Your search keyword '"Koster AJ"' showing total 175 results

1. The Weibel-Palade Body Localized SNARE (Soluble NSF Attachment Protein Receptor) Syntaxin-3 Modulates Von Willebrand Factor Secretion From Endothelial Cells

Author

Schillemans, M, Karampini, E, van den Eshof, B, Gangaev, A, Hofman, M, van Breevoort, D, Meems, H, Janssen, H, Mulder, AA, Jost, CR, Escher, JC, Adam, R, Carter, TD, Koster, AJ, van den Biggelaar, M, Voorberg, J, and Bierings, R

Subjects

biological phenomena, cell phenomena, and immunity

Abstract

Objective\ud Endothelial cells store von Willebrand factor (VWF) in rod-shaped secretory organelles, called Weibel-Palade bodies (WPBs). WPB exocytosis is coordinated by a complex network of Rab GTPases, Rab-effectors and SNARE proteins. We have previously identified STXBP1 as the link between the Rab27A-Slp4-a complex on WPBs and the SNARE proteins syntaxin-2 and -3. In this study we investigate the function of syntaxin-3 in VWF secretion. \ud Approach and Results\ud In human umbilical vein endothelial cells (HUVECs) and in blood outgrowth endothelial cells (BOECs) from healthy controls endogenous syntaxin-3 immunolocalized to WPBs. A detailed analysis of BOECs isolated from a patient with variant microvillus inclusion disease (MVID), carrying a homozygous mutation in STX3 (STX3-/-), showed a loss of syntaxin-3 protein and absence of WPB-associated syntaxin-3 immunoreactivity. Ultrastructural analysis revealed no detectable differences in morphology or prevalence of immature or mature WPBs in control versus STX3-/- BOECs. VWF \ud multimer analysis showed normal patterns in plasma of the MVID patient, and media from STX3-/- BOECs, together indicating WPB formation and maturation are unaffected by absence of syntaxin-3. However, a defect in basal as well as Ca2+ - and cAMP-mediated VWF secretion was found in the STX3-/- BOECs. We also show that syntaxin-3 interacts with the WPB-associated SNARE protein VAMP8.\ud Conclusions\ud Our data reveal syntaxin-3 as a novel WPB-associated SNARE protein that controls WPB exocytosis.

Published

2018

2. Weibel-Palade Body Localized Syntaxin-3 Modulates Von Willebrand Factor Secretion From Endothelial Cells

Author

Schillemans, M, Karampini, E, van den Eshof, BL, Gangaev, A, Hofman, M, van Breevoort, D, Meems, H, Janssen, H, Mulder, AA, Jost, CR, Escher, Hankje, Adam, R, Carter, T, Koster, AJ, van den Biggelaar, M, Voorberg, J, Bierings, R, Schillemans, M, Karampini, E, van den Eshof, BL, Gangaev, A, Hofman, M, van Breevoort, D, Meems, H, Janssen, H, Mulder, AA, Jost, CR, Escher, Hankje, Adam, R, Carter, T, Koster, AJ, van den Biggelaar, M, Voorberg, J, and Bierings, R

Published

2018

3. Renal Subcapsular Transplantation of PSC-Derived Kidney Organoids Induces Neo-vasculogenesis and Significant Glomerular and Tubular Maturation In Vivo

Author

van den Berg, CW, Ritsma, L, Avramut, MC, Wiersma, LE, van den Berg, BM, Leuning, DG, Lievers, E, Koning, M, Vanslambrouck, JM, Koster, AJ, Howden, SE, Takasato, M, Little, MH, Rabelink, TJ, van den Berg, CW, Ritsma, L, Avramut, MC, Wiersma, LE, van den Berg, BM, Leuning, DG, Lievers, E, Koning, M, Vanslambrouck, JM, Koster, AJ, Howden, SE, Takasato, M, Little, MH, and Rabelink, TJ

Abstract

Human pluripotent stem cell (hPSC)-derived kidney organoids may facilitate disease modeling and the generation of tissue for renal replacement. Long-term application, however, will require transferability between hPSC lines and significant improvements in organ maturation. A key question is whether time or a patent vasculature is required for ongoing morphogenesis. Here, we show that hPSC-derived kidney organoids, derived in fully defined medium conditions and in the absence of any exogenous vascular endothelial growth factor, develop host-derived vascularization. In vivo imaging of organoids under the kidney capsule confirms functional glomerular perfusion as well as connection to pre-existing vascular networks in the organoids. Wide-field electron microscopy demonstrates that transplantation results in formation of a glomerular basement membrane, fenestrated endothelial cells, and podocyte foot processes. Furthermore, compared with non-transplanted organoids, polarization and segmental specialization of tubular epithelium are observed. These data demonstrate that functional vascularization is required for progressive morphogenesis of human kidney organoids.

Published

2018

4. SAT0015 Anca-associated vasculitis- and systemic lupus erythematosus-induced neutrophil extracellular traps have intrinsically different features

Author

Dam, LS Van, primary, Kraaij, T, additional, Kamerling, SW, additional, Avramut, MC, additional, Jost, CR, additional, Koster, AJ, additional, Scherer, HU, additional, Pusey, CD, additional, Rabelink, AJ, additional, Kooten, C van, additional, and Teng, YK, additional

Published

2017

5. Multiple capsid-stabilizing interactions revealed in a high-resolution structure of an emerging picornavirus causing neonatal sepsis

Author

Shakeel, S, Westerhuis, BM, Domanska, A, Koning, RI, Matadeen, R, Koster, AJ, Bakker, AQ, Beaumont, T, Wolthers, KC, Butcher, SJ, Shakeel, S, Westerhuis, BM, Domanska, A, Koning, RI, Matadeen, R, Koster, AJ, Bakker, AQ, Beaumont, T, Wolthers, KC, and Butcher, SJ

Abstract

The poorly studied picornavirus, human parechovirus 3 (HPeV3) causes neonatal sepsis with no therapies available. Our 4.3-Å resolution structure of HPeV3 on its own and at 15 Å resolution in complex with human monoclonal antibody Fabs demonstrates the expected picornavirus capsid structure with three distinct features. First, 25% of the HPeV3 RNA genome in 60 sites is highly ordered as confirmed by asymmetric reconstruction, and interacts with conserved regions of the capsid proteins VP1 and VP3. Second, the VP0 N terminus stabilizes the capsid inner surface, in contrast to other picornaviruses where on expulsion as VP4, it forms an RNA translocation channel. Last, VP1's hydrophobic pocket, the binding site for the antipicornaviral drug, pleconaril, is blocked and thus inappropriate for antiviral development. Together, these results suggest a direction for development of neutralizing antibodies, antiviral drugs based on targeting the RNA-protein interactions and dissection of virus assembly on the basis of RNA nucleation.

Published

2016

6. Isolation of cyanophage CrV infecting Cylindrospermopsis raciborskii and the influence of temperature and irradiance on CrV proliferation

Author

Steenhauer, LM, primary, Wierenga, J, additional, Carreira, C, additional, Limpens, RWAL, additional, Koster, AJ, additional, Pollard, PC, additional, and Brussaard, CPD, additional

Published

2016

7. Optimisations and Challenges Involved in the Creation of Various Bioluminescent and Fluorescent Influenza A Virus Strains for In Vitro and In Vivo Applications

Author

Spronken, Monique, Short, Kirsty, Herfst, Sander, Bestebroer, Theo, Vaes, Vincent, van der Hoeven, B, Koster, AJ, Kremers, Gert-Jan, Scott, DP, Gultyaev, AP, Sorell, EM, de Graaf, Miranda, Barcena, M, Rimmelzwaan, Guus, Fouchier, Ron, Spronken, Monique, Short, Kirsty, Herfst, Sander, Bestebroer, Theo, Vaes, Vincent, van der Hoeven, B, Koster, AJ, Kremers, Gert-Jan, Scott, DP, Gultyaev, AP, Sorell, EM, de Graaf, Miranda, Barcena, M, Rimmelzwaan, Guus, and Fouchier, Ron

Abstract

Bioluminescent and fluorescent influenza A viruses offer new opportunities to study influenza virus replication, tropism and pathogenesis. To date, several influenza A reporter viruses have been described. These strategies typically focused on a single reporter gene (either bioluminescent or fluorescent) in a single virus backbone. However, whilst bioluminescence is suited to in vivo imaging, fluorescent viruses are more appropriate for microscopy. Therefore, the ideal reporter virus varies depending on the experiment in question, and it is important that any reporter virus strategy can be adapted accordingly. Herein, a strategy was developed to create five different reporter viruses in a single virus backbone. Specifically, enhanced green fluorescent protein (eGFP), far-red fluorescent protein (fRFP), near-infrared fluorescent protein (iRFP), Gaussia luciferase (gLUC) and firefly luciferase (fLUC) were inserted into the PA gene segment of A/PR/8/34 (H1N1). This study provides a comprehensive characterisation of the effects of different reporter genes on influenza virus replication and reporter activity. In vivo reporter gene expression, in lung tissues, was only detected for eGFP, fRFP and gLUC expressing viruses. In vitro, the eGFP-expressing virus displayed the best reporter stability and could be used for correlative light electron microscopy (CLEM). This strategy was then used to create eGFP-expressing viruses consisting entirely of pandemic H1N1, highly pathogenic avian influenza (HPAI) H5N1 and H7N9. The HPAI H5N1 eGFP-expressing virus infected mice and reporter gene expression was

Published

2015

8. Novel Methods for Cryo-Fluorescence Microscopy Permitting Correlative Cryo-Electron Microscopy

Author

Valentijn, JA, primary, Driel, LF van, additional, Agronskaia, AV, additional, Knoops, K, additional, Koning, RI, additional, Barcena, M, additional, Gerritsen, HC, additional, and Koster, AJ, additional

Published

2008

9. On The Structure of Coronaviruses: Cryo-electron Tomography of Mouse Hepatitis Virus

Author

Bárcena, M, primary, Bosch, BJ, additional, Baterlink, W, additional, Oostergetel, GT, additional, Verkleij, A, additional, Rottier, PJM, additional, and Koster, AJ, additional

Published

2008

10. Development of Electron Tomography Methods to Link Cellular Architecture to Function for Cell Biological Applications

Author

Verkleij, AJ, primary, Geerts, WJ C, additional, Barcena-Martin, M, additional, Valentijn, KM, additional, Jansen, KA, additional, Krift, TP van der, additional, Post, JA, additional, Yukashevska, A, additional, Lebbink, MN, additional, Humbel, BH, additional, and Koster, AJ, additional

Published

2006

11. Structural Analysis of Self-assembled Nanotubes of Bacteriophage T4 Capsid Protein gp23 by Cryo Electron Microscopy and Mass Spectrometry

Author

Kaletas, BK, primary, Duijn, E Van, additional, Heck, AJ R, additional, Geels, RB J, additional, Haas, F De, additional, Balen, A van, additional, Vies, SM Van der, additional, Koster, AJ, additional, Hertzberger, LO, additional, and Heeren, RM A, additional

