Real-time Imaging of Leukotriene B₄ Mediated Cell Migration and BLT1 Interactions with β-arrestin

JoVE 2315 12/23/2010

Venkatakrishna R. Jala, Bodduluri Haribabu

Microbiology and Immunology, James Graham Brown Cancer Center, University of Louisville

This paper describes the methodology to determine the chemotactic response of leukocytes to specific ligands and identify interactions between the cell surface receptors and cytosolic proteins using live cell imaging techniques.

Creating Adhesive and Soluble Gradients for Imaging Cell Migration with Fluorescence Microscopy

JoVE 50310 4/04/2013

Siti Hawa Ngalim¹, Astrid Magenau¹, Ying Zhu², Lotte Tønnesen¹, Zoe Fairjones¹, J. Justin Gooding², Till Böcking¹, Katharina Gaus¹

¹Centre for Vascular Research and Australian Centre for Nanomedicine, The University of New South Wales, ²School of Chemistry and Australian Centre for Nanomedicine, The University of New South Wales

A method for the assembly of adhesive and soluble gradients in a microscopy chamber for live cell migration studies is described. The engineered environment combines antifouling surfaces and adhesive tracks with solution gradients and therefore allows one to determine the relative importance of guidance cues.

Analysis of Schwann-astrocyte Interactions Using In Vitro Assays

JoVE 2214 1/13/2011

Fardad T. Afshari, Jessica C. Kwok, James W. Fawcett

Cambridge Centre for Brain Repair, Department of Clinical Neurosciences, University of Cambridge

This article intends to describe in stepwise fashion the commonly used in vitro assays used in studying Schwann cell-asrtocyte interactions.

Quantitative Analysis of Random Migration of Cells Using Time-lapse Video Microscopy

JoVE 3585 5/13/2012

Prachi Jain¹, Rebecca A. Worthylake², Suresh K. Alahari^1,3

¹Department of Biochemistry and Molecular Biology, LSU School of Medicine, ²Department of Oral Biology, LSU School of Dentistry, ³Stanley S. Scott Cancer Center, LSU School of Medicine

This method allows monitoring of cells in real time and quantitative measurements of different cell migration parameters such as speed, displacement, and velocity. Unlike the traditional methods, this real time approach is not based on endpoint quantitative migration measurements; instead it allows monitoring and calculating different parameters continuously.

Monitoring Dendritic Cell Migration using ¹⁹F / ¹H Magnetic Resonance Imaging

JoVE 50251 3/20/2013

Helmar Waiczies^1,2, Martin Guenther^1,2, Julia Skodowski^1,2, Stefano Lepore^1,2, Andreas Pohlmann², Thoralf Niendorf^1,2, Sonia Waiczies^1,2

¹Experimental and Clinical Research Center, A joint cooperation between the Charité Medical Faculty and the Max Delbrück Center for Molecular Medicine, ²Berlin Ultrahigh Field Facility (B.U.F.F.), Max Delbrück Center for Molecular Medicine

Tracking of cells using MRI has gained remarkable attention in the past years. This protocol describes the labeling of dendritic cells with fluorine (¹⁹F)-rich particles, the in vivo application of these cells, and monitoring the extent of their migration to the draining lymph node with ¹⁹F/¹H MRI and ¹⁹F MRS.

Competitive Homing Assays to Study Gut-tropic T Cell Migration

JoVE 2619 3/01/2011

Eduardo J. Villablanca, J. Rodrigo Mora

Gastrointestinal Unit, Massachusetts General Hospital, Harvard Medical School

Competitive homing experiments allow to directly assessing the migratory properties of two different cell populations in a single mouse. Here we illustrate this procedure by comparing the migration of ex vivo-generated gut-tropic versus non-gut tropic T cells.

An In vitro FluoroBlok Tumor Invasion Assay

JoVE 1475 7/20/2009

Jeff Partridge, Paula Flaherty

BD Biosciences, Discovery Labware

This video demonstrates how to measure cell invasion through cell culture inserts using a fluorescence-based methodology.

