S'identifier

Leiden University Medical Center

36 ARTICLES PUBLISHED IN JoVE

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Medicine

Accurate and Simple Evaluation of Vascular Anastomoses in Monochorionic Placenta using Colored Dye
Enrico Lopriore 1, Femke Slaghekke 2, Johanna M. Middeldorp 2, Frans J. Klumper 2, Jan M. van Lith 3, Frans J. Walther 1, Dick Oepkes 2
1Division of Neonatology, Department of Pediatrics, Leiden University Medical Center, 2Division of Fetal Therapy, Department of Obstetrics, Leiden University Medical Center, 3Department of Obstetrics, Leiden University Medical Center

Twin-to-twin transfusion syndrome and twin anemia polycythemia sequence are two potentially devastating problems in perinatal medicine. Both disorders occur only in monochorionic twins and result from unbalanced blood flow through placental vascular anastomoses. We provide a simple protocol to accurately evaluate the presence of vascular anastomoses using colored dye injection of placental vessels after birth.

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Biology

Monitoring of Ubiquitin-proteasome Activity in Living Cells Using a Degron (dgn)-destabilized Green Fluorescent Protein (GFP)-based Reporter Protein
Ruth Greussing 1, Hermann Unterluggauer 1, Rafal Koziel 1, Andrea B. Maier 2, Pidder Jansen-Dürr 1
1Molecular and Cell Biology, Institute for Biomedical Aging Research, 2Department of Gerontology and Geriatrics, Netherlands Consortium for Healthy Aging, Leiden University Medical Center

A method to monitor ubiquitin-proteasome activity in living cells is described. A degron-destabilized GFP- (GFP-dgn) and a stable GFP-dgnFS fusion protein are generated and transduced into the cell using a lentiviral expression vector. This technique allows to generate a stable GFP-dgn/GFP-dgnFS expressing cell line in which ubiquitin-proteasome activity can be easily assessed using epifluorescence or flow cytometry.

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Medicine

Spheroid Assay to Measure TGF-β-induced Invasion
Hildegonda P.H. Naber 1, Eliza Wiercinska 1, Peter ten Dijke 1, Theo van Laar 1
1Department of Molecular Cell Biology and Centre for Biomedial Genetics, Leiden University Medical Centre

An assay to quantitatively measure Transforming Growth Factor (TGF)-β-induced invasion in 3-dimensional collagen gels is described. This assay takes advantage of the MCF10A series of cell lines, which represent different stages of breast cancer development. This method can be adopted to be used with other cell lines and might be used to investigate other potential activators or inhibitors of invasion.

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Behavior

Assessing Functional Performance in the Mdx Mouse Model
Annemieke Aartsma-Rus 1, Maaike van Putten 1
1Department of Human Genetics, Leiden University Medical Center

The primary outcome measure in clinical trials for neuromuscular disorders is generally improved muscle function. Therefore, assessing the effect of potential therapeutic compounds on muscle performance pre clinically in mouse models is of great importance. We here describe several functional tests to address this.

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Medicine

Orthotopic Injection of Breast Cancer Cells into the Mammary Fat Pad of Mice to Study Tumor Growth.
Begüm Kocatürk 1, Henri H. Versteeg 1
1Department of Hemostasis and Thrombosis, Leiden University Medical Center

Cancer is a complex disease that is influenced by the tissue surrounding the tumor as well as local pro- and anti-inflammatory mediators. Therefore, orthotropic injection models, rather than subcutaneous models may be useful to study cancer progression in a manner that better mimics human pathology.

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Medicine

State of the Art Cranial Ultrasound Imaging in Neonates
Ginette M. Ecury-Goossen 1, Fleur A. Camfferman 2, Lara M. Leijser 3,4, Paul Govaert 1,5, Jeroen Dudink 1,2
1Department of Pediatrics, Division of Neonatology, Erasmus MC-Sophia Children's Hospital, 2Department of Radiology, Erasmus MC-Sophia Children's Hospital, 3Department of Pediatrics, Division of Neonatology, UZ Brussel, 4Department of Pediatrics, Division of Neonatology, Leiden University Medical Center, 5Department of Pediatrics, Division of Neonatology, Isala Hospital, 6Department of Pediatrics, Koningin Paola Children's Hospital

Cranial ultrasound (CUS) is a valuable tool for brain imaging in critically ill neonates. This video shows a comprehensive approach for neonatal (Doppler) CUS for both clinical and research purposes, including a bedside demonstration of the technique.