Published

2006

12. Electron Tomography of Corneal Collagen Fibrils

Author

Gilpin, C J, Holmes, DF, Ziese, U, Koster, AJ, and Kadler, KE

Abstract

The ability of cornea to transmit light whilst being mechanically resilient is directly attributable to the formation of an extracellular matrix containing orthogonally arranged sheets of densely packed uniformly-narrow collagen fibrils, in which each sheet contains parallel arrays of fibrils. An understanding of the molecular basis of tissue organisation requires knowledge of the detailed 3-dimensional structure of individual collagen fibrils and how they interact to generate higher order structures. in this study adult bovine corneal collagen fibrils were examined using transmission electron microscopy and automated electron tomography to generate three-dimensional volumes of individual fibrils which had been negatively stained. Tilt series images were collected with an angular increment of 2° over a range of ± 70° using a Philips CM200FEG coupled to a TVIPS automated electron tomography system. A microfibrillar substructure was observed throughout the thickness of the fibril (Figure 1). The microfibrils were ∼4 nm in diameter and were oriented in a right-handed helical twist along the length of fibrils. The microfibrils were observed at an angle of 15° to the long axis of the fibril. As the technique of electron tomography generates a threedimensional volume from the data it was possible, for the first time, to visualise the lateral arrangement of molecules within individual fibrils. There were regions where there was a distinct lateral order and other regions which showed a more fluid-like arrangement. The axial positions of most crystallinity corresponded with the location of the C-telopeptides and N-telopeptides as well as a region close to the d-band in the gap structure of the fibrils. The study also demonstrated that the microfibrils are organised in a quasi-hexagonal packing arrangement

Published

2001

13. Macromolecular Assemblies Designed for Controlled Proteolysis

Author

Walz, J, Koster, AJ, Tamura, T, and Baumeister, W

Abstract

Since cellular structures are rebuilt continually, protein degradation is essential for the maintenance of homeostasis. Misfolded proteins ensuing from genetic defects or environmental stress, are prone to aggregation; chaperones and proteases cooperate in minimizing such unproductive interactions. Last, but not least, protein degradation serves to terminate the lifespan of many regulatory proteins at distinct times and thus features as a key regulatory element itself. Proteins destined for degradation must be recognized and selected within the crowded environment of the cell. The stratagem of self-compartmentalization is key to controlling cellular proteolysis (1).In recent years, a number of multisubunit proteolytic complexes have been described which possess large internal cavities or nano-compartments. This allows them to confine the proteolytic action to their interior; access to these inner compartments is usually restricted to the unfolded proteins. This, in turn, makes it necessary for these proteases to interact - either in a transient or in a permanent manner

Published

1998

14. Ultrastructural characterization of maturing iPSC-derived nephron structures upon transplantation.

Author

Wiersma LE, Avramut MC, Koster AJ, van den Berg CW, and Rabelink TJ

Subjects

Animals, Mice, Cell Differentiation, Nephrons metabolism, Kidney ultrastructure, Induced Pluripotent Stem Cells, Pluripotent Stem Cells

Abstract

Pluripotent stem cell-derived kidney organoids hold great promise as a potential auxiliary transplant tissue for individuals with end-stage renal disease and as a platform for studying kidney diseases and drug discovery. To establish accurate models, it is crucial to thoroughly characterize the morphological features and maturation stages of the cellular components within these organoids. Nephrons, the functional units of the kidney, possess distinct morphological structures that directly correlate with their specific functions. High spatial resolution imaging emerges as a powerful technique for capturing ultrastructural details that may go unnoticed with other methods such as immunofluorescent imaging and scRNA sequencing. In our study, we have applied software capable of seamlessly stitching virtual slides generated from electron microscopy, resulting in high-definition overviews of tissue slides. With this technology, we can comprehensively characterize the development and maturation of kidney organoids when transplanted under the renal capsule of mice. These organoids exhibit advanced ultrastructural developments upon transplantation, including the formation of the filtration barrier in the renal corpuscle, the presence of microvilli in the proximal tubule, and various types of cell sub-segmentation in the connecting tubule similarly to those seen in the adult kidney. Such ultrastructural characterization provides invaluable insights into the structural development and functional morphology of nephron segments within kidney organoids and how to advance them by interventions such as a transplantation. Research Highlights High-resolution imaging is crucial to determine morphological maturation of hiPSC-derived kidney organoids. Upon transplantation, refined ultrastructural development of nephron segments was observed, such as the development of the glomerular filtration barrier., (© 2023 The Authors. Microscopy Research and Technique published by Wiley Periodicals LLC.)

Published

2024

15. CRB1 is required for recycling by RAB11A+ vesicles in human retinal organoids.

Author

Buck TM, Quinn PMJ, Pellissier LP, Mulder AA, Jongejan A, Lu X, Boon N, Koot D, Almushattat H, Arendzen CH, Vos RM, Bradley EJ, Freund C, Mikkers HMM, Boon CJF, Moerland PD, Baas F, Koster AJ, Neefjes J, Berlin I, Jost CR, and Wijnholds J

Subjects

Animals, Humans, Retina metabolism, Mutation, Organoids metabolism, Eye Proteins genetics, Membrane Proteins genetics, Membrane Proteins metabolism, Nerve Tissue Proteins genetics, Nerve Tissue Proteins metabolism, Induced Pluripotent Stem Cells metabolism, Retinal Degeneration genetics, Retinitis Pigmentosa genetics

Abstract

CRB1 gene mutations can cause early- or late-onset retinitis pigmentosa, Leber congenital amaurosis, or maculopathy. Recapitulating human CRB1 phenotypes in animal models has proven challenging, necessitating the development of alternatives. We generated human induced pluripotent stem cell (iPSC)-derived retinal organoids of patients with retinitis pigmentosa caused by biallelic CRB1 mutations and evaluated them against autologous gene-corrected hiPSCs and hiPSCs from healthy individuals. Patient organoids show decreased levels of CRB1 and NOTCH1 expression at the retinal outer limiting membrane. Proximity ligation assays show that human CRB1 and NOTCH1 can interact via their extracellular domains. CRB1 patient organoids feature increased levels of WDFY1+ vesicles, fewer RAB11A+ recycling endosomes, decreased VPS35 retromer complex components, and more degradative endolysosomal compartments relative to isogenic control organoids. Taken together, our data demonstrate that patient-derived retinal organoids enable modeling of retinal degeneration and highlight the importance of CRB1 in early endosome maturation receptor recycling in the retina., Competing Interests: Conflict of interests The authors declare no competing interests. The LUMC is holder of patent number PCT/NL2014/050549, which describes the potential clinical use of CRB2; J.W. and L.P.P. are listed as co-inventor of this patent, and J.W. is an employee of the LUMC., (Copyright © 2023 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2023

16. A cryogenic, coincident fluorescence, electron, and ion beam microscope.

Author

Boltje DB, Hoogenboom JP, Jakobi AJ, Jensen GJ, Jonker CTH, Kaag MJ, Koster AJ, Last MGF, de Agrela Pinto C, Plitzko JM, Raunser S, Tacke S, Wang Z, van der Wee EB, Wepf R, and den Hoedt S

Subjects

Cryoelectron Microscopy methods, Microscopy, Fluorescence, Ions, Electrons, Electron Microscope Tomography methods

Abstract

Cryogenic electron tomography (cryo-ET) combined with subtomogram averaging, allows in situ visualization and structure determination of macromolecular complexes at subnanometre resolution. Cryogenic focused ion beam (cryo-FIB) micromachining is used to prepare a thin lamella-shaped sample out of a frozen-hydrated cell for cryo-ET imaging, but standard cryo-FIB fabrication is blind to the precise location of the structure or proteins of interest. Fluorescence-guided focused ion beam (FIB) milling at target locations requires multiple sample transfers prone to contamination, and relocation and registration accuracy is often insufficient for 3D targeting. Here, we present in situ fluorescence microscopy-guided FIB fabrication of a frozen-hydrated lamella to address this problem: we built a coincident three-beam cryogenic correlative microscope by retrofitting a compact cryogenic microcooler, custom positioning stage, and an inverted widefield fluorescence microscope (FM) on an existing FIB scanning electron microscope. We show FM controlled targeting at every milling step in the lamella fabrication process, validated with transmission electron microscope tomogram reconstructions of the target regions. The ability to check the lamella during and after the milling process results in a higher success rate in the fabrication process and will increase the throughput of fabrication for lamellae suitable for high-resolution imaging., Competing Interests: DB is an employee of Delmic B.V, JH, Sd has a financial interest in Delmic B.V, AJ, GJ, MK, AK, Cd, JP, SR, ST, ZW, Ev, RW No competing interests declared, CJ, ML were employees of Delmic B.V, (© 2022, Boltje et al.)

Published

2022

17. Author Correction: Correlative cryo super-resolution light and electron microscopy on mammalian cells using fluorescent proteins.

Author

Tuijtel MW, Koster AJ, Jakobs S, Faas FGA, and Sharp TH

Published

2022

18. Automated vitrification of cryo-EM samples with controllable sample thickness using suction and real-time optical inspection.

Author

Koning RI, Vader H, van Nugteren M, Grocutt PA, Yang W, Renault LLR, Koster AJ, Kamp ACF, and Schwertner M

Subjects

Cryoelectron Microscopy methods, Humans, Proteins, Suction, Electron Microscope Tomography, Vitrification

Abstract

The speed and efficiency of data collection and image processing in cryo-electron microscopy have increased over the last decade. However, cryo specimen preparation techniques have lagged and faster, more reproducible specimen preparation devices are needed. Here, we present a vitrification device with highly automated sample handling, requiring only limited user interaction. Moreover, the device allows inspection of thin films using light microscopy, since the excess liquid is removed through suction by tubes, not blotting paper. In combination with dew-point control, this enables thin film preparation in a controlled and reproducible manner. The advantage is that the quality of the prepared cryo specimen is characterized before electron microscopy data acquisition. The practicality and performance of the device are illustrated with experimental results obtained by vitrification of protein suspensions, lipid vesicles, bacterial and human cells, followed by imaged using single particle analysis, cryo-electron tomography, and cryo correlated light and electron microscopy., (© 2022. The Author(s).)

Published

2022

19. AreTomo: An integrated software package for automated marker-free, motion-corrected cryo-electron tomographic alignment and reconstruction.

Author

Zheng S, Wolff G, Greenan G, Chen Z, Faas FGA, Bárcena M, Koster AJ, Cheng Y, and Agard DA

Abstract

AreTomo, an abbreviation for Alignment and Reconstruction for Electron Tomography, is a GPU accelerated software package that fully automates motion-corrected marker-free tomographic alignment and reconstruction in a single package. By correcting in-plane rotation, translation, and importantly, the local motion resulting from beam-induced motion from tilt to tilt, AreTomo can produce tomograms with sufficient accuracy to be directly used for subtomogram averaging. Another major application is the on-the-fly reconstruction of tomograms in parallel with tilt series collection to provide users with real-time feedback of sample quality allowing users to make any necessary adjustments of collection parameters. Here, the multiple alignment algorithms implemented in AreTomo are described and the local motions measured on a typical tilt series are analyzed. The residual local motion after correction for global motion was found in the range of ± 80 Å, indicating that the accurate correction of local motion is critical for high-resolution cryo-electron tomography (cryoET)., Competing Interests: The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (© 2022 The Author(s).)

