their corresponding glomerulus, which is thought to behave as a uniform functional unit. It is however unclear to which degree axons within a glomerulus show identical activity, how many converge into a glomerulus, and to answer these questions, how it is possible to visually separate them in live imaging. Here we investigate activity of olfactory receptor neurons and their axon terminals throughout olfactory glomeruli using electrophysiological recordings and rapid 4D calcium imaging. While single olfactory receptor neurons responsive to the same odor stimulus show a diversity of responses in terms of sensitivity and spontaneous firing rate on the level of the somata, their pre-synaptic calcium activity in the glomerulus is homogeneous. In addition, we could not observe the correlated spontaneous calcium activity that is found on the post-synaptic side throughout mitral cell dendrites and has been used in activity correlation imaging. However, it is possible to induce spatio-temporal presynaptic response inhomogeneities by applying trains of olfactory stimuli with varying amino acid concentrations. Automated region-of-interest detection and correlation analysis then visually distinguishes at least two axon subgroups per glomerulus that differ in odor sensitivity.

Published

2021