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Medicine

Human Dupuytren's Ex Vivo Culture for the Study of Myofibroblasts and Extracellular Matrix Interactions
Sofia Karkampouna 1, Peter Kloen 2, Miryam C. Obdeijn 3, Scott M. Riester 4, Andre J. van Wijnen 4,5, Marianna Kruithof-de Julio 1,6
1Department of Molecular Cell Biology, Cancer Genomics Centre and Centre for Biomedical Genetics, Leiden University Medical Center, 2Department of Orthopedic Surgery, Academic Medical Center, 3Department of Plastic, Reconstructive and Hand Surgery, Academic Medical Center, 4Department of Orthopedic Surgery, Mayo Clinic, 5Department of Biochemistry and Molecular Biology, Mayo Clinic, 6Department of Dermatology, Leiden University Medical Center

Dupuytren’s disease (DD) is a fibroproliferative disease of the palm of the hand. Here, we present a protocol to culture resection specimens from DD in a three-dimensional (3D) culture system. Such short-term culture system allows preservation of the 3D structure and molecular properties of the fibrotic tissue.

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Bioengineering

Culturing Mouse Cardiac Valves in the Miniature Tissue Culture System
Boudewijn P.T. Kruithof 1, Samuel C. Lieber 2, Marianna Kruithof-de Julio 3, Vincian Gaussin 4, Marie José Goumans 1
1Department of Molecular Cell Biology, Leiden University Medical Center, 2Department of Engineering Technology, New Jersey Institute of Technology, 3Department of Urology, Leiden University Medical Center, 4Cardiovascular Research Institute, Department of Cell Biology and Molecular Medicine, Rutgers New Jersey Medical School

Here, we present an ex vivo flow model in which murine cardiac valves can be cultured allowing the study of the biology of the valve.

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Medicine

A Novel Murine Model of Arteriovenous Fistula Failure: The Surgical Procedure in Detail
Chun Yu Wong 1,2,3, Margreet R. de Vries 2,3, Yang Wang 4, Joost R. van der Vorst 3, Alexander L. Vahrmeijer 3, Anton-Jan van Zonneveld 1,2, Jaap F. Hamming 3, Prabir Roy-Chaudhury 4, Ton J. Rabelink 1,2, Paul H. A. Quax 2,3, Joris I. Rotmans 1,2
1Department of Nephrology, Leiden University Medical Center, 2Einthoven Laboratory for Experimental Vascular Medicine, Leiden University Medical Center, 3Department of Surgery, Leiden University Medical Center, 4Division of Nephrology, University of Cincinnati

Here we present a murine model of arteriovenous fistula (AVF) failure in which a clinically relevant anastomotic configuration is incorporated. This model can be used to study the pathophysiology and to test possible therapeutic interventions.

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Medicine

Percutaneous Hepatic Perfusion (PHP) with Melphalan as a Treatment for Unresectable Metastases Confined to the Liver
Eleonora M. de Leede 1, Mark C. Burgmans 2, Christian H. Martini 3, Fred G. J. Tijl 4, Arian R. van Erkel 2, Jaap Vuyk 3, Ellen Kapiteijn 5, Cornelis Verhoef 6, Cornelis J. H. van de Velde 1, Alexander L. Vahrmeijer 1
1Department of Surgery, Leiden University Medical Centre, 2Department of Radiology, Leiden University Medical Centre, 3Department of Anesthesiology, Leiden University Medical Centre, 4Department of Extracorporeal Circulation, Leiden University Medical Centre, 5Department of Medical Oncology, Leiden University Medical Centre, 6Department of Surgery, Erasmus MC Cancer Institute

In this manuscript, we describe percutaneous isolated hepatic perfusion with simultaneous chemofiltration as treatment for unresectable liver metastases. This procedure is performed under general anaesthesia in the angiosuite by an experienced team, consisting of an interventional radiologist, a clinical perfusionist and anaesthesiologist.

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Cancer Research

Invasive Behavior of Human Breast Cancer Cells in Embryonic Zebrafish
Jiang Ren *1, Sijia Liu *1, Chao Cui 1, Peter ten Dijke 1
1Department of Molecular Cell Biology, Cancer Genomics Centre Netherlands, Leiden University Medical Center

Here, we describe xenograft zebrafish models using two different injection sites, i.e., perivitelline space and duct of Cuvier, to investigate the invasive behavior and to assess the intravasation and extravasation potential of human breast cancer cells, respectively.

