"Exocytosis" in JoVE

Exocytosis: Cellular release of material within membrane-limited vesicles by fusion of the vesicles with the Cell membrane.

Lateral Diffusion and Exocytosis of Membrane Proteins in Cultured Neurons Assessed using Fluorescence Recovery and Fluorescence-loss Photobleaching

JoVE 3747 2/29/2012

Keri L. Hildick, Inmaculada M. González-González, Frédéric Jaskolski, Jeremy. M. Henley

MRC Centre for Synaptic Plasticity, University of Bristol

This report describes the use of live cell imaging and photobleach techniques to determine the surface expression, transport pathways and trafficking kinetics of exogenously expressed, pH-sensitive GFP-tagged proteins at the plasma membrane of neurons.

Blood Collection from the American Horseshoe Crab, Limulus Polyphemus

JoVE 958 10/13/2008

Peter Armstrong^1,2, Mara Conrad³

¹Department of Molecular and Cell Biology, University of California, Davis, ²Marine Biological Laboratory - MBL- woods hole, ³Department of Biological Sciences, Hunter College of CUNY

The American horseshoe crab, Limulus polyphemus, is arguably the most convenient source for large quantities of blood of any invertebrate. The blood is simple in composition, with only one cell-type in the general circulation, the granular amebocyte, and only three abundant proteins in the plasma, hemocyanin, the C-reactive proteins, and α2-macroglobulin. Blood is collected from the heart and the blood cells and plasma are separated by centrifugation.

Imaging Exocytosis in Retinal Bipolar Cells with TIRF Microscopy

JoVE 1305 6/09/2009

Christina Joselevitch, David Zenisek

Cellular and Molecular Physiology, Yale University School of Medicine

In this video, we demonstrate how to label and visualize single synaptic vesicle exocytosis and trafficking in goldfish retinal bipolar cells using total internal reflectance fluorescence (TIRF) microscopy.

Measuring Exocytosis in Neurons Using FM Labeling

JoVE 117 11/30/2006

Jamila Newton, Venkatesh Murthy

Department of Molecular and Cell Biology, Harvard

The ability to measure the kinetics of vesicle release can help provide insight into some of the basics of neurotransmission. Here we used real-time imaging of vesicles labeled with the red fluorescent dye FM 4-64 to measure the rate of presynaptic vesicle release in hippocampal neuronal cultures.

Quantitative Analysis of Synaptic Vesicle Pool Replenishment in Cultured Cerebellar Granule Neurons using FM Dyes

JoVE 3143 11/11/2011

Giselle Cheung, Michael A. Cousin

Membrane Biology Group, Centre for integrative Physiology, University of Edinburgh

A live fluorescence imaging technique to quantify the replenishment and mobilisation of specific synaptic vesicle (SV) pools in central nerve terminals is described. Two rounds of SV recycling are monitored in the same nerve terminals providing an internal control.

Patch-clamp Capacitance Measurements and Ca²⁺ Imaging at Single Nerve Terminals in Retinal Slices

JoVE 3345 1/19/2012

Mean-Hwan Kim, Evan Vickers, Henrique von Gersdorff

The Vollum Institute, Oregon Health and Science University

Here we describe a protocol for the preparation of agar-embedded retinal slices that are suitable for electrophysiology and Ca²⁺ imaging. This method allows one to study ribbon-type synapses in retinal microcircuits using direct patch-clamp recordings of single presynaptic nerve terminals.

Methods for Patch Clamp Capacitance Recordings from the Calyx

JoVE 244 7/29/2007

Kenneth Paradiso, Wei Wu, Ling-Gang Wu

National Institute of Neurological Disorders and Stroke, National Institute of Health

We demonstrate the basic techniques for presynaptic patch clamp recording at the calyx of Held, a mammalian central nervous system nerve terminal.

Presynaptically Silent Synapses Studied with Light Microscopy

JoVE 1676 1/04/2010

Krista L. Moulder¹, Xiaoping Jiang¹, Amanda A. Taylor¹, Ann M. Benz¹, Steven Mennerick^1,2,3

¹Department of Psychiatry, Washington University School of Medicine, ²Department of Anatomy, Washington University School of Medicine, ³Department of Neurobiology, Washington University School of Medicine

Glutamatergic synapses can switch from an active mode to a silent mode. We demonstrate that presynaptic activity status in dissociated culture of rodent neurons is visualized using a fixable form of the FM1-43 dye to visualize active synapses and immunostaining with vGluT-1 antibody to visualize all glutamate synapses.