JoVE 7th Issue

JoVE 274 8/30/2007

Transplantation of Cells Directly into the Kidney of Adult Zebrafish

JoVE 2725 5/18/2011

Cuong Q. Diep, Alan J. Davidson

Center for Regenerative Medicine, Massachusetts General Hospital

Cell transplantation is an essential technique for studying tissue regeneration and for developing cell-based therapies of disease. We demonstrate here a microsurgical technique that permits the transplantation of genetically labeled cells directly into the kidney of adult zebrafish fish.

Evaluation of Cancer Stem Cell Migration Using Compartmentalizing Microfluidic Devices and Live Cell Imaging

JoVE 3297 12/23/2011

Yu Huang*^1,2, Basheal Agrawal*³, Paul A. Clark³, Justin C. Williams^1,2,3, John S. Kuo^3,4

¹Department of Biomedical Engineering, University of Wisconsin-Madison, ²Materials Science Program, University of Wisconsin-Madison, ³Department of Neurological Surgery, University of Wisconsin-Madison, ⁴Carbone Comprehensive Cancer Center and Center for Stem Cell and Regenerative Medicine, University of Wisconsin-Madison

A compartmentalizing microfluidic device for investigating cancer stem cell migration is described. This novel platform creates a viable cellular microenvironment and enables microscopic visualization of live cell locomotion. Highly motile cancer cells are isolated to study molecular mechanisms of aggressive infiltration, potentially leading to more effective future therapies.

Live Imaging Of Drosophila melanogaster Embryonic Hemocyte Migrations

JoVE 1696 2/12/2010

Iwan R. Evans¹, Jennifer Zanet², Will Wood¹, Brian M. Stramer²

¹Department of Biology and Biochemistry, University of Bath, ²Randall Division of Cell and Molecular Biophysics, King's College London

Drosophila hemocytes disperse over the entirety of the developing embryo. This protocol demonstrates how to mount and image these migrations using embryos with fluorescently labelled hemocytes.

Time-lapse Imaging of Neuroblast Migration in Acute Slices of the Adult Mouse Forebrain

JoVE 4061 9/12/2012

Jivan Khlghatyan, Armen Saghatelyan

The Cellular Neurobiology Unit, Centre de Recherche Université Laval Robert-Giffard

We describe a protocol for real-time videoimaging of neuronal migration in the mouse forebrain. The migration of virally-labeled or grafted neuronal precursors was recorded in acute live slices using wide-field fluorescent imaging with a relatively rapid acquisition interval to study the different phases of cell migration, including the durations of the stationary and migration phases and the speed of migration.

Matrix-assisted Autologous Chondrocyte Transplantation for Remodeling and Repair of Chondral Defects in a Rabbit Model

JoVE 4422 5/21/2013

Markus T. Berninger^1,2, Gabriele Wexel³, Ernst J. Rummeny², Andreas B. Imhoff¹, Martina Anton³, Tobias D. Henning*^2,4, Stephan Vogt*¹

¹Department of Orthopaedic Sports Medicine, Klinikum rechts der Isar der Technischen Universität München, ²Department of Radiology, Klinikum rechts der Isar der Technischen Universität München, ³Institute of Experimental Oncology and Therapy Research, Klinikum rechts der Isar der Technischen Universität München, ⁴Department of Radiology, Uniklinik Köln

An experimental technique for the treatment of chondral defects in the rabbit's knee joint is described. The implantation of autologous chondrocytes seeded on a matrix is a well-accepted method for the remodeling and repair of articular cartilage lesions providing satisfying long-term results. Matrix-assisted autologous chondrocyte transplantation (MACT) offers a standardized and clinically established implantation method.

Generating Chimeric Zebrafish Embryos by Transplantation

JoVE 1394 7/17/2009

Hilary A. Kemp, Amanda Carmany-Rampey, Cecilia Moens

HHMI and Division of Basic Sciences, Fred Hutchinson Cancer Research Center - FHCRC

A step-by-step guide to generating targeted chimeric zebrafish embryos by transplantation at the blastula or gastrula stage.