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Developmental Biology

Electrophysiological Analysis of human Pluripotent Stem Cell-derived Cardiomyocytes (hPSC-CMs) Using Multi-electrode Arrays (MEAs)
Luca Sala 1, Dorien Ward-van Oostwaard 1, Leon G. J. Tertoolen 1, Christine L Mummery 1,2, Milena Bellin 1
1Department of Anatomy and Embryology, Leiden University Medical Center, 2Department of Applied Stem Cell Technologies, University of Twente

Electrophysiological characterization of cardiomyocytes derived from human Pluripotent Stem Cells (hPSC-CMs) is crucial for cardiac disease modeling and for determining drug responses. This protocol provides the necessary information to dissociate and plate hPSC-CMs on multi-electrode arrays, measure their field potential, and a method for analyzing QT and RR intervals.

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Cancer Research

Four-color Fluorescence Immunohistochemistry of T-cell Subpopulations in Archival Formalin-fixed, Paraffin-embedded Human Oropharyngeal Squamous Cell Carcinoma Samples
Simone Punt 1, Robert J. Baatenburg de Jong 2, Ekaterina S. Jordanova 1,3
1Department of Pathology, Leiden University Medical Center, 2Department of Otorhinolaryngology and Head and Neck Surgery, Erasmus University Medical Center, 3Center for Gynecological Oncology Amsterdam, VU Medical Center

Multiparameter fluorescence immunohistochemistry can be used to assess the number, relative distribution, and localization of immune cell populations in the tumor microenvironment. This manuscript describes the use of this technique to analyze T-cell subpopulations in oropharyngeal cancer.

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Medicine

A Novel Clinical Grade Isolation Method for Human Kidney Perivascular Stromal Cells
Daniëlle G. Leuning 1, Ellen Lievers 1, Marlies E.J. Reinders 1, Cees van Kooten 1, Marten A. Engelse 1, Ton J. Rabelink 1
1Department of Internal Medicine, Leiden University Medical Centre

Here we present a novel clinical grade isolation and culture method for kidney Perivascular Stromal Cells (kPSCs) based on whole organ perfusion with digestive enzymes and NG2-cell enrichment. With this method, it is possible to acquire sufficient cell numbers for cellular therapy.

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Developmental Biology

The Isolation and Culture of Primary Epicardial Cells Derived from Human Adult and Fetal Heart Specimens
Esther Dronkers 1, Asja T. Moerkamp 1, Tessa van Herwaarden 1, Marie-José Goumans 1, Anke M. Smits 1
1Department of Molecular Cell Biology, Leiden University Medical Center

The epicardium plays a crucial role in the development and repair of the heart by providing cells and growth factors to the myocardial wall. Here, we describe a method to culture human primary epicardial cells that enables the study and comparison of their developmental and adult characteristics.

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Medicine

Impact of Intracardiac Neurons on Cardiac Electrophysiology and Arrhythmogenesis in an Ex Vivo Langendorff System
Christiane Jungen 1,2, Katharina Scherschel 1,2, Nadja I. Bork 2,3, Pawel Kuklik 1, Christian Eickholt 1, Helge Kniep 1, Niklas Klatt 1,2, Stephan Willems 1,2, Viacheslav O. Nikolaev 2,3, Christian Meyer 1,2
1Department of Cardiology-Electrophysiology, cNEP (cardiac Neuro- and Electrophysiology research group), University Heart Center, University Hospital Hamburg-Eppendorf, 2DZHK (German Center for Cardiovascular Research), 3Institute of Experimental Cardiovascular Research, University Medical Center Hamburg-Eppendorf

Here, we present a protocol for the modulation of the intracardiac autonomic nervous system and the assessment of its influence on basic electrophysiology, arrhythmogenesis, and cAMP dynamics using an ex vivo Langendorff setup.

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Developmental Biology

Microfluidic Assay for the Assessment of Leukocyte Adhesion to Human Induced Pluripotent Stem Cell-derived Endothelial Cells (hiPSC-ECs)
Oleh V. Halaidych 1, Francijna van den Hil 1, Christine L. Mummery 1,2, Valeria V. Orlova 1
1Department of Anatomy and Embryology, Leiden University Medical Center, 2Department of Applied Stem Cell Technologies, University of Twente

This step-by-step protocol provides a detailed description of the experimental setup and data analysis for the assessment of inflammatory responses in hiPSC-ECs and the analysis of leukocyte adhesion under physiological flow.