Published

2022

20. Doublecortin-like expressing astrocytes of the suprachiasmatic nucleus are implicated in the biosynthesis of vasopressin and influences circadian rhythms.

Author

Coomans C, Saaltink DJ, Deboer T, Tersteeg M, Lanooij S, Schneider AF, Mulder A, van Minnen J, Jost C, Koster AJ, and Vreugdenhil E

Subjects

Animals, Doublecortin Domain Proteins, Doublecortin-Like Kinases, Mice, Suprachiasmatic Nucleus metabolism, Vasopressins metabolism, Astrocytes metabolism, Circadian Rhythm physiology

Abstract

We have recently identified a novel plasticity protein, doublecortin-like (DCL), that is specifically expressed in the shell of the mouse suprachiasmatic nucleus (SCN). DCL is implicated in neuroplastic events, such as neurogenesis, that require structural rearrangements of the microtubule cytoskeleton, enabling dynamic movements of cell bodies and dendrites. We have inspected DCL expression in the SCN by confocal microscopy and found that DCL is expressed in GABA transporter-3 (GAT3)-positive astrocytes that envelope arginine vasopressin (AVP)-expressing cells. To investigate the role of these DCL-positive astrocytes in circadian rhythmicity, we have used transgenic mice expressing doxycycline-induced short-hairpin (sh) RNA's targeting DCL mRNA (DCL knockdown mice). Compared with littermate wild type (WT) controls, DCL-knockdown mice exhibit significant shorter circadian rest-activity periods in constant darkness and adjusted significantly faster to a jet-lag protocol. As DCL-positive astrocytes are closely associated with AVP-positive cells, we analyzed AVP expression in DCL-knockdown mice and in their WT littermates by 3D reconstructions and transmission electron microscopy (TEM). We found significantly higher numbers of AVP-positive cells with increased volume and more intensity in DCL-knockdown mice. We found alterations in the numbers of dense core vesicle-containing neurons at ZT8 and ZT20 suggesting that the peak and trough of neuropeptide biosynthesis is dampened in DCL-knockdown mice compared to WT littermates. Together, our data suggest an important role for the astrocytic plasticity in the regulation of circadian rhythms and point to the existence of a specific DCL + astrocyte-AVP + neuronal network located in the dorsal SCN implicated in AVP biosynthesis., (© 2021 The Authors. GLIA published by Wiley Periodicals LLC.)

Published

2021

21. Distinct antigen uptake receptors route to the same storage compartments for cross-presentation in dendritic cells.

Author

Ho NI, Camps MG, Garcia-Vallejo JJ, Bos E, Koster AJ, Verdoes M, van Kooyk Y, and Ossendorp F

Subjects

Animals, Antigen Presentation, Antigens immunology, Cathepsins metabolism, Dendritic Cells metabolism, Dendritic Cells ultrastructure, Endosomes immunology, Endosomes metabolism, Endosomes ultrastructure, Histocompatibility Antigens Class I metabolism, Histocompatibility Antigens Class II metabolism, Lysosomes immunology, Lysosomes metabolism, Lysosomes ultrastructure, Mice, Microscopy, Electron, Transmission, Models, Animal, NIH 3T3 Cells, Primary Cell Culture, Antigens metabolism, Cross-Priming, Dendritic Cells immunology, Lectins, C-Type metabolism, Receptors, IgG metabolism

Abstract

An exclusive feature of dendritic cells (DCs) is their capacity to present exogenous antigens by MHC class I molecules, called cross-presentation. Here, we show that protein antigen can be conserved in mature murine DCs for several days in a lysosome-like storage compartment, distinct from MHC class II and early endosomal compartments, as an internal source for the supply of MHC class I ligands. Using two different uptake routes via Fcγ receptors and C-type lectin receptors, we could show that antigens were routed towards the same endolysosomal compartments after 48 h. The antigen-containing compartments lacked co-expression of molecules involved in MHC class I processing and presentation including TAP and proteasome subunits as shown by single-cell imaging flow cytometry. Moreover, we observed the absence of cathepsin S but selective co-localization of active cathepsin X with protein antigen in the storage compartments. This indicates cathepsin S-independent antigen degradation and a novel but yet undefined role for cathepsin X in antigen processing and cross-presentation by DCs. In summary, our data suggest that these antigen-containing compartments in DCs can conserve protein antigens from different uptake routes and contribute to long-lasting antigen cross-presentation., (© 2021 The Authors. Immunology published by John Wiley & Sons Ltd.)

Published

2021

22. The adapter protein Myd88 plays an important role in limiting mycobacterial growth in a zebrafish model for tuberculosis.

Author

Hosseini R, Lamers GEM, Bos E, Hogendoorn PCW, Koster AJ, Meijer AH, Spaink HP, and Schaaf MJM

Subjects

Animals, Animals, Genetically Modified, Bacterial Load, Disease Models, Animal, Granuloma genetics, Granuloma metabolism, Granuloma pathology, Hydrogen-Ion Concentration, Leukocytes metabolism, Leukocytes microbiology, Leukocytes ultrastructure, Lysosomes metabolism, Lysosomes microbiology, Lysosomes ultrastructure, Microscopy, Electron, Transmission, Mycobacterium Infections, Nontuberculous genetics, Mycobacterium Infections, Nontuberculous metabolism, Mycobacterium Infections, Nontuberculous pathology, Mycobacterium marinum ultrastructure, Myeloid Differentiation Factor 88 genetics, Signal Transduction, Tuberculosis genetics, Tuberculosis metabolism, Tuberculosis pathology, Zebrafish embryology, Zebrafish genetics, Zebrafish metabolism, Zebrafish Proteins genetics, Granuloma microbiology, Mycobacterium Infections, Nontuberculous microbiology, Mycobacterium marinum growth & development, Myeloid Differentiation Factor 88 metabolism, Tuberculosis microbiology, Zebrafish microbiology, Zebrafish Proteins metabolism

Abstract

Tuberculosis (TB) is the most prevalent bacterial infectious disease in the world, caused by the pathogen Mycobacterium tuberculosis (Mtb). In this study, we have used Mycobacterium marinum (Mm) infection in zebrafish larvae as an animal model for this disease to study the role of the myeloid differentiation factor 88 (Myd88), the key adapter protein of Toll-like receptors. Previously, Myd88 has been shown to enhance innate immune responses against bacterial infections, and in the present study, we have investigated the effect of Myd88 deficiency on the granuloma morphology and the intracellular distribution of bacteria during Mm infection. Our results show that granulomas formed in the tail fin from myd88 mutant larvae have a more compact structure and contain a reduced number of leukocytes compared to the granulomas observed in wild-type larvae. These morphological differences were associated with an increased bacterial burden in the myd88 mutant. Electron microscopy analysis showed that the majority of Mm in the myd88 mutant are located extracellularly, whereas in the wild type, most bacteria were intracellular. In the myd88 mutant, intracellular bacteria were mainly present in compartments that were not electron-dense, suggesting that these compartments had not undergone fusion with a lysosome. In contrast, approximately half of the intracellular bacteria in wild-type larvae were found in electron-dense compartments. These observations in a zebrafish model for tuberculosis suggest a role for Myd88-dependent signalling in two important phenomena that limit mycobacterial growth in the infected tissue. It reduces the number of leukocytes at the site of infection and the acidification of bacteria-containing compartments inside these cells., (© 2021. The Author(s).)

Published

2021

23. Defining Phenotype, Tropism, and Retinal Gene Therapy Using Adeno-Associated Viral Vectors (AAVs) in New-Born Brown Norway Rats with a Spontaneous Mutation in Crb1 .

Author

Boon N, Alves CH, Mulder AA, Andriessen CA, Buck TM, Quinn PMJ, Vos RM, Koster AJ, Jost CR, and Wijnholds J

Subjects

Animals, Animals, Newborn, Calcium-Binding Proteins metabolism, Carrier Proteins genetics, Dependovirus genetics, Ependymoglial Cells metabolism, Eye Proteins genetics, Genetic Vectors administration & dosage, Genetic Vectors pharmacology, Intravitreal Injections, Membrane Proteins genetics, Mutation, Nerve Tissue Proteins metabolism, Phenotype, Rats, Rats, Mutant Strains, Retina physiopathology, Retinal Dystrophies etiology, Retinal Dystrophies therapy, Retinal Pigment Epithelium metabolism, Viral Tropism, Calcium-Binding Proteins genetics, Dependovirus physiology, Genetic Therapy methods, Nerve Tissue Proteins genetics, Retinal Dystrophies genetics

Abstract

Mutations in the Crumbs homologue 1 ( CRB1 ) gene cause inherited retinal dystrophies, such as early-onset retinitis pigmentosa and Leber congenital amaurosis. A Brown Norway rat strain was reported with a spontaneous insertion-deletion (indel) mutation in exon 6 of Crb1 . It has been reported that these Crb1 mutant rats show vascular abnormalities associated with retinal telangiectasia and possess an early-onset retinal degenerative phenotype with outer limiting membrane breaks and focal loss of retinal lamination at 2 months of age. Here, we further characterized the morphological phenotype of new-born and adult Crb1 mutant rats in comparison with age-matched Brown Norway rats without a mutation in Crb1 . A significantly decreased retinal function and visual acuity was observed in Crb1 mutant rats at 1 and 3 months of age, respectively. Moreover, in control rats, the subcellular localization of canonical CRB1 was observed at the subapical region in Müller glial cells while CRB2 was observed at the subapical region in both photoreceptors and Müller glial cells by immuno-electron microscopy. CRB1 localization was lost in the Crb1 mutant rats, whereas CRB2 was still observed. In addition, we determined the tropism of subretinal or intravitreally administered AAV5-, AAV9- or AAV6-variant ShH10 Y445F vectors in new-born control and Crb1 mutant rat retinas. We showed that subretinal injection of AAV5 and AAV9 at postnatal days 5 (P5) or 8 (P8) predominantly infected the retinal pigment epithelium (RPE) and photoreceptor cells; while intravitreal injection of ShH10 Y445F at P5 or P8 resulted in efficient infection of mainly Müller glial cells. Using knowledge of the subcellular localization of CRB1 and the ability of ShH10 Y445F to infect Müller glial cells, canonical h CRB1 and h CRB2 AAV-mediated gene therapy were explored in new-born Crb1 mutant rats. Enhanced retinal function after gene therapy delivery in the Crb1 rat was not observed. No timely rescue of the retinal phenotype was observed using retinal function and visual acuity, suggesting the need for earlier onset of expression of recombinant hCRB proteins in Müller glial cells to rescue the severe retinal phenotype in Crb1 mutant rats.

Published

2021

24. Application of a Highly Selective Cathepsin S Two-step Activity-Based Probe in Multicolor Bio-Orthogonal Correlative Light-Electron Microscopy.