Electric Field-controlled Directed Migration of Neural Progenitor Cells in 2D and 3D Environments

JoVE 3453 2/16/2012

Xiaoting Meng*¹, Wenfei Li*^2,3, Fraser Young¹, Runchi Gao³, Laura Chalmers³, Min Zhao³, Bing Song¹

¹School of Dentistry, Cardiff Institute of Tissue Engineering & Repair, Cardiff University, ²Shandong Qianfoshan Hospital, Shandong University School of Medicine, ³Dermatology and Ophthalmology Research, Institute for Regenerative Cures, University of California at Davis

This protocol demonstrates methods used to establish 2D and 3D environments in custom-designed electrotactic chambers, which can track cells in vivo/ex vivo using time-lapse recording at the single cell level, in order to investigate galvanotaxis/electrotaxis and other cellular responses to direct current (DC) electric fields (EFs).

Analyzing Murine Schwann Cell Development Along Growing Axons

JoVE 50016 11/21/2012

Stephan Heermann^1,2, Kerstin Krieglstein^1,3

¹Department of Molecular Embryology, Institute of Anatomy and Cell Biology, University of Freiburg, ²Department of Neuroanatomy, University of Heidelberg, ³FRIAS, University of Freiburg

Here we describe a Schwann cell (SC) migration assay in which SCs are able to develop along extending axons.

September 2012: This Month in JoVE

JoVE 5022 9/01/2012

Wendy Chao¹, Aaron Kolski-Andreaco²

¹Department of Ophthalmology, Massachusetts Eye and Ear, ²JoVE Content Production

This September in JoVE, researchers from the School of Medicine at the Free University of Berlin demonstrate a novel method for studying how stroke patients compensate for visual field defects. To do this, our authors make use of a driving simulator complete with brakes, a steering wheel, and turn signals. Using driving simulation software and sophisticated eye tracking, researchers can compare the gaze behavior of stroke patients as they navigate through virtual driving courses with varying degrees of complexity. Though posterior cerebral artery infarction can lead to similar visual deficits in patients, some are able to navigate through the driving courses by developing compensatory eye movements, while others crash into dangerous obstacles, like wild boars. Through the analysis of compensatory gaze behavior employed by patients, our authors see great potential for using driving simulation as a tool to rehabilitate stroke patients trying to overcome the blind spots in their visual fields.

Ex vivo Imaging of T Cells in Murine Lymph Node Slices with Widefield and Confocal Microscopes

JoVE 3054 7/15/2011

Hélène Salmon^1,2, Ana Rivas-Caicedo^1,2, François Asperti-Boursin^1,2, Camille Lebugle^1,2, Pierre Bourdoncle^1,2, Emmanuel Donnadieu^1,2

¹Institut Cochin, Université Paris Descartes, CNRS (UMR 8104), ²Inserm, U1016, Paris, France

This protocol describes a method to image fluorescent T cells introduced into lymph node slices. The technique permits real-time analyses of T cell migration with traditional widefield fluorescence or confocal microscopes.

January 2012: This Month in JoVE

JoVE 4194 1/02/2012

Aaron Kolski-Andreaco

Here are some highlights from the January 2012 Issue of Journal of Visualized Experiments (JoVE).

Multimodal Imaging of Stem Cell Implantation in the Central Nervous System of Mice

JoVE 3906 6/13/2012

Nathalie De Vocht^1,2, Kristien Reekmans¹, Irene Bergwerf², Jelle Praet^1,2, Chloé Hoornaert¹, Debbie Le Blon¹, Jasmijn Daans¹, Zwi Berneman¹, Annemie Van der Linden², Peter Ponsaerts¹

¹Laboratory of Experimental Hematology, University of Antwerp, ²Bio Imaging Lab, University of Antwerp

This article describes an optimized sequence of events for multimodal imaging of cellular grafts in rodent brain using: (i) in vivo bioluminescence and magnetic resonance imaging, and (ii) post mortem histological analysis. Combining these imaging modalities on a single animal allows cellular graft evaluation with high resolution, sensitivity and specificity.