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Immunology and Infection

A High-throughput Assay to Assess and Quantify Neutrophil Extracellular Trap Formation
Eline J. Arends *1, Laura S. van Dam *1, Tineke Kraaij 1, Sylvia W.A. Kamerling 1, Ton J. Rabelink 1, Cees van Kooten 1, Y.K. Onno Teng 1
1Department of Nephrology, Leiden University Medical Center

This protocol describes a highly sensitive and high throughput neutrophil extracellular trap (NET) assay for the semi-automated quantification of ex vivo NET formation by immunofluorescence three-dimensional confocal microscopy. This protocol can be used to evaluate NET formation and degradation after different stimuli and can be used to study potential NET-targeted therapies.

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Environment

Using Caenorhabditis elegans for Studying Trans- and Multi-Generational Effects of Toxicants
Zhuo Li 1,2, Fangting Ai 3, Jing Zhang 4, Zhenyang Yu 1,2, Daqiang Yin 1,2
1College of Environmental Sciences and Engineering, Tongji University, 2Shanghai Institute of Pollution Control and Ecological Security, 3Jiaxing Tongji Institute of Environment, 4College of Ecological Technique and Engineering, Shanghai Institute of Technology

Trans- and multi-generational effects of persistent chemicals are essential in judging their long-term consequences in the environment and on the human health. We provide novel detailed methods for studying trans- and multi-generational effects using free-living nematode Caenorhabditis elegans.

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Bioengineering

Standardized and Scalable Assay to Study Perfused 3D Angiogenic Sprouting of iPSC-derived Endothelial Cells In Vitro
Vincent van Duinen 1,2, Wendy Stam 1, Viola Borgdorff 3, Arie Reijerkerk 3, Valeria Orlova 4, Paul Vulto 5, Thomas Hankemeier 2, Anton Jan van Zonneveld 1
1Department of Internal Medicine (Nephrology) and the Einthoven Laboratory for Vascular and Regenerative Medicine, Leiden University Medical Center, 2Division of Systems Biomedicine and Pharmacology, Department of Analytical BioSciences and Metabolomics, Leiden University, 3Ncardia, 4Department of Anatomy and Embryology, Leiden University Medical Center, 5Mimetas

This method describes the culture of iPSC-derived endothelial cells as 40 perfused 3D microvessels in a standardized microfluidic platform. This platform enables the study of gradient-driven angiogenic sprouting in 3D, including anastomosis and stabilization of the angiogenic sprouts in a scalable and high-throughput manner.

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JoVE Core

CO2-Lasertonsillotomy Under Local Anesthesia in Adults
Justin E.R.E. Wong Chung 1,2, Noud van Helmond 3, Rozemarie van Geet 1, Peter Paul G. van Benthem 2, Henk M. Blom 1,2
1Department of Otolaryngology, HagaZiekenhuis, 2Department of Otolaryngology, Leiden University Medical Center, 3Department of Anesthesiology, Cooper Medical School of Rowan University, Cooper University Hospital

CO2-lasertonsillotomy under local anesthesia is an interesting alternative treatment method for tonsillectomy under general anesthesia for tonsil-related complaints in adults. This report presents a step-by-step protocol detailing the execution of CO2-lasertonsillotomy under local anesthesia.

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Immunology and Infection

Visualization and Quantification of High-Dimensional Cytometry Data using Cytofast and the Upstream Clustering Methods FlowSOM and Cytosplore
Guillaume Beyrend 1, Koen Stam 2, Ferry Ossendorp 1, Ramon Arens 1
1Department of Immunohematology and Blood Transfusion, Leiden University Medical Center, 2Department of Parasitology, Leiden University Medical Center

Cytofast is a visualization tool used to analyze output from clustering. Cytofast can be used to compare two clustering methods: FlowSOM and Cytosplore. Cytofast can rapidly generate a quantitative and qualitative overview of mass cytometry data and highlight the main differences between different clustering algorithms.