Author

van Dalen FJ, Bakkum T, van Leeuwen T, Groenewold M, Deu E, Koster AJ, van Kasteren SI, and Verdoes M

Abstract

Cathepsin S is a lysosomal cysteine protease highly expressed in immune cells such as dendritic cells, B cells and macrophages. Its functions include extracellular matrix breakdown and cleavage of cell adhesion molecules to facilitate immune cell motility, as well as cleavage of the invariant chain during maturation of major histocompatibility complex II. The identification of these diverse specific functions has brought the challenge of delineating cathepsin S activity with great spatial precision, relative to related enzymes and substrates. Here, the development of a potent and highly selective two-step activity-based probe for cathepsin S and the application in multicolor bio-orthogonal correlative light-electron microscopy is presented. LHVS, which has been reported as a selective inhibitor of cathepsin S with nanomolar potency, formed the basis for our probe design. However, in competitive activity-based protein profiling experiments LHVS showed significant cross-reactivity toward Cat L. Introduction of an azide group in the P2 position expanded the selectivity window for cathepsin S, but rendered the probe undetectable, as demonstrated in bio-orthogonal competitive activity-based protein profiling. Incorporation of an additional azide handle for click chemistry on the solvent-exposed P1 position allowed for selective labeling of cathepsin S. This highlights the influence of click handle positioning on probe efficacy. This probe was utilized in multicolor bio-orthogonal confocal and correlative light-electron microscopy to investigate the localization of cathepsin S activity at an ultrastructural level in bone marrow-derived dendritic cells. The tools developed in this study will aid the characterization of the variety of functions of cathepsin S throughout biology., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2021 van Dalen, Bakkum, van Leeuwen, Groenewold, Deu, Koster, van Kasteren and Verdoes.)

Published

2021

25. Super-resolution correlative light-electron microscopy using a click-chemistry approach for studying intracellular trafficking.

Author

Andrian T, Bakkum T, van Elsland DM, Bos E, Koster AJ, Albertazzi L, van Kasteren SI, and Pujals S

Subjects

Microscopy, Electron, Microscopy, Electron, Transmission, Microscopy, Fluorescence, Staining and Labeling, Single Molecule Imaging

Abstract

Correlative light and electron microscopy (CLEM) entails a group of multimodal imaging techniques that are combined to pinpoint to the location of fluorescently labeled molecules in the context of their ultrastructural cellular environment. Here we describe a detailed workflow for STORM-CLEM, in which STochastic Optical Reconstruction Microscopy (STORM), an optical super-resolution technique, is correlated with transmission electron microscopy (TEM). This protocol has the advantage that both imaging modalities have resolution at the nanoscale, bringing higher synergies on the information obtained. The sample is prepared according to the Tokuyasu method followed by click-chemistry labeling and STORM imaging. Then, after heavy metal staining, electron microscopy imaging is performed followed by correlation of the two images. The case study presented here is on intracellular pathogens, but the protocol is versatile and could potentially be applied to many types of samples., (Copyright © 2021 Elsevier Inc. All rights reserved.)

Published

2021

26. Bioorthogonal Correlative Light-Electron Microscopy of Mycobacterium tuberculosis in Macrophages Reveals the Effect of Antituberculosis Drugs on Subcellular Bacterial Distribution.

Author

Bakkum T, Heemskerk MT, Bos E, Groenewold M, Oikonomeas-Koppasis N, Walburg KV, van Veen S, van der Lienden MJC, van Leeuwen T, Haks MC, Ottenhoff THM, Koster AJ, and van Kasteren SI

Abstract

Bioorthogonal correlative light-electron microscopy (B-CLEM) can give a detailed overview of multicomponent biological systems. It can provide information on the ultrastructural context of bioorthogonal handles and other fluorescent signals, as well as information about subcellular organization. We have here applied B-CLEM to the study of the intracellular pathogen Mycobacterium tuberculosis ( Mtb ) by generating a triply labeled Mtb through combined metabolic labeling of the cell wall and the proteome of a DsRed-expressing Mtb strain. Study of this pathogen in a B-CLEM setting was used to provide information about the intracellular distribution of the pathogen, as well as its in situ response to various clinical antibiotics, supported by flow cytometric analysis of the bacteria, after recovery from the host cell ( ex cellula ). The RNA polymerase-targeting drug rifampicin displayed the most prominent effect on subcellular distribution, suggesting the most direct effect on pathogenicity and/or viability, while the cell wall synthesis-targeting drugs isoniazid and ethambutol effectively rescued bacterial division-induced loss of metabolic labels. The three drugs combined did not give a more pronounced effect but rather an intermediate response, whereas gentamicin displayed a surprisingly strong additive effect on subcellular distribution., Competing Interests: The authors declare the following competing financial interest(s): The abstract figure was designed by bergdesigns.nl., (© 2020 American Chemical Society.)

Published

2020

27. A molecular pore spans the double membrane of the coronavirus replication organelle.

Author

Wolff G, Limpens RWAL, Zevenhoven-Dobbe JC, Laugks U, Zheng S, de Jong AWM, Koning RI, Agard DA, Grünewald K, Koster AJ, Snijder EJ, and Bárcena M

Subjects

Animals, Cryoelectron Microscopy, Cytoplasmic Vesicles ultrastructure, Cytoplasmic Vesicles virology, Electron Microscope Tomography, Intracellular Membranes ultrastructure, Intracellular Membranes virology, Mice, Viral Nonstructural Proteins chemistry, Cytoplasmic Vesicles chemistry, Intracellular Membranes chemistry, Murine hepatitis virus physiology, RNA, Viral biosynthesis, Virus Replication

Abstract

Coronavirus genome replication is associated with virus-induced cytosolic double-membrane vesicles, which may provide a tailored microenvironment for viral RNA synthesis in the infected cell. However, it is unclear how newly synthesized genomes and messenger RNAs can travel from these sealed replication compartments to the cytosol to ensure their translation and the assembly of progeny virions. In this study, we used cellular cryo-electron microscopy to visualize a molecular pore complex that spans both membranes of the double-membrane vesicle and would allow export of RNA to the cytosol. A hexameric assembly of a large viral transmembrane protein was found to form the core of the crown-shaped complex. This coronavirus-specific structure likely plays a key role in coronavirus replication and thus constitutes a potential drug target., (Copyright © 2020 The Authors, some rights reserved; exclusive licensee American Association for the Advancement of Science. No claim to original U.S. Government Works.)

Published

2020

28. A unifying structural and functional model of the coronavirus replication organelle: Tracking down RNA synthesis.

Author

Snijder EJ, Limpens RWAL, de Wilde AH, de Jong AWM, Zevenhoven-Dobbe JC, Maier HJ, Faas FFGA, Koster AJ, and Bárcena M

Subjects

Animals, Betacoronavirus genetics, Betacoronavirus physiology, COVID-19, Cell Line, Chlorocebus aethiops, Electron Microscope Tomography, Endoplasmic Reticulum ultrastructure, Humans, Middle East Respiratory Syndrome Coronavirus physiology, Pandemics, Pneumonia, Viral pathology, Pneumonia, Viral virology, RNA, Viral metabolism, SARS-CoV-2, Vero Cells, Coronavirus classification, Coronavirus physiology, Coronavirus Infections pathology, Coronavirus Infections virology, Endoplasmic Reticulum pathology, Endoplasmic Reticulum virology, Virus Replication

Abstract

Zoonotic coronavirus (CoV) infections, such as those responsible for the current severe acute respiratory syndrome-CoV 2 (SARS-CoV-2) pandemic, cause grave international public health concern. In infected cells, the CoV RNA-synthesizing machinery associates with modified endoplasmic reticulum membranes that are transformed into the viral replication organelle (RO). Although double-membrane vesicles (DMVs) appear to be a pan-CoV RO element, studies to date describe an assortment of additional CoV-induced membrane structures. Despite much speculation, it remains unclear which RO element(s) accommodate viral RNA synthesis. Here we provide detailed 2D and 3D analyses of CoV ROs and show that diverse CoVs essentially induce the same membrane modifications, including the small open double-membrane spherules (DMSs) previously thought to be restricted to gamma- and delta-CoV infections and proposed as sites of replication. Metabolic labeling of newly synthesized viral RNA followed by quantitative electron microscopy (EM) autoradiography revealed abundant viral RNA synthesis associated with DMVs in cells infected with the beta-CoVs Middle East respiratory syndrome-CoV (MERS-CoV) and SARS-CoV and the gamma-CoV infectious bronchitis virus. RNA synthesis could not be linked to DMSs or any other cellular or virus-induced structure. Our results provide a unifying model of the CoV RO and clearly establish DMVs as the central hub for viral RNA synthesis and a potential drug target in CoV infection., Competing Interests: The authors have declared that no competing interests exist.

Published

2020

29. Human-iPSC-Derived Cardiac Stromal Cells Enhance Maturation in 3D Cardiac Microtissues and Reveal Non-cardiomyocyte Contributions to Heart Disease.

Author

Giacomelli E, Meraviglia V, Campostrini G, Cochrane A, Cao X, van Helden RWJ, Krotenberg Garcia A, Mircea M, Kostidis S, Davis RP, van Meer BJ, Jost CR, Koster AJ, Mei H, Míguez DG, Mulder AA, Ledesma-Terrón M, Pompilio G, Sala L, Salvatori DCF, Slieker RC, Sommariva E, de Vries AAF, Giera M, Semrau S, Tertoolen LGJ, Orlova VV, Bellin M, and Mummery CL

Subjects

Cell Differentiation, Endothelial Cells, Humans, Myocytes, Cardiac, Stromal Cells, Heart Diseases, Induced Pluripotent Stem Cells

Abstract

Cardiomyocytes (CMs) from human induced pluripotent stem cells (hiPSCs) are functionally immature, but this is improved by incorporation into engineered tissues or forced contraction. Here, we showed that tri-cellular combinations of hiPSC-derived CMs, cardiac fibroblasts (CFs), and cardiac endothelial cells also enhance maturation in easily constructed, scaffold-free, three-dimensional microtissues (MTs). hiPSC-CMs in MTs with CFs showed improved sarcomeric structures with T-tubules, enhanced contractility, and mitochondrial respiration and were electrophysiologically more mature than MTs without CFs. Interactions mediating maturation included coupling between hiPSC-CMs and CFs through connexin 43 (CX43) gap junctions and increased intracellular cyclic AMP (cAMP). Scaled production of thousands of hiPSC-MTs was highly reproducible across lines and differentiated cell batches. MTs containing healthy-control hiPSC-CMs but hiPSC-CFs from patients with arrhythmogenic cardiomyopathy strikingly recapitulated features of the disease. Our MT model is thus a simple and versatile platform for modeling multicellular cardiac diseases that will facilitate industry and academic engagement in high-throughput molecular screening., Competing Interests: Declaration of Interests C.L.M. is co-founder of Ncardia bv., (Copyright © 2020 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2020

30. Progression and Classification of Granular Osmiophilic Material (GOM) Deposits in Functionally Characterized Human NOTCH3 Transgenic Mice.