Adult and Embryonic Skeletal Muscle Microexplant Culture and Isolation of Skeletal Muscle Stem Cells

JoVE 2051 9/21/2010

Deborah Merrick, Hung-Chih Chen, Dean Larner, Janet Smith

School of Biosciences, University of Birmingham

The micro-dissected explants technique is a robust and reliable method for isolating proliferative skeletal muscle cells from juvenile, adult or embryonic muscles as a source of skeletal muscle stem cells. Uniquely, these cells have been clonally derived to produce skeletal muscle stem cell lines used for in vivo transplantation.

Modeling and Imaging 3-Dimensional Collective Cell Invasion

JoVE 3525 12/07/2011

Rebecca W. Scott¹, Diane Crighton², Michael F. Olson²

¹Strathclyde Institute for Pharmacy and Biomedical Sciences, University of Strathclyde, ²The Beatson Institute for Cancer Research

Models of tumor cell invasion into three-dimensional extracellular matrix better reflect the in vivo situation than two-dimensional motility assays. Using matrix invasion assays combined with confocal imaging of fluorescently-labeled cells, detailed information on invasion modes and the distinct contributions of leading versus following cells can be obtained.

MAME Models for 4D Live-cell Imaging of Tumor: Microenvironment Interactions that Impact Malignant Progression

JoVE 3661 2/17/2012

Mansoureh Sameni¹, Arulselvi Anbalagan¹, Mary B. Olive¹, Kamiar Moin^1,2, Raymond R. Mattingly^1,2, Bonnie F. Sloane^1,2

¹Department of Pharmacology, Wayne State University, ²Barbara Ann Karmanos Cancer Institute, Wayne State University

We have developed 3D coculture models for live-cell imaging in real-time of interactions among breast tumor cells and other cells in their microenvironment that impact progression to an invasive phenotype. These models can serve as preclinical screens for drugs to target paracrine-induced proteolytic, chemokine/cytokine and kinase pathways implicated in invasiveness.

A Quantitative Evaluation of Cell Migration by the Phagokinetic Track Motility Assay

JoVE 4165 12/04/2012

Maciej T. Nogalski^1,2, Gary C.T. Chan³, Emily V. Stevenson^1,2, Donna K. Collins-McMillen^1,2, Andrew D. Yurochko^1,2,4

¹Department of Microbiology and Immunology, Louisiana State University Health Sciences Center, ²Center for Molecular and Tumor Virology, Louisiana State University Health Sciences Center, ³Department of Microbiology and Immunology, SUNY Upstate Medical University, ⁴Feist-Weiller Cancer Center, Louisiana State University Health Sciences Center

The phagokinetic motility track assay is a method used to assess the movement of cells. Specifically, the assay measures chemokinesis (random cell motility) over time in a quantitative manner. The assay takes advantage of the ability of cells to create a measurable track of their movement on colloidal gold-coated coverslips.

Processing of Human Reduction Mammoplasty and Mastectomy Tissues for Cell Culture

JoVE 50011 1/03/2013

Mark A. LaBarge, James C. Garbe, Martha R. Stampfer

Life Science Division, Lawrence Berkeley National Laboratory

A method to process human mammary surgical discard material is described. Processed tissue, in the form of organoids, can be stored frozen indefinitely or placed in culture for long-term growth. This method enables experimental examination of normal human epithelial cell biology, and the effects of exogenous perturbations.

July 2011: This Month in JoVE

JoVE 3688 7/01/2011

Aaron Kolski-Andreaco

Here are some highlights from the July 2011 Issue of Journal of Visualized Experiments (JoVE).

Optimized Fibrin Gel Bead Assay for the Study of Angiogenesis

JoVE 186 4/29/2007

Martin N. Nakatsu, Jaeger Davis, Christopher C.W. Hughes

Department of Molecular Biology and Biochemistry, University of California, Irvine (UCI)

This video demonstrates the protocol of an in vitro angiogenesis assay that recapitulates several stages of angiogenesis. Time-lapse images of sprouting, lumen formation, branching and anastomosis - key features of angiogenesis - are shown.