Measuring Near Plasma Membrane and Global Intracellular Calcium Dynamics in Astrocytes

JoVE 1142 4/26/2009

Eiji Shigetomi, Baljit S. Khakh

Departments of Physiology and Neurobiology, David Geffen School of Medicine, University of California, Los Angeles

We describe how to measure near membrane and global intracellular calcium dynamics in cultured astrocytes using total internal reflection and epifluorescence microscopy.

Survivable Stereotaxic Surgery in Rodents

JoVE 880 10/06/2008

Brenda M. Geiger, Lauren E. Frank, Angela D. Caldera-Siu, Emmanuel N. Pothos

Department of Pharmacology and Experimental Therapeutics, Tufts University

The monitoring of extracellular neurotransmitter levels in distinct brain regions of freely moving animals offers insights on the link between neurotransmitter release and behavior. In vivo microdialysis coupled with electrochemical detection provides excellent anatomical and chemical resolution; and information on how basal neurotransmission is altered by pharmacological or physiological manipulations.

Primary Dissociated Midbrain Dopamine Cell Cultures from Rodent Neonates

JoVE 820 11/05/2008

Lauren E. Frank, Angela D. Caldera-Siu, Emmanuel N. Pothos

Department of Pharmacology and Experimental Therapeutics, Tufts University

Primary dissociated midbrain dopamine cell cultures allow for the study of presynaptic characteristics of dopamine neurons. They can be used to monitor real-time dopamine release kinetics and protein/mRNA levels of regulators of dopamine exocytosis. Here, we show you how to generate these cultures from rodent neonates.

Paired Patch Clamp Recordings from Motor-neuron and Target Skeletal Muscle in Zebrafish

JoVE 2351 11/20/2010

Hua Wen, Paul Brehm

Vollum Institute, Oregon Health and Sciences University

Larval zebrafish represent the first vertebrate model system to allow simultaneous patch clamp recording from a spinal motor-neuron and target skeletal muscle. This video demonstrates the microscopic methods used to identify a segmental CaP motor-neuron and target muscle cells as well as the methodologies for recording from each cell type.

Studying Synaptic Vesicle Pools using Photoconversion of Styryl Dyes

JoVE 1790 2/15/2010

Felipe Opazo, Silvio O. Rizzoli

STED Microscopy of Synaptic Function, European Neuroscience Institute Göttingen

FM dyes have been of invaluable help in the understanding of synaptic dynamics. FMs are normally followed under the fluorescent microscope during different stimulation conditions. However, photoconversion of FM dyes combined with electron microscopy allows the visualization of distinct synaptic vesicle pools, among other ultrastructure components, in synaptic boutons.

Ex Vivo Red Blood Cell Hemolysis Assay for the Evaluation of pH-responsive Endosomolytic Agents for Cytosolic Delivery of Biomacromolecular Drugs

JoVE 50166 3/09/2013

Brian C. Evans*^1,2, Christopher E. Nelson*^1,2, Shann S. Yu*^1,2, Kelsey R. Beavers^2,3, Arnold J. Kim¹, Hongmei Li^1,2, Heather M. Nelson⁴, Todd D. Giorgio^1,2,5,6, Craig L. Duvall^1,2

¹Department of Biomedical Engineering, Vanderbilt University, ²Vanderbilt Institute for Nanoscale Science & Engineering, Vanderbilt University, ³Interdisciplinary Materials Science Program, Vanderbilt University, ⁴Monroe Carell Jr. Children's Hospital, Vanderbilt University Medical Center, ⁵Department of Chemical & Biomolecular Engineering, Vanderbilt University, ⁶Department of Cancer Biology, Vanderbilt University

A hemolysis assay can be used as a rapid, high-throughput screen of drug delivery systems' cytocompatibility and endosomolytic activity for intracellular cargo delivery. The assay measures the disruption of erythrocyte membranes as a function of environmental pH.

Dopamine Release at Individual Presynaptic Terminals Visualized with FFNs

JoVE 1562 8/31/2009

Hui Zhang^1,2, Niko G. Gubernator^3,4, Minerva Yue¹, Roland G. W. Staal¹, Eugene V. Mosharov¹, Daniela Pereira¹, Vojtech Balsanek³, Paul A. Vadola³, Bipasha Mukherjee⁵, Robert H. Edwards⁵, David Sulzer^1,2,6, Dalibor Sames³

¹Departments of Neurology, Columbia University, ²Departments of Psychiatry and Pharmacology, Columbia University, ³Department of Chemistry, Columbia University, ⁴eMolecules, Inc., ⁵Departments of Neurology and Physiology, University of California School of Medicine, San Francisco, ⁶Division of Molecular Therapeutics, New York Psychiatric Institute

A new means to measure neurotransmission optically using fluorescent dopamine analogs.