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Engineering

Measurement of Chladni Mode Shapes with an Optical Lever Method
Rong Feng *1, Yan Luo *1, Yixue Dong 1, Mengke Ma 2, Yuqi Wang 2, Jing Zhang 3, Wenjiang Ma 3, Donghuan Liu 4
1School of Materials Science and Engineering, University of Science and Technology Beijing, 2School of Civil and Resource Engineering, University of Science and Technology Beijing, 3Basic Experimental Center for Natural Science, University of Science and Technology Beijing, 4School of Mathematics and Physics, University of Science and Technology Beijing

A simple method of measuring the Chladni mode shape on an elastic plate by the principle of an optical lever is proposed.

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Medicine

Evaluation of Color Difference in Placenta with Twin Anemia Polycythemia Sequence
Depeng Zhao 1, Lisanne S.A. Tollenaar 2, Femke Slaghekke 2, Dick Oepkes 2, Tao Duan 3, Enrico Lopriore 4
1Department of Reproductive Medicine, Affiliated Shenzhen Maternity and Child Healthcare Hospital, Southern Medical University, 2Division of Fetal Medicine, Department of Obstetrics, Leiden University Medical Center, 3Fetal Medicine Unit & Prenatal Diagnosis Center, Department of Obstetrics, Shanghai First Maternity and Infant Hospital, Tongji University School of Medicine, 4Division of Neonatology, Department of Pediatrics, Leiden University Medical Center

In monochorionic twins with twin anemia polycythemia sequence (TAPS), the donor twin and its corresponding placenta share are pale, while the recipient twin and its placental share have a plethoric aspect. Presented here is a protocol to quantify the color difference in maternal side of TAPS placenta after birth.

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Cancer Research

Studying TGF-β Signaling and TGF-β-induced Epithelial-to-mesenchymal Transition in Breast Cancer and Normal Cells
Jing Zhang 1, Midory Thorikay 1, Gerard van der Zon 1, Maarten van Dinther 1, Peter ten Dijke 1
1Oncode Institute and Department of Cell Chemical Biology, Leiden University Medical Center

We describe a systematic workflow to investigate TGF-β signaling and TGF-β-induced EMT by studying the protein and gene expression involved in this signaling pathway. The methods include Western blotting, a luciferase reporter assay, qPCR, and immunofluorescence staining.

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Medicine

Location, Dissection, and Analysis of the Murine Stellate Ganglion
Katharina Scherschel 1,2,3, Hanna Bräuninger 2,4, Klara Glufke 2, Christiane Jungen 2,4,5, Nikolaj Klöcker 3, Christian Meyer 1,2,3
1Division of Cardiology, EVK Düsseldorf, cNEP, cardiac Neuro- and Electrophysiology Research Consortium, 2DZHK (German Centre for Cardiovascular Research), 3Institute of Neural and Sensory Physiology, Medical Faculty, Heinrich Heine University Düsseldorf, 4Clinic for Cardiology, University Heart & Vascular Centre, University Hospital Hamburg-Eppendorf, 5Department of Cardiology, Leiden University Medical Center

Pathophysiological changes in the cardiac autonomic nervous system, especially in its sympathetic branch, contribute to the onset and maintenance of ventricular arrhythmias. In the present protocol, we show how to characterize murine stellate ganglia to improve the understanding of the underlying molecular and cellular processes.

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Developmental Biology

Flow Cytometry and Confocal Imaging Analysis of Low Wnt Expression in Axin2-mTurquoise2 Reporter Thymocytes
Jolanda J. D. de Roo 1, Brigitta A.E. Naber 1, Sandra A. Vloemans 1, Edwin F.E. de Haas 1, Annelies M.A. van der Laan 2, Frank J.T Staal 1
1Department of Immunology, Leiden University Medical Center, 2Department of Cell and Chemical Biology, Leiden University Medical Center

Signaling levels are known to regulate cell fate, indicating that regulation of Wnt signaling constitutes an interesting therapeutic target. Here, we describe flow cytometry and confocal microscopy analysis methods for a robust murine canonical Wnt signaling reporter model that measures distinct Wnt signaling levels.

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Biology

TGF-β-mediated Endothelial to Mesenchymal Transition (EndMT) and the Functional Assessment of EndMT Effectors using CRISPR/Cas9 Gene Editing
Jin Ma 1,2, Gerard van der Zon 1,2, Gonzalo Sanchez-Duffhues 1, Peter ten Dijke 1,2
1Dept. Cell Chemical Biology, Leiden University Medical Center, 2Oncode Institute, Leiden University Medical Center

We describe methods to investigate TGF-β2-induced EndMT in endothelial cells by observing cell morphology changes and examining the expression EndMT-related marker changes using immunofluorescence staining. CRISPR/Cas9 gene editing was described and used to deplete the gene encoding Snail to investigate its role in TGF-β2-induced EndMT.

