Amsterdam UMC

6 ARTICLES PUBLISHED IN JoVE

Bioengineering

A Zebrafish Embryo Model for In Vivo Visualization and Intravital Analysis of Biomaterial-associated Staphylococcus aureus Infection

Xiaolin Zhang^1,2, Leonie de Boer¹, Oliver W. Stockhammer¹, Dirk W. Grijpma^2,3, Herman P. Spaink⁴, Sebastian A.J. Zaat¹

¹Department of Medical Microbiology, Amsterdam UMC, ²Technical Medical Center, Department of Biomaterials Science and Technology, University of Twente, ³Department of Biomedical Engineering, W.J. Kolff Institute, University Medical Center Groningen, University of Groningen, ⁴Institute of Biology, Leiden University

The present study describes a zebrafish embryo model for in vivo visualization and intravital analysis of biomaterial-associated infection over time based on fluorescence microscopy. This model is a promising system complementing mammalian animal models such as mouse models for studying biomaterial-associated infections in vivo.

Biology

Isolating Myofibrils from Skeletal Muscle Biopsies and Determining Contractile Function with a Nano-Newton Resolution Force Transducer

Martijn van de Locht¹, Josine M. de Winter¹, Dilson E. Rassier², Michiel H.B. Helmes^1,3, Coen A.C. Ottenheijm¹

¹Department of Physiology, Amsterdam UMC, ²Department of Kinesiology and Physical Education, Faculty of Education, McGill University, ³IONOptix BV

Presented here is a protocol to assess the contractile properties of striated muscle myofibrils with nano-Newton resolution. The protocol employs a setup with an interferometry-based, optical force probe. This setup generates data with a high signal-to-noise ratio and enables the assessment of the contractile kinetics of myofibrils.

JoVE Core

Acetylcholine Re-Challenge After Intracoronary Nitroglycerine Administration

Rutger G. T. Feenstra¹, Tim P. van de Hoef¹, Marcel A. M. Beijk¹, Jan J. Piek¹

¹Heart Center, Department of Cardiology, Amsterdam Cardiovascular Sciences, Amsterdam UMC

This protocol presents the acetylcholine rechallenge after nitroglycerine as an add-on procedure to spasm provocation testing. The purpose of this technique is to unmask co-existing microvascular spasm in patients with epicardial spasm and to assess the protective efficacy of nitroglycerine on a per-patient level to guide medical therapy.

Biology

High-Throughput Contractile Measurements of Hydrogel-Embedded Intact Mouse Muscle Fibers Using an Optics-Based System

Leander A. Vonk^*1, Osman Esen^*1, Michaela Yuen^1,4, Tyler J. Kirby^1,2,3

¹Department of Physiology, Amsterdam UMC, ²Amsterdam Cardiovascular Sciences, Heart Failures and Arrhythmias, Amsterdam UMC, ³Amsterdam Movement Sciences, Tissue Function and Regeneration, Amsterdam UMC, ⁴Discipline of Child and Adolescent Health, Faculty of Health and Medicine, University of Sydney

Skeletal muscle function can be assessed by quantifying the contractility of isolated muscle fibers, traditionally using laborious, low-throughput approaches. Here, we describe an optics-based, high-throughput method to quantify the contractility of hydrogel-embedded muscle fibers. This approach has applications for drug screening and therapeutic development.

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 Metzemaekers⁶, 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.

Medicine

Induction of Cerebral Arterial Gas Embolism in Rat

Raoul A. Fakkert^1,2,3, Nina C. Weber³, Benedikt Preckel^1,3, Robert A. van Hulst^1,2, Inge A. Mulder^*4,5,6, Robert P. Weenink^*1,2

¹Department of Anesthesiology, Amsterdam UMC, ²Department of Hyperbaric Medicine, Amsterdam UMC, ³Laboratory of Experimental Intensive Care and Anesthesiology, Amsterdam UMC, ⁴Biomedical Engineering and Physics, Amsterdam UMC, ⁵Microcirculation, Amsterdam Cardiovascular Sciences, ⁶Neurovascular Disorders, Amsterdam Neurosciences

This protocol provides a detailed description of inducing cerebral air emboli in rats. It compares direct injection into the common carotid artery and introduction through the external carotid artery. It provides a technical description of the air bubble generator, the effect of different air volumes, and procedural challenges.