Live-cell Video Microscopy of Fungal Pathogen Phagocytosis

JoVE 50196 1/09/2013

Leanne E. Lewis¹, Judith M. Bain¹, Blessing Okai¹, Neil A.R. Gow², Lars Peter Erwig^1,2

¹Division of Applied Medicine, University of Aberdeen, ²Aberdeen Fungal Group, University of Aberdeen

We describe methods for live-cell video microscopy of Candida albicans phagocytosis by macrophages. These methods enable stage-specific analysis of macrophage migration, recognition, engulfment and phagosome maturation and reveal novel aspects of phagocytosis.

Postsynaptic Recordings at Afferent Dendrites Contacting Cochlear Inner Hair Cells: Monitoring Multivesicular Release at a Ribbon Synapse

JoVE 2442 2/10/2011

Lisa Grant*¹, Eunyoung Yi*¹, Juan D. Goutman², Elisabeth Glowatzki¹

¹Department of Otolaryngology-Head and Neck Surgery., The Johns Hopkins School of Medicine, ²Instituto de Investigaciones en Ingeniería Genética y Biología Molecular, Consejo Nacional de Investigaciones Científicas y Técnicas

Whole-cell patch-clamp recordings from auditory nerve fiber dendrites at the inner hair cell ribbon synapse in the mammalian cochlea.

Determining Genetic Expression Profiles in C. elegans Using Microarray and Real-time PCR

JoVE 2777 7/30/2011

Kassandra L. Guthmueller, Maggie L. Yoder, Andrea M. Holgado

Department of Biological Sciences, Southwestern Oklahoma State University

Microarray analysis was conducted to determine genetic expression profiles in C. elegans, and real-time PCR was used to validate and quantify microarray data.

Transurethral Induction of Mouse Urinary Tract Infection

JoVE 2070 8/05/2010

Kim H. Thai¹, Anuradha Thathireddy², Michael H. Hsieh²

¹Earth Systems Program, School of Earth Sciences, Stanford University, ²Department of Urology, Stanford University School of Medicine

This video will demonstrate methods to transurethrally induce mouse urinary tract infections and quantify the extent of resulting infections.

Electrophysiological Recording in the Drosophila Embryo

JoVE 1348 5/21/2009

Kaiyun Chen¹, David E. Featherstone¹, Kendal Broadie²

¹Department of Biological Sciences, University of Illinois, ²Department of Biological Sciences, Vanderbilt University

Electrophysiological recordings from Drosophila embryos allow analyses of developing muscle and neuron electrical properties, as well as characterization of functional synaptogenesis at the glutamatergic neuromuscular junction and central cholinergic and GABAergic synapses.

Preparation of Developing and Adult Drosophila Brains and Retinae for Live Imaging

JoVE 1936 3/15/2010

W. Ryan Williamson, P. Robin Hiesinger

Department of Physiology and Green Center for Systems Biology, University of Texas Southwestern Medical Center

This protocol describes three Drosophila preparations: 1) adult brain dissection, 2) adult retina dissection and 3) developing eye disc- brain complexes dissection. Emphasis is laid on special preparation techniques and conditions for live imaging, although all preparations can be used for fixed tissue immunohistochemistry.

Patch Clamp Recordings in Inner Ear Hair Cells Isolated from Zebrafish

JoVE 4281 10/17/2012

Rachel Einarsson, Marshall Haden, Gabrielle DiCiolli, Andrea Lim, Kolina Mah-Ginn, Kathleen Aguilar, Lucy Yazejian, Bruce Yazejian

Natural Science Division, Pepperdine University

The purpose of this video is to demonstrate procedures for obtaining healthy, intact hair cells from the inner ear organs of adult zebrafish and then using them for patch clamp studies aimed at characterizing the biophysical properties of their voltage-gated channels.

Analysis of SNARE-mediated Membrane Fusion Using an Enzymatic Cell Fusion Assay

JoVE 4378 10/19/2012

Nazarul Hasan, David Humphrey, Krista Riggs, Chuan Hu

Department of Biochemistry and Molecular Biology, University of Louisville School of Medicine

We have developed a cell fusion assay that quantifies SNARE-mediated membrane fusion events by activated expression of β-galactosidase.