Author

Gravesteijn G, Munting LP, Overzier M, Mulder AA, Hegeman I, Derieppe M, Koster AJ, van Duinen SG, Meijer OC, Aartsma-Rus A, van der Weerd L, Jost CR, van den Maagdenberg AMJM, Rutten JW, and Lesnik Oberstein SAJ

Subjects

Animals, Brain physiopathology, Brain ultrastructure, Cerebrovascular Circulation, Humans, Mice, Inbred C57BL, Mice, Transgenic, Brain blood supply, Brain pathology, CADASIL genetics, CADASIL pathology, Receptor, Notch3 genetics

Abstract

CADASIL is a NOTCH3-associated cerebral small vessel disease. A pathological ultrastructural disease hallmark is the presence of NOTCH3-protein containing deposits called granular osmiophilic material (GOM), in small arteries. How these GOM deposits develop over time and what their role is in disease progression is largely unknown. Here, we studied the progression of GOM deposits in humanized transgenic NOTCH3 Arg182Cys mice, compared them to GOM deposits in patient material, and determined whether GOM deposits in mice are associated with a functional CADASIL phenotype. We found that GOM deposits are not static, but rather progress in ageing mice, both in terms of size and aspect. We devised a GOM classification system, reflecting size, morphology and electron density. Six-month-old mice showed mostly early stage GOM, whereas older mice and patient vessels showed predominantly advanced stage GOM, but also early stage GOM. Mutant mice did not develop the most severe GOM stage seen in patient material. This absence of end-stage GOM in mice was associated with an overall lack of histological vascular pathology, which may explain why the mice did not reveal functional deficits in cerebral blood flow, cognition and motor function. Taken together, our data indicate that GOM progress over time, and that new GOM deposits are continuously being formed. The GOM staging system we introduce here allows for uniform GOM deposit classification in future mouse and human studies, which may lead to more insight into a potential association between GOM stage and CADASIL disease severity, and the role of GOM in disease progression.

Published

2020

31. Mind the gap: Micro-expansion joints drastically decrease the bending of FIB-milled cryo-lamellae.

Author

Wolff G, Limpens RWAL, Zheng S, Snijder EJ, Agard DA, Koster AJ, and Bárcena M

Subjects

Animals, Electron Microscope Tomography methods, Equipment Design, Frozen Sections instrumentation, Mice, Workflow, Electron Microscope Tomography instrumentation, Frozen Sections methods

Abstract

Cryo-focused ion beam (FIB)-milling of biological samples can be used to generate thin electron-transparent slices from cells grown or deposited on EM grids. These so called cryo-lamellae allow high-resolution structural studies of the natural cellular environment by in situ cryo-electron tomography. However, the cryo-lamella workflow is a low-throughput technique and can easily be hindered by technical issues like the bending of the lamellae during the final cryo-FIB-milling steps. The severity of lamella bending seems to correlate with crinkling of the EM grid support film at cryogenic temperatures, which could generate tensions that may be transferred onto the thin lamella, leading to its bending and breakage. To protect the lamellae from such forces, we milled "micro-expansion joints" alongside the lamellae, creating gaps in the support that can act as physical buffers to safely absorb material motion. We demonstrate that the presence of micro-expansion joints drastically decreases bending of lamellae milled from eukaryotic cells grown and frozen on EM grids. Furthermore, we show that this adaptation does not create additional instabilities that could impede subsequent parts of the cryo-lamella workflow, as we obtained high-quality Volta phase plate tomograms revealing macromolecules in their natural structural context. The minimal additional effort required to implement micro-expansion joints in the cryo-FIB-milling workflow makes them a straightforward solution against cryo-lamella bending to increase the throughput of in situ structural biology studies., (Copyright © 2019 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2019

32. Glomerular permeability is not affected by heparan sulfate glycosaminoglycan deficiency in zebrafish embryos.

Author

Khalil R, Lalai RA, Wiweger MI, Avramut CM, Koster AJ, Spaink HP, Bruijn JA, Hogendoorn PCW, and Baelde HJ

Subjects

Animals, Gene Expression Regulation, Heparitin Sulfate metabolism, Mutation, N-Acetylglucosaminyltransferases genetics, N-Acetylglucosaminyltransferases metabolism, Zebrafish, Zebrafish Proteins genetics, Zebrafish Proteins metabolism, Embryo, Nonmammalian physiology, Heparitin Sulfate deficiency, Kidney Glomerulus physiology

Abstract

Proteinuria develops when specific components in the glomerular filtration barrier have impaired function. Although the precise components involved in maintaining this barrier have not been fully identified, heparan sulfate proteoglycans are believed to play an essential role in maintaining glomerular filtration. Although in situ studies have shown that a loss of heparan sulfate glycosaminoglycans increases the permeability of the glomerular filtration barrier, recent studies using experimental models have shown that podocyte-specific deletion of heparan sulfate glycosaminoglycan assembly does not lead to proteinuria. However, tubular reabsorption of leaked proteins might have masked an increase in glomerular permeability in these models. Furthermore, not only podocytes but also glomerular endothelial cells are involved in heparan sulfate synthesis in the glomerular filtration barrier. Therefore, we investigated the effect of a global heparan sulfate glycosaminoglycan deficiency on glomerular permeability. We used a zebrafish embryo model carrying a homozygous germline mutation in the ext2 gene. Glomerular permeability was assessed with a quantitative dextran tracer injection method. In this model, we accounted for tubular reabsorption. Loss of anionic sites in the glomerular basement membrane was measured using polyethyleneimine staining. Although mutant animals had significantly fewer negatively charged areas in the glomerular basement membrane, glomerular permeability was unaffected. Moreover, heparan sulfate glycosaminoglycan-deficient embryos had morphologically intact podocyte foot processes. Glomerular filtration remains fully functional despite a global reduction of heparan sulfate.

Published

2019

33. CRB2 Loss in Rod Photoreceptors Is Associated with Progressive Loss of Retinal Contrast Sensitivity.

Author

Alves CH, Boon N, Mulder AA, Koster AJ, Jost CR, and Wijnholds J

Subjects

Animals, Contrast Sensitivity genetics, Disease Models, Animal, Electroretinography, Immunohistochemistry, Leber Congenital Amaurosis pathology, Membrane Proteins genetics, Mice, Mice, Inbred C57BL, Mice, Knockout, Microscopy, Electron, Transmission, Retinal Degeneration metabolism, Retinal Degeneration pathology, Retinitis Pigmentosa metabolism, Retinitis Pigmentosa pathology, Contrast Sensitivity physiology, Leber Congenital Amaurosis metabolism, Membrane Proteins metabolism, Retina metabolism, Retina pathology, Retinal Rod Photoreceptor Cells metabolism

Abstract

Variations in the Crumbs homolog-1 ( CRB1 ) gene are associated with a wide variety of autosomal recessive retinal dystrophies, including early onset retinitis pigmentosa (RP) and Leber congenital amaurosis (LCA). CRB1 belongs to the Crumbs family, which in mammals includes CRB2 and CRB3. Here, we studied the specific roles of CRB2 in rod photoreceptor cells and whether ablation of CRB2 in rods exacerbates the Crb1 -disease. Therefore, we assessed the morphological, retinal, and visual functional consequences of specific ablation of CRB2 from rods with or without concomitant loss of CRB1. Our data demonstrated that loss of CRB2 in mature rods resulted in RP. The retina showed gliosis and disruption of the subapical region and adherens junctions at the outer limiting membrane. Rods were lost at the peripheral and central superior retina, while gross retinal lamination was preserved. Rod function as measured by electroretinography was impaired in adult mice. Additional loss of CRB1 exacerbated the retinal phenotype leading to an early reduction of the dark-adapted rod photoreceptor a-wave and reduced contrast sensitivity from 3-months-of-age, as measured by optokinetic tracking reflex (OKT) behavior testing. The data suggest that CRB2 present in rods is required to prevent photoreceptor degeneration and vision loss.

Published

2019

34. Insights into IgM-mediated complement activation based on in situ structures of IgM-C1-C4b.

Author

Sharp TH, Boyle AL, Diebolder CA, Kros A, Koster AJ, and Gros P

Subjects

Antibodies immunology, Antigens immunology, Binding Sites immunology, Humans, Models, Molecular, Complement Activation immunology, Complement C1 immunology, Complement C4 immunology, Immunoglobulin M immunology

Abstract

Antigen binding by serum Ig-M (IgM) protects against microbial infections and helps to prevent autoimmunity, but causes life-threatening diseases when mistargeted. How antigen-bound IgM activates complement-immune responses remains unclear. We present cryoelectron tomography structures of IgM, C1, and C4b complexes formed on antigen-bearing lipid membranes by normal human serum at 4 °C. The IgM-C1-C4b complexes revealed C4b product release as the temperature-limiting step in complement activation. Both IgM hexamers and pentamers adopted hexagonal, dome-shaped structures with Fab pairs, dimerized by hinge domains, bound to surface antigens that support a platform of Fc regions. C1 binds IgM through widely spread C1q-collagen helices, with C1r proteases pointing outward and C1s bending downward and interacting with surface-attached C4b, which further interacts with the adjacent IgM-Fab 2 and globular C1q-recognition unit. Based on these data, we present mechanistic models for antibody-mediated, C1q-transmitted activation of C1 and for C4b deposition, while further conformational rearrangements are required to form C3 convertases., Competing Interests: The authors declare no conflict of interest., (Copyright © 2019 the Author(s). Published by PNAS.)

Published

2019

35. Origins of Enterovirus Replication Organelles Established by Whole-Cell Electron Microscopy.

Author

Melia CE, Peddie CJ, de Jong AWM, Snijder EJ, Collinson LM, Koster AJ, van der Schaar HM, van Kuppeveld FJM, and Bárcena M

Subjects

Animals, Chlorocebus aethiops, Endoplasmic Reticulum virology, Enterovirus Infections, Golgi Apparatus virology, Image Processing, Computer-Assisted, Lipid Droplets ultrastructure, Vero Cells, Endoplasmic Reticulum ultrastructure, Enterovirus physiology, Golgi Apparatus ultrastructure, Microscopy, Electron, Scanning, Virus Replication

Abstract

Enterovirus genome replication occurs at virus-induced structures derived from cellular membranes and lipids. However, the origin of these replication organelles (ROs) remains uncertain. Ultrastructural evidence of the membrane donor is lacking, suggesting that the sites of its transition into ROs are rare or fleeting. To overcome this challenge, we combined live-cell imaging and serial block-face scanning electron microscopy of whole cells to capture emerging enterovirus ROs. The first foci of fluorescently labeled viral protein correlated with ROs connected to the endoplasmic reticulum (ER) and preceded the appearance of ROs stemming from the trans -Golgi network. Whole-cell data sets further revealed striking contact regions between ROs and lipid droplets that may represent a route for lipid shuttling to facilitate RO proliferation and genome replication. Our data provide direct evidence that enteroviruses use ER and then Golgi membranes to initiate RO formation, demonstrating the remarkable flexibility with which enteroviruses usurp cellular organelles. IMPORTANCE Enteroviruses are causative agents of a range of human diseases. The replication of these viruses within cells relies on specialized membranous structures termed replication organelles (ROs) that form during infection but whose origin remains elusive. To capture the emergence of enterovirus ROs, we use correlative light and serial block-face scanning electron microscopy, a powerful method to pinpoint rare events in their whole-cell ultrastructural context. RO biogenesis was found to occur first at ER and then at Golgi membranes. Extensive contacts were found between early ROs and lipid droplets (LDs), which likely serve to provide LD-derived lipids required for replication. Together, these data establish the dual origin of enterovirus ROs and the chronology of their biogenesis at different supporting cellular membranes., (Copyright © 2019 Melia et al.)