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Medicine

Intraoperative Assessment of Resection Margins in Oral Cavity Cancer: This is the Way
Yassine Aaboubout 1,2, Elisa M. Barroso 1,3,4, Mahesh Algoe 1, Patricia C. Ewing-Graham 1, Ivo ten Hove 3,6, Hetty Mast 3, José A. Hardillo 2, Aniel Sewnaik 2, Dominiek A. Monserez 2, Stijn Keereweer 2, Brend P. Jonker 3, Cornelia G. F. van Lanschot 2, Roeland W. H. Smits 2, Maria R. Nunes Soares 1,4, Lars Ottevanger 1, Sanne E. Matlung 1, Paul A. Seegers 5, Vera van Dis 1, Robert M. Verdijk 1, Eppo B. Wolvius 3, Peter J. Caspers 4, Tom C. Bakker Schut 4, Robert J. Baatenburg de Jong 2, Gerwin J. Puppels 4, Senada Koljenović 1
1Department of Pathology, Erasmus MC University Medical Center, 2Department of Otorhinolaryngology and Head and Neck Surgery, Erasmus MC University Medical Center, 3Department of Oral and Maxillofacial Surgery, Erasmus MC University Medical Center, 4Department of Dermatology, Erasmus MC University Medical Center, 5PALGA foundation, The nationwide network and registry of histo- and cytopathology, 6Department of Oral and Maxillofacial Surgery, Leiden University Medical Center

The goal of this protocol is to provide a clear overview of specimen-driven intraoperative assessment of resection margins. It is encouraged to implement this protocol to improve patient care at other institutes.

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Biology

In Vitro Three-Dimensional Sprouting Assay of Angiogenesis Using Mouse Embryonic Stem Cells for Vascular Disease Modeling and Drug Testing
Georgios Galaris 1, Jérémy H. Thalgott 1, Eliott Teston 1, Franck P.G. Lebrin 1,2,3
1Einthoven Laboratory for Experimental Vascular Medicine, Department of Internal Medicine (Nephrology), Leiden University Medical Center, 2Institute Physics for Medicine Paris, INSERM U1273, ESPCI Paris, CNRS FRE 2031, 3MEMOLIFE Laboratory of Excellence and PSL Research University

This assay utilizes mouse embryonic stem cells differentiated into embryoid bodies cultured in 3D-collagen gel to analyze the biological processes that control sprouting angiogenesis in vitro. The technique can be applied for testing drugs, modeling diseases, and for studying specific genes in the context of deletions that are embryonically lethal.

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Biology

Isolation of Primary Patient-specific Aortic Smooth Muscle Cells and Semiquantitative Real-time Contraction Measurements In Vitro
Natalija Bogunovic *1,2,3, Karlijn B. Rombouts *1,2, Kak Khee Yeung 1,2
1Department of Vascular Surgery, Amsterdam UMC, Vrije Universiteit Amsterdam, 2Department of Physiology, Amsterdam Cardiovascular Sciences, Amsterdam UMC, Vrije Universiteit Amsterdam, 3Laboratory of Experimental Cardiology, Department of Cardiology, Leiden University Medical Center

This paper describes an explant culture-based method for the isolation and culturing of primary, patient-specific human aortic smooth muscle cells and dermal fibroblasts. Furthermore, a novel method is presented for measuring cell contraction and subsequent analysis, which can be used to study patient-specific differences in these cells.

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Medicine

Low-input Nucleus Isolation and Multiplexing with Barcoded Antibodies of Mouse Sympathetic Ganglia for Single-nucleus RNA Sequencing
Yang Ge 1,2, Lieke van Roon 1, H. Sophia Chen 1,2, Ruben Methorst 1, Martin Paton 2, Marco C. DeRuiter 1, Szymon M. Kielbasa 3, Monique R. M. Jongbloed 1,2
1Department of Anatomy & Embryology, Leiden University Medical Center, 2Department of Cardiology, Leiden University Medical Center, 3Department of Medical Statistics and Bioinformatics, Leiden University Medical Center

This protocol describes the detailed, low-input sample preparation for single-nucleus sequencing, including the dissection of mouse superior cervical and stellate ganglia, cell dissociation, cryopreservation, nucleus isolation, and hashtag barcoding.