Harvesting and Preparing Drosophila Embryos for Electrophysiological Recording and Other Procedures

JoVE 1347 5/20/2009

David E. Featherstone¹, Kaiyun Chen¹, Kendal Broadie²

¹Department of Biological Sciences, University of Illinois, ²Department of Biological Sciences, Vanderbilt University

This technique exposes the Drosophila embryonic neuromusculature for immunohistochemistry or electrophysiological recording. It is useful for studying early events in neuromuscular development or performing electrophysiology in mutants that cannot hatch.

Vibrodissociation of Neurons from Rodent Brain Slices to Study Synaptic Transmission and Image Presynaptic Terminals

JoVE 2752 5/25/2011

Sang Beom Jun^1,2, Verginia Cuzon Carlson¹, Stephen Ikeda³, David Lovinger¹

¹Section on Synaptic Pharmacology/Laboratory for Integrative Neuroscience, National Institutes of Health/National Institute on Alcohol Abuse and Alcoholism, ²Department of Electronics Engineering, Ewha Womans University, ³Section on Transmitter Signaling/Laboratory of Molecular Physiology, National Institutes of Health/National Institute on Alcohol Abuse and Alcoholism

This report demonstrates a technique for mechanical isolation of individual viable neurons retaining attached presynaptic boutons. Vibrodissociated neurons have the advantages of rapid production, excellent pharmacological control and improved space-clamp without influence from neighboring cells. This method can be used for imaging of synaptic elements and patch-clamp recording.

Imaging pHluorin-tagged Receptor Insertion to the Plasma Membrane in Primary Cultured Mouse Neurons

JoVE 4450 11/20/2012

Yun Li, Brittany D. Roy, Wei Wang, Lifeng Zhang, Stephen B. Sampson, Da-Ting Lin

The Jackson Laboratory

By tagging the extracellular domains of membrane receptors with superecliptic pHluorin, and by imaging these fusion receptors in cultured mouse neurons, we can directly visualize individual vesicular insertion events of the receptors to the plasma membrane. This technique will be instrumental in elucidating the molecular mechanisms governing receptor insertion to the plasma membrane.

Gene Transfer to the Developing Mouse Inner Ear by In Vivo Electroporation

JoVE 3653 6/30/2012

Lingyan Wang, Han Jiang, John V. Brigande

Oregon Hearing Research Center, Oregon Health & Science University

The mouse inner ear is a placode-derived sensory organ whose developmental program is elaborated during gestation. We define an in utero gene transfer technique consisting of three steps: mouse ventral laparotomy, transuterine microinjection, and in vivo electroporation. We use digital video microscopy to demonstrate the critical experimental embryological techniques.

Imaging C. elegans Embryos using an Epifluorescent Microscope and Open Source Software

JoVE 2625 3/24/2011

Koen J. C. Verbrugghe, Raymond C. Chan

Human Genetics, University of Michigan

The C. elegans embryo is a powerful system for studying cell biology and development. We present a protocol for live imaging of C. elegans embryos utilizing DIC optics or fluorescence using readily available epifluorescent microscopes and open-source software.

Imaging Cell Shape Change in Living Drosophila Embryos

JoVE 2503 3/30/2011

Lauren Figard¹, Anna Marie Sokac^1,2

¹Program in Cell & Molecular Biology, Baylor College of Medicine (BCM), ²Verna & Marrs McLean Department of Biochemistry & Molecular Biology, Baylor College of Medicine (BCM)

Early development of the fruit fly, Drosophila melanogaster, is characterized by a number of cell shape changes that are well suited for imaging approaches. This article will describe basic tools and methods required for live confocal imaging of Drosophila embryos, and will focus on a cell shape change called cellularization.

Constant Pressure-controlled Extrusion Method for the Preparation of Nano-sized Lipid Vesicles

JoVE 4151 6/22/2012

Leslie A. Morton*^1,2, Jonel P. Saludes*^1,2, Hang Yin^1,2

¹Department of Chemistry & Biochemistry, University of Colorado Boulder, ²Biofrontiers Institute, University of Colorado Boulder

This protocol describes an extrusion method for preparing lipid vesicles of sub-micron sizes with a high degree of homogeneity. This method uses a pressure-controlled system with controlled nitrogen flow rates for liposome preparation. The lipid preparation^1,2, liposome extrusion, and size characterization will be presented herein.

A Genetic Screen to Isolate Toxoplasma gondii Host-cell Egress Mutants

JoVE 3807 2/08/2012

Bradley I. Coleman, Marc-Jan Gubbels

Department of Biology, Boston College

Forward genetics is a powerful method to unravel the molecular level of how Toxoplasma egresses from its host cell. Protocols are provided to chemically mutagenize parasites, enrich for mutants with defects in induced egress, and validate the phenotype of cloned mutants.

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