Published

2019

36. Human iPSC-Derived Retinas Recapitulate the Fetal CRB1 CRB2 Complex Formation and Demonstrate that Photoreceptors and Müller Glia Are Targets of AAV5.

Author

Quinn PM, Buck TM, Mulder AA, Ohonin C, Alves CH, Vos RM, Bialecka M, van Herwaarden T, van Dijk EHC, Talib M, Freund C, Mikkers HMM, Hoeben RC, Goumans MJ, Boon CJF, Koster AJ, Chuva de Sousa Lopes SM, Jost CR, and Wijnholds J

Subjects

Adult, Carrier Proteins genetics, Cells, Cultured, Dependovirus genetics, Ependymoglial Cells cytology, Ependymoglial Cells ultrastructure, Eye Proteins genetics, Female, Fetus, Humans, Immunohistochemistry, Induced Pluripotent Stem Cells cytology, Membrane Proteins genetics, Microscopy, Immunoelectron, Multiprotein Complexes genetics, Multiprotein Complexes metabolism, Nerve Tissue Proteins genetics, Organoids cytology, Photoreceptor Cells, Vertebrate ultrastructure, Pregnancy, Retina cytology, Retina embryology, Carrier Proteins metabolism, Ependymoglial Cells metabolism, Eye Proteins metabolism, Induced Pluripotent Stem Cells metabolism, Membrane Proteins metabolism, Nerve Tissue Proteins metabolism, Organoids metabolism, Photoreceptor Cells, Vertebrate metabolism, Retina metabolism

Abstract

Human retinal organoids from induced pluripotent stem cells (hiPSCs) can be used to confirm the localization of proteins in retinal cell types and to test transduction and expression patterns of gene therapy vectors. Here, we compared the onset of CRB protein expression in human fetal retina with human iPSC-derived retinal organoids. We show that CRB2 protein precedes the expression of CRB1 in the developing human retina. Our data suggest the presence of CRB1 and CRB2 in human photoreceptors and Müller glial cells. Thus the fetal CRB complex formation is replicated in hiPSC-derived retina. CRB1 patient iPSC retinal organoids showed disruptions at the outer limiting membrane as found in Crb1 mutant mice. Furthermore, AAV serotype 5 (AAV5) is potent in infecting human Müller glial cells and photoreceptors in hiPSC-derived retinas and retinal explants. Our data suggest that human photoreceptors can be efficiently transduced by AAVs in the presence of photoreceptor segments., (Copyright © 2019 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2019

37. Localization of active endogenous and exogenous β-glucocerebrosidase by correlative light-electron microscopy in human fibroblasts.

Author

van Meel E, Bos E, van der Lienden MJC, Overkleeft HS, van Kasteren SI, Koster AJ, and Aerts JMFG

Subjects

Cells, Cultured, Fibroblasts ultrastructure, Glucosylceramidase genetics, HEK293 Cells, Humans, Lectins, C-Type genetics, Lectins, C-Type metabolism, Lysosomal Membrane Proteins genetics, Lysosomal Membrane Proteins metabolism, Lysosomes metabolism, Lysosomes ultrastructure, Mannose Receptor, Mannose-Binding Lectins genetics, Mannose-Binding Lectins metabolism, Protein Transport, Receptors, Cell Surface genetics, Receptors, Cell Surface metabolism, Receptors, Scavenger genetics, Receptors, Scavenger metabolism, Fibroblasts metabolism, Glucosylceramidase metabolism

Abstract

β-Glucocerebrosidase (GBA) is the enzyme that degrades glucosylceramide in lysosomes. Defects in GBA that result in overall loss of enzymatic activity give rise to the lysosomal storage disorder Gaucher disease, which is characterized by the accumulation of glucosylceramide in tissue macrophages. Gaucher disease is currently treated by infusion of mannose receptor-targeted recombinant GBA. The recombinant GBA is thought to reach the lysosomes of macrophages, based on the impressive clinical response that is observed in Gaucher patients (type 1) receiving this enzyme replacement therapy. In this study, we used cyclophellitol-derived activity-based probes (ABPs) with a fluorescent reporter that irreversibly bind to the catalytic pocket of GBA, to visualize the active enzymes in a correlative microscopy approach. The uptake of pre-labeled recombinant enzyme was monitored by fluorescence and electron microscopy in human fibroblasts that stably expressed the mannose receptor. The endogenous active enzyme was simultaneously visualized by in situ labeling with the ABP containing an orthogonal fluorophore. This method revealed the efficient delivery of recombinant GBA to lysosomal target compartments that contained endogenous active enzyme., (© 2019 The Authors. Traffic published by John Wiley & Sons Ltd.)

Published

2019

38. Correlative cryo super-resolution light and electron microscopy on mammalian cells using fluorescent proteins.

Author

Tuijtel MW, Koster AJ, Jakobs S, Faas FGA, and Sharp TH

Subjects

Animals, Cell Line, Tumor, Humans, Lasers, Lipids chemistry, Nanotubes chemistry, Nanotubes ultrastructure, Vitrification, Cryoelectron Microscopy, Green Fluorescent Proteins metabolism, Mammals metabolism, Microscopy, Fluorescence

Abstract

Sample fixation by vitrification is critical for the optimal structural preservation of biomolecules and subsequent high-resolution imaging by cryo-correlative light and electron microscopy (cryoCLEM). There is a large resolution gap between cryo fluorescence microscopy (cryoFLM), ~400-nm, and the sub-nanometre resolution achievable with cryo-electron microscopy (cryoEM), which hinders interpretation of cryoCLEM data. Here, we present a general approach to increase the resolution of cryoFLM using cryo-super-resolution (cryoSR) microscopy that is compatible with successive cryoEM investigation in the same region. We determined imaging parameters to avoid devitrification of the cryosamples without the necessity for cryoprotectants. Next, we examined the applicability of various fluorescent proteins (FPs) for single-molecule localisation cryoSR microscopy and found that all investigated FPs display reversible photoswitchable behaviour, and demonstrated cryoSR on lipid nanotubes labelled with rsEGFP2 and rsFastLime. Finally, we performed SR-cryoCLEM on mammalian cells expressing microtubule-associated protein-2 fused to rsEGFP2 and performed 3D cryo-electron tomography on the localised areas. The method we describe exclusively uses commercially available equipment to achieve a localisation precision of 30-nm. Furthermore, all investigated FPs displayed behaviour compatible with cryoSR microscopy, making this technique broadly available without requiring specialised equipment and will improve the applicability of this emerging technique for cellular and structural biology.

Published

2019

39. Loss of CRB2 in Müller glial cells modifies a CRB1-associated retinitis pigmentosa phenotype into a Leber congenital amaurosis phenotype.

Author

Quinn PM, Mulder AA, Henrique Alves C, Desrosiers M, de Vries SI, Klooster J, Dalkara D, Koster AJ, Jost CR, and Wijnholds J

Subjects

Animals, Carrier Proteins genetics, Carrier Proteins physiology, Disease Models, Animal, Electroretinography, Ependymoglial Cells metabolism, Ependymoglial Cells physiology, Eye Proteins genetics, Eye Proteins physiology, Leber Congenital Amaurosis genetics, Leber Congenital Amaurosis physiopathology, Macaca fascicularis, Membrane Proteins physiology, Mice, Mice, Inbred C57BL, Mice, Knockout, Mutation, Nerve Tissue Proteins physiology, Neuroglia physiology, Phenotype, Photoreceptor Cells metabolism, Photoreceptor Cells, Vertebrate metabolism, Retina metabolism, Retinal Dystrophies metabolism, Retinitis Pigmentosa metabolism, Retinitis Pigmentosa physiopathology, Membrane Proteins genetics, Nerve Tissue Proteins genetics, Retinitis Pigmentosa genetics

Abstract

Variations in the human Crumbs homolog-1 (CRB1) gene lead to an array of retinal dystrophies including early onset of retinitis pigmentosa (RP) and Leber congenital amaurosis (LCA) in children. To investigate the physiological roles of CRB1 and CRB2 in retinal Müller glial cells (MGCs), we analysed mouse retinas lacking both proteins in MGC. The peripheral retina showed a faster progression of dystrophy than the central retina. The central retina showed retinal folds, disruptions at the outer limiting membrane, protrusion of photoreceptor nuclei into the inner and outer segment layers and ingression of photoreceptor nuclei into the photoreceptor synaptic layer. The peripheral retina showed a complete loss of the photoreceptor synapse layer, intermingling of photoreceptor nuclei within the inner nuclear layer and ectopic photoreceptor cells in the ganglion cell layer. Electroretinography showed severe attenuation of the scotopic a-wave at 1 month of age with responses below detection levels at 3 months of age. The double knockout mouse retinas mimicked a phenotype equivalent to a clinical LCA phenotype due to loss of CRB1. Localization of CRB1 and CRB2 in non-human primate (NHP) retinas was analyzed at the ultrastructural level. We found that NHP CRB1 and CRB2 proteins localized to the subapical region adjacent to adherens junctions at the outer limiting membrane in MGC and photoreceptors. Our data suggest that loss of CRB2 in MGC aggravates the CRB1-associated RP-like phenotype towards an LCA-like phenotype.

Published

2019

40. Weibel-Palade Body Localized Syntaxin-3 Modulates Von Willebrand Factor Secretion From Endothelial Cells.

Author

Schillemans M, Karampini E, van den Eshof BL, Gangaev A, Hofman M, van Breevoort D, Meems H, Janssen H, Mulder AA, Jost CR, Escher JC, Adam R, Carter T, Koster AJ, van den Biggelaar M, Voorberg J, and Bierings R

Subjects

Calcium metabolism, Cells, Cultured, Cyclic AMP metabolism, Endothelial Cells ultrastructure, Human Umbilical Vein Endothelial Cells metabolism, Humans, Malabsorption Syndromes diagnosis, Malabsorption Syndromes genetics, Microvilli genetics, Microvilli metabolism, Mucolipidoses diagnosis, Mucolipidoses genetics, Mutation, Qa-SNARE Proteins genetics, R-SNARE Proteins metabolism, Secretory Pathway, Signal Transduction, Weibel-Palade Bodies ultrastructure, Endothelial Cells metabolism, Exocytosis, Malabsorption Syndromes metabolism, Microvilli pathology, Mucolipidoses metabolism, Qa-SNARE Proteins metabolism, Weibel-Palade Bodies metabolism, von Willebrand Factor metabolism

Abstract

Objective: Endothelial cells store VWF (von Willebrand factor) in rod-shaped secretory organelles, called Weibel-Palade bodies (WPBs). WPB exocytosis is coordinated by a complex network of Rab GTPases, Rab effectors, and SNARE (soluble NSF attachment protein receptor) proteins. We have previously identified STXBP1 as the link between the Rab27A-Slp4-a complex on WPBs and the SNARE proteins syntaxin-2 and -3. In this study, we investigate the function of syntaxin-3 in VWF secretion., Approach and Results: In human umbilical vein endothelial cells and in blood outgrowth endothelial cells (BOECs) from healthy controls, endogenous syntaxin-3 immunolocalized to WPBs. A detailed analysis of BOECs isolated from a patient with variant microvillus inclusion disease, carrying a homozygous mutation in STX3 (STX3 -/- ), showed a loss of syntaxin-3 protein and absence of WPB-associated syntaxin-3 immunoreactivity. Ultrastructural analysis revealed no detectable differences in morphology or prevalence of immature or mature WPBs in control versus STX3 -/- BOECs. VWF multimer analysis showed normal patterns in plasma of the microvillus inclusion disease patient, and media from STX3 -/- BOECs, together indicating WPB formation and maturation are unaffected by absence of syntaxin-3. However, a defect in basal as well as Ca 2+ - and cAMP-mediated VWF secretion was found in the STX3 -/- BOECs. We also show that syntaxin-3 interacts with the WPB-associated SNARE protein VAMP8 (vesicle-associated membrane protein-8)., Conclusions: Our data reveal syntaxin-3 as a novel WPB-associated SNARE protein that controls WPB exocytosis., (© 2018 American Heart Association, Inc.)