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Developmental Biology

Efficient Vascularization of Kidney Organoids through Intracelomic Transplantation in Chicken Embryos
Marije Koning 1,2, Ellen Lievers 1,2, Thierry Jaffredo 3, Cathelijne W. van den Berg 1,2,4, Ton J. Rabelink 1,2,4
1Department of Internal Medicine - Nephrology, Leiden University Medical Center, 2Einthoven Laboratory of Vascular and Regenerative Medicine, Leiden University Medical Center, 3IBPS, CNRS UMR7622, Developmental Biology Laboratory, Sorbonne Université, 4The Novo Nordisk Foundation Center for Stem Cell Medicine (reNEW), Leiden University Medical Center

Here, we present a detailed protocol for the transplantation of kidney organoids in the celomic cavity of chicken embryos. This method induces vascularization and enhanced maturation of the organoids within 8 days and can be used to study these processes in an efficient manner.

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Immunology and Infection

Isolating Bronchial Epithelial Cells from Resected Lung Tissue for Biobanking and Establishing Well-Differentiated Air-Liquid Interface Cultures
Dennis K. Ninaber 1, Anne M. van der Does 1, Pieter S. Hiemstra 1
1PulmoScience Laboratory, Department of Pulmonology, Leiden University Medical Center

Presented here is a reproducible, affordable, and robust method for the isolation and expansion of primary bronchial epithelial cells for long-term biobanking and the generation of differentiated epithelial cells by culture at the air-liquid interface.

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Medicine

Imaging and Quantification of the Hepatic Vasculature of Mice Using Ultrafast Doppler Ultrasound
Katerina Stripling 1,2, Finn Timmermans 1,2, Sofiane Décombas-Deschamps 3, Jérémy H. Thalgott 1,2, David Lemonnier 1,2,3, Margreet R. de Vries 2,4,5, Ton J. Rabelink 1,2,6, Mickael Tanter 3, Thomas Deffieux 3, Franck Lebrin 1,2,3
1Department of Internal Medicine - Nephrology, Leiden University Medical Center, 2Einthoven Laboratory of Vascular and Regenerative Medicine, Leiden University Medical Center, 3Institute Physics for Medicine Paris, Inserm, ESPCI-Paris-PSL, 4Department of Surgery - Vascular surgery, Leiden University Medical Center, 5Department of Surgery, Brigham & Women's Hospital, Harvard Medical School, 6The Novo Nordisk Foundation Center for Stem Cell Medicine (reNEW), Leiden University Medical Center

Ultrafast Doppler ultrasound (UFUS) with high spatial resolution (100 mm) and sensitivity represents a suitable noninvasive imaging modality for obtaining a comprehensive qualitative overview of the hepatic vasculature. UFUS also facilitates quantitative measurements of the microvasculature, aiming to enhance our understanding of vascular disease mechanisms.

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Developmental Biology

Human Ovarian Surface Epithelium Organoids as a Platform to Study Tissue Regeneration
Julieta S. Del Valle 1,2, Azra Husetic *1, Dina Diek *1, Laurens F. Rutgers *1, Joyce D. Asseler 3,4,5, Jeroen Metzemaekers 6, Norah M. van Mello 3,4,5, Susana M. Chuva de Sousa Lopes 1,2,7
1Department of Anatomy and Embryology, Leiden University Medical Center, 2The Novo Nordisk Foundation Center for Stem Cell Medicine (reNEW), Leiden University Medical Center, 3Department of Obstetrics and Gynaecology, Amsterdam University Medical Center, 4Centre of Expertise on Gender Dysphoria, Amsterdam UMC, 5Amsterdam Reproduction and Development Research Institute, 6Department of Gynaecology, Leiden University Medical Center, 7Ghent-Fertility and Stem Cell Team (G-FAST), Department of Reproductive Medicine, Ghent University Hospital

This protocol describes establishing three-dimensional (3D) tissue organoids from primary human ovarian surface epithelium (hOSE) cells. The protocol includes isolation of hOSE from freshly collected ovaries, cellular expansion of the hOSE, cryopreservation-thawing procedures, and organoid derivation. Immunofluorescence, quantitative analysis, and showcasing utility as a screening platform are included.

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