Published

2018

41. Ultrastructural Imaging of Salmonella-Host Interactions Using Super-resolution Correlative Light-Electron Microscopy of Bioorthogonal Pathogens.

Author

van Elsland DM, Pujals S, Bakkum T, Bos E, Oikonomeas-Koppasis N, Berlin I, Neefjes J, Meijer AH, Koster AJ, Albertazzi L, and van Kasteren SI

Abstract

The imaging of intracellular pathogens inside host cells is complicated by the low resolution and sensitivity of fluorescence microscopy and by the lack of ultrastructural information to visualize the pathogens. Herein, we present a new method to visualize these pathogens during infection that circumvents these problems: by using a metabolic hijacking approach to bioorthogonally label the intracellular pathogen Salmonella Typhimurium and by using these bioorthogonal groups to introduce fluorophores compatible with stochastic optical reconstruction microscopy (STORM) and placing this in a correlative light electron microscopy (CLEM) workflow, the pathogen can be imaged within its host cell context Typhimurium with a resolution of 20 nm. This STORM-CLEM approach thus presents a new approach to understand these pathogens during infection., (© 2018 The Authors. Published by Wiley-VCH Verlag GmbH & Co. KGaA.)

Published

2018

42. Correlative microscopy for structural microbiology.

Author

Howes SC, Koning RI, and Koster AJ

Subjects

Bacteria ultrastructure, Communicable Diseases microbiology, Humans, Mass Spectrometry, Microscopy instrumentation, Microscopy, Electron instrumentation, Single Molecule Imaging methods, Viruses ultrastructure, Host Microbial Interactions, Microscopy methods, Microscopy, Electron methods, Single Molecule Imaging instrumentation

Abstract

Understanding how microbes utilize their environment is aided by visualizing them in their natural context at high resolution. Correlative imaging enables efficient targeting and identification of labelled viral and bacterial components by light microscopy combined with high resolution imaging by electron microscopy. Advances in genetic and bioorthogonal labelling, improved workflows for targeting and image correlation, and large-scale data collection are increasing the applicability of correlative imaging methods. Furthermore, developments in mass spectroscopy and soft X-ray imaging are expanding the correlative imaging modalities available. Investigating the structure and organization of microbes within their host by combined imaging methods provides important insights into mechanisms of infection and disease which cannot be obtained by other techniques., (Copyright © 2018 Elsevier Ltd. All rights reserved.)

Published

2018

43. Advances in cryo-electron tomography for biology and medicine.

Author

Koning RI, Koster AJ, and Sharp TH

Subjects

Animals, Humans, Image Processing, Computer-Assisted, Tissue Fixation, Cryoelectron Microscopy methods, Electron Microscope Tomography methods

Abstract

Cryo-electron tomography (CET) utilizes a combination of specimen cryo-fixation and multi-angle electron microscopy imaging to produce three-dimensional (3D) volume reconstructions of native-state macromolecular and subcellular biological structures with nanometer-scale resolution. In recent years, cryo-electron microscopy (cryoEM) has experienced a dramatic increase in the attainable resolution of 3D reconstructions, resulting from technical improvements of electron microscopes, improved detector sensitivity, the implementation of phase plates, automated data acquisition schemes, and improved image reconstruction software and hardware. These developments also greatly increased the usability and applicability of CET as a diagnostic and research tool, which is now enabling structural biologists to determine the structure of proteins in their native cellular environment to sub-nanometer resolution. These recent technical developments have stimulated us to update on our previous review (Koning, R.I., Koster, A.J., 2009. Cryo-electron tomography in biology and medicine. Ann Anat 191, 427-445) in which we described the fundamentals of CET. In this follow-up, we extend this basic description in order to explain the aforementioned recent advances, and describe related 3D techniques that can be applied to the anatomy of biological systems that are relevant for medicine., (Copyright © 2018 Elsevier GmbH. All rights reserved.)

Published

2018

44. The Origin, Dynamic Morphology, and PI4P-Independent Formation of Encephalomyocarditis Virus Replication Organelles.

Author

Melia CE, van der Schaar HM, de Jong AWM, Lyoo HR, Snijder EJ, Koster AJ, van Kuppeveld FJM, and Bárcena M

Subjects

Electron Microscope Tomography, Endoplasmic Reticulum metabolism, Endoplasmic Reticulum ultrastructure, HeLa Cells, Humans, Organelles ultrastructure, Encephalomyocarditis virus physiology, Organelle Biogenesis, Organelles virology, Phosphatidylinositol Phosphates metabolism, Virus Replication

Abstract

Picornaviruses induce dramatic rearrangements of endomembranes in the cells that they infect to produce dedicated platforms for viral replication. These structures, termed replication organelles (ROs), have been well characterized for the Enterovirus genus of the Picornaviridae However, it is unknown whether the diverse RO morphologies associated with enterovirus infection are conserved among other picornaviruses. Here, we use serial electron tomography at different stages of infection to assess the three-dimensional architecture of ROs induced by encephalomyocarditis virus (EMCV), a member of the Cardiovirus genus of the family of picornaviruses that is distantly related. Ultrastructural analyses revealed connections between early single-membrane EMCV ROs and the endoplasmic reticulum (ER), establishing the ER as a likely donor organelle for their formation. These early single-membrane ROs appear to transform into double-membrane vesicles (DMVs) as infection progresses. Both single- and double-membrane structures were found to support viral RNA synthesis, and progeny viruses accumulated in close proximity, suggesting a spatial association between RNA synthesis and virus assembly. Further, we explored the role of phosphatidylinositol 4-phosphate (PI4P), a critical host factor for both enterovirus and cardiovirus replication that has been recently found to expedite enterovirus RO formation rather than being strictly required. By exploiting an EMCV escape mutant, we found that low-PI4P conditions could also be overcome for the formation of cardiovirus ROs. Collectively, our data show that despite differences in the membrane source, there are striking similarities in the biogenesis, morphology, and transformation of cardiovirus and enterovirus ROs, which may well extend to other picornaviruses. IMPORTANCE Like all positive-sense RNA viruses, picornaviruses induce the rearrangement of host cell membranes to form unique structures, or replication organelles (ROs), that support viral RNA synthesis. Here, we investigate the architecture and biogenesis of cardiovirus ROs and compare them with those induced by enteroviruses, members of the well-characterized picornavirus genus Enterovirus The origins and dynamic morphologies of cardiovirus ROs are revealed using electron tomography, which points to the endoplasmic reticulum as the donor organelle usurped to produce single-membrane tubules and vesicles that transform into double-membrane vesicles. We show that PI4P, a critical lipid for cardiovirus and enterovirus replication, is not strictly required for the formation of cardiovirus ROs, as functional ROs with typical morphologies are formed under phosphatidylinositol 4-kinase type III alpha (PI4KA) inhibition in cells infected with an escape mutant. Our data show that the transformation from single-membrane structures to double-membrane vesicles is a conserved feature of cardiovirus and enterovirus infections that likely extends to other picornavirus genera., (Copyright © 2018 Melia et al.)

Published

2018

45. Renal Subcapsular Transplantation of PSC-Derived Kidney Organoids Induces Neo-vasculogenesis and Significant Glomerular and Tubular Maturation In Vivo.

Author

van den Berg CW, Ritsma L, Avramut MC, Wiersma LE, van den Berg BM, Leuning DG, Lievers E, Koning M, Vanslambrouck JM, Koster AJ, Howden SE, Takasato M, Little MH, and Rabelink TJ

Subjects

Animals, Cell Differentiation physiology, Endothelial Cells physiology, Humans, Kidney Transplantation methods, Mice, Morphogenesis physiology, Podocytes physiology, Kidney Glomerulus physiology, Kidney Tubules physiology, Organoids physiology, Pluripotent Stem Cells physiology

Abstract

Human pluripotent stem cell (hPSC)-derived kidney organoids may facilitate disease modeling and the generation of tissue for renal replacement. Long-term application, however, will require transferability between hPSC lines and significant improvements in organ maturation. A key question is whether time or a patent vasculature is required for ongoing morphogenesis. Here, we show that hPSC-derived kidney organoids, derived in fully defined medium conditions and in the absence of any exogenous vascular endothelial growth factor, develop host-derived vascularization. In vivo imaging of organoids under the kidney capsule confirms functional glomerular perfusion as well as connection to pre-existing vascular networks in the organoids. Wide-field electron microscopy demonstrates that transplantation results in formation of a glomerular basement membrane, fenestrated endothelial cells, and podocyte foot processes. Furthermore, compared with non-transplanted organoids, polarization and segmental specialization of tubular epithelium are observed. These data demonstrate that functional vascularization is required for progressive morphogenesis of human kidney organoids., (Copyright © 2018 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2018

46. The Mixed Opioid Receptor Antagonist Naltrexone Mitigates Stimulant-Induced Euphoria: A Double-Blind, Placebo-Controlled Trial of Naltrexone.

Author

Spencer TJ, Bhide P, Zhu J, Faraone SV, Fitzgerald M, Yule AM, Uchida M, Spencer AE, Hall AM, Koster AJ, Feinberg L, Kassabian S, Storch B, and Biederman J

Subjects

Adolescent, Adult, Central Nervous System Stimulants administration & dosage, Double-Blind Method, Drug Administration Schedule, Female, Humans, Male, Methylphenidate administration & dosage, Naltrexone administration & dosage, Narcotic Antagonists administration & dosage, Treatment Outcome, Young Adult, Attention Deficit Disorder with Hyperactivity drug therapy, Central Nervous System Stimulants adverse effects, Drug-Related Side Effects and Adverse Reactions drug therapy, Euphoria drug effects, Methylphenidate adverse effects, Naltrexone pharmacology, Narcotic Antagonists pharmacology

Abstract

Objective: Supratherapeutic doses of methylphenidate activate μ-opioid receptors, which are linked to euphoria. This study assessed whether naltrexone, a mixed μ-opioid antagonist, may attenuate the euphoric effects of stimulants, thereby minimizing their abuse potential in subjects with attention-deficit/hyperactivity disorder (ADHD)., Methods: We conducted a 6-week, double-blind, placebo-controlled, randomized clinical trial of naltrexone in adults with DSM-IV ADHD receiving open treatment with a long-acting formulation of methylphenidate (January 2013 to June 2015). Spheroidal Oral Drug Absorption System methylphenidate (SODAS-MPH) was administered twice daily, was titrated to ~1 mg/kg/d over 3 weeks, and was continued for 3 additional weeks depending on response and adverse effects. Subjects were adults with ADHD preselected for having experienced euphoria with an oral test dose of 60 mg of immediate-release methylphenidate (IR-MPH). The primary outcome measure was Question 2 (Liking a Drug Effect) on the Drug Rating Questionnaire, Subject version, which was assessed after oral test doses of 60 mg of IR-MPH were administered after the third and sixth weeks of treatment with SODAS-MPH., Results: Thirty-seven subjects who experienced stimulant-induced (mild) euphoria at a baseline visit were started in the open trial of SODAS-MPH and randomized to naltrexone 50 mg/d or placebo. Thirty-one subjects completed through week 3, and 25 completed through week 6. Naltrexone significantly diminished the euphoric effect of IR-MPH during the heightened-risk titration phase (primary outcome; first 3 weeks) (χ² = 5.07, P = .02) but not the maintenance phase (weeks 4-6) (χ² = 0.22, P = .64) of SODAS-MPH treatment., Conclusions: Preclinical findings are extended to humans showing that naltrexone may mitigate stimulant-associated euphoria. Our findings provide support for further studies combining opioid receptor antagonists with stimulants to reduce abuse potential., Trial Registration: ClinicalTrials.gov identifier: NCT01673594., (© Copyright 2018 Physicians Postgraduate Press, Inc.)

Published

2018

47. Structures of C1-IgG1 provide insights into how danger pattern recognition activates complement.

Author

Ugurlar D, Howes SC, de Kreuk BJ, Koning RI, de Jong RN, Beurskens FJ, Schuurman J, Koster AJ, Sharp TH, Parren PWHI, and Gros P

Subjects

Alarmins ultrastructure, Antibodies, Monoclonal chemistry, Antibodies, Monoclonal ultrastructure, Binding Sites, Complement C1 ultrastructure, Cryoelectron Microscopy, Humans, Immunoglobulin G genetics, Immunoglobulin G ultrastructure, Alarmins chemistry, Complement Activation, Complement C1 chemistry, Immunoglobulin G chemistry

Abstract

Danger patterns on microbes or damaged host cells bind and activate C1, inducing innate immune responses and clearance through the complement cascade. How these patterns trigger complement initiation remains elusive. Here, we present cryo-electron microscopy analyses of C1 bound to monoclonal antibodies in which we observed heterogeneous structures of single and clustered C1-immunoglobulin G1 (IgG1) hexamer complexes. Distinct C1q binding sites are observed on the two Fc-CH2 domains of each IgG molecule. These are consistent with known interactions and also reveal additional interactions, which are supported by functional IgG1-mutant analysis. Upon antibody binding, the C1q arms condense, inducing rearrangements of the C1r 2 s 2 proteases and tilting C1q's cone-shaped stalk. The data suggest that C1r may activate C1s within single, strained C1 complexes or between neighboring C1 complexes on surfaces., (Copyright © 2018 The Authors, some rights reserved; exclusive licensee American Association for the Advancement of Science. No claim to original U.S. Government Works.)

Published

2018

48. Postmortem MRI and histology demonstrate differential iron accumulation and cortical myelin organization in early- and late-onset Alzheimer's disease.

Author

Bulk M, Abdelmoula WM, Nabuurs RJA, van der Graaf LM, Mulders CWH, Mulder AA, Jost CR, Koster AJ, van Buchem MA, Natté R, Dijkstra J, and van der Weerd L

Subjects

Adult, Aged, Aged, 80 and over, Amyloid beta-Peptides metabolism, Autopsy, Disease Susceptibility, Female, Humans, Male, Middle Aged, tau Proteins metabolism, Alzheimer Disease diagnostic imaging, Alzheimer Disease pathology, Cerebral Cortex metabolism, Cerebral Cortex pathology, Diffusion Magnetic Resonance Imaging, Iron metabolism, Myelin Sheath metabolism, Myelin Sheath pathology

Abstract

Previous MRI studies reported cortical iron accumulation in early-onset (EOAD) compared to late-onset (LOAD) Alzheimer disease patients. However, the pattern and origin of iron accumulation is poorly understood. This study investigated the histopathological correlates of MRI contrast in both EOAD and LOAD. T2*-weighted MRI was performed on postmortem frontal cortex of controls, EOAD, and LOAD. Images were ordinally scored using predefined criteria followed by histology. Nonlinear histology-MRI registration was used to calculate pixel-wise spatial correlations based on the signal intensity. EOAD and LOAD were distinguishable based on 7T MRI from controls and from each other. Histology-MRI correlation analysis of the pixel intensities showed that the MRI contrast is best explained by increased iron accumulation and changes in cortical myelin, whereas amyloid and tau showed less spatial correspondence with T2*-weighted MRI. Neuropathologically, subtypes of Alzheimer's disease showed different patterns of iron accumulation and cortical myelin changes independent of amyloid and tau that may be detected by high-field susceptibility-based MRI., (Copyright © 2017 Elsevier Inc. All rights reserved.)

Published

2018

49. Opiate Antagonists Do Not Interfere With the Clinical Benefits of Stimulants in ADHD: A Double-Blind, Placebo-Controlled Trial of the Mixed Opioid Receptor Antagonist Naltrexone.

Author

Spencer TJ, Bhide P, Zhu J, Faraone SV, Fitzgerald M, Yule AM, Uchida M, Spencer AE, Hall AM, Koster AJ, and Biederman J

Subjects

Adolescent, Adult, Central Nervous System Stimulants adverse effects, Central Nervous System Stimulants therapeutic use, Delayed-Action Preparations therapeutic use, Double-Blind Method, Drug Therapy, Combination adverse effects, Female, Humans, Male, Methylphenidate adverse effects, Naltrexone adverse effects, Narcotic Antagonists adverse effects, Narcotic Antagonists therapeutic use, Young Adult, Attention Deficit Disorder with Hyperactivity drug therapy, Euphoria drug effects, Methylphenidate therapeutic use, Naltrexone therapeutic use

Abstract

Objective: Methylphenidate activates μ-opioid receptors, which are linked to euphoria. μ-Opioid antagonists, such as naltrexone, may attenuate the euphoric effects of stimulants, thereby minimizing their abuse potential. This study assessed whether the combination of naltrexone with methylphenidate is well-tolerated while preserving the clinical benefits of stimulants in subjects with attention-deficit/hyperactivity disorder (ADHD)., Methods: We conducted a 6-week, double-blind, placebo-controlled, randomized clinical trial of naltrexone in adults with DSM-IV ADHD receiving open treatment with a long-acting formulation of methylphenidate from January 2013 to July 2015. Spheroidal Oral Drug Absorption System (SODAS) methylphenidate was administered twice daily, was titrated to approximately 1 mg/kg/d over 3 weeks, and was continued for 3 additional weeks depending on response and adverse effects. Subjects were adults with ADHD preselected for having experienced euphoria with a test dose of immediate-release methylphenidate. The primary outcome measure was the Adult ADHD Investigator Symptom Report Scale (AISRS)., Results: Thirty-seven subjects who experienced stimulant-induced (mild) euphoria at a baseline visit were started in the open trial of SODAS methylphenidate and randomly assigned to naltrexone 50 mg or placebo. Thirty-one subjects completed the study through week 3, and 25 completed through week 6. Throughout 6 weeks of blinded naltrexone and open methylphenidate treatment, the coadministration of naltrexone with methylphenidate did not interfere with the clinical effectiveness of methylphenidate for ADHD symptoms. Additionally, the combination of naltrexone and methylphenidate did not produce an increase in adverse events compared with methylphenidate alone., Conclusions: Our findings provide support for the concept of combining opioid receptor antagonists with stimulants to provide an effective stimulant formulation with less abuse potential., Trial Registration: ClinicalTrials.gov identifier: NCT01673594​., (© Copyright 2017 Physicians Postgraduate Press, Inc.)

Published

2018

50. Intradermal vaccination with hollow microneedles: A comparative study of various protein antigen and adjuvant encapsulated nanoparticles.

Author

Du G, Hathout RM, Nasr M, Nejadnik MR, Tu J, Koning RI, Koster AJ, Slütter B, Kros A, Jiskoot W, Bouwstra JA, and Mönkäre J

Subjects

Animals, Antigens chemistry, Drug Liberation, Female, Injections, Intradermal, Lactic Acid administration & dosage, Lactic Acid chemistry, Liposomes, Mice, Inbred BALB C, Mice, Inbred C57BL, Microinjections, Nanoparticles chemistry, Ovalbumin chemistry, Poly I-C chemistry, Polyglycolic Acid administration & dosage, Polyglycolic Acid chemistry, Polylactic Acid-Polyglycolic Acid Copolymer, Vaccination methods, Adjuvants, Immunologic administration & dosage, Antigens administration & dosage, Nanoparticles administration & dosage, Needles, Ovalbumin administration & dosage, Poly I-C administration & dosage, Vaccination instrumentation

Abstract

In this study, we investigated the potential of intradermal delivery of nanoparticulate vaccines to modulate the immune response of protein antigen using hollow microneedles. Four types of nanoparticles covering a broad range of physiochemical parameters, namely poly (lactic-co-glycolic) (PLGA) nanoparticles, liposomes, mesoporous silica nanoparticles (MSNs) and gelatin nanoparticles (GNPs) were compared. The developed nanoparticles were loaded with a model antigen (ovalbumin (OVA)) with and without an adjuvant (poly(I:C)), followed by the characterization of size, zeta potential, morphology, and loading and release of antigen and adjuvant. An in-house developed hollow-microneedle applicator was used to inject nanoparticle suspensions precisely into murine skin at a depth of about 120μm. OVA/poly(I:C)-loaded nanoparticles and OVA/poly(I:C) solution elicited similarly strong total IgG and IgG1 responses. However, the co-encapsulation of OVA and poly(I:C) in nanoparticles significantly increased the IgG2a response compared to OVA/poly(I:C) solution. PLGA nanoparticles and liposomes induced stronger IgG2a responses than MSNs and GNPs, correlating with sustained release of the antigen and adjuvant and a smaller nanoparticle size. When examining cellular responses, the highest CD8 + and CD4 + T cell responses were induced by OVA/poly(I:C)-loaded liposomes. In conclusion, the applicator controlled hollow microneedle delivery is an excellent method for intradermal injection of nanoparticle vaccines, allowing selection of optimal nanoparticle formulations for humoral and cellular immune responses., (Copyright © 2017 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2017