October 2012: This Month in JoVE

JoVE 5025 10/01/2012

Wendy Chao¹, Aaron Kolski-Andreaco²

¹Department of Ophthalmology, Massachusetts Eye and Ear, ²JoVE Content Production

Here are some highlights from the October 2012 Issue of Journal of Visualized Experiments (JoVE).

RhoC GTPase Activation Assay

JoVE 2083 8/22/2010

Michelle Lucey, Heather Unger, Kenneth L. van Golen

Department of Biological Sciences, The Center for Translational Cancer Research, University of Delaware

This protocol utilizes a pull down assay to determine the levels of active RhoC GTPase within cells.

Live Imaging of Glial Cell Migration in the Drosophila Eye Imaginal Disc

JoVE 1155 7/09/2009

Patrick Cafferty, Xiaojun Xie, Kristen Browne, Vanessa J. Auld

Department of Zoology, University of British Columbia - UBC

Here we describe a protocol to examine the migration of glial cells into the developing Drosophila eye using live microscopic analysis paired with GFP tagged glial cells.

December 2011: This Month in JoVE

JoVE 4114 12/01/2011

Aaron Kolski-Andreaco

Here are some highlights from the December 2011 Issue of Journal of Visualized Experiments (JoVE).

Human T Lymphocyte Isolation, Culture and Analysis of Migration In Vitro

JoVE 2017 6/01/2010

Craig T. Lefort, Minsoo Kim

Center for Vaccine Biology and Immunology, University of Rochester

T lymphocyte migration occurs during homing to lymphoid organs, exit from the vasculature, and entering into peripheral tissues. Here, we describe a protocol that can be used to analyze T lymphocyte migration in vitro.

Long-term Culture of Human Breast Cancer Specimens and Their Analysis Using Optical Projection Tomography

JoVE 3085 7/29/2011

Alexander D. Leeper¹, Joanne Farrell², J. Michael Dixon¹, Sarah E. Wedden², David J. Harrison¹, Elad Katz¹

¹Breakthrough Breast Cancer Research Unit, Institute of Genetics and Molecular Medicine, University of Edinburgh, ²MRC Technology

We have developed a collagen-based in vitro assay which promotes proliferation and invasion from samples of all breast cancer subtypes. Optical Projection Tomography, a three dimensional microscopy technique was utilised to visualise and quantify tumour expansion. This assay may be used to quantify drug response of individual tumour samples.

Quantitative Measurement of Invadopodia-mediated Extracellular Matrix Proteolysis in Single and Multicellular Contexts

JoVE 4119 8/27/2012

Karen H. Martin, Karen E. Hayes, Elyse L. Walk, Amanda Gatesman Ammer, Steven M. Markwell, Scott A. Weed

Department of Neurobiology and Anatomy, Program in Cancer Cell Biology, Mary Babb Randolph Cancer Center, West Virginia University

We describe the prototypical method for producing microscope coverslips coated with fluorescent gelatin for visualizing invadopodia-mediated matrix degradation. Computational techniques using available software are presented for quantifying the resultant levels of matrix proteolysis by single cells within a mixed population and for multicellular groups encompassing entire microscopic fields.

Generation and Labeling of Murine Bone Marrow-derived Dendritic Cells with Qdot Nanocrystals for Tracking Studies

JoVE 2785 6/02/2011

Maria Muccioli*¹, Michelle Pate*², Omowaleola Omosebi², Fabian Benencia^1,2,3

¹Molecular and Cell Biology Program, Ohio University, ²Department of Biomedical Sciences, College of Osteopathic Medicine, Ohio University, ³Department of Biomedical Engineering, Russ College of Engineering and Technology, Ohio University

Dendritic cells uptake antigens and migrate towards immune organs to present processed antigens to T cells. Qdot nanocrystal labeling provides a long-lasting and stable fluorescent signal. This allows tracking of dendritic cells to different organs by fluorescent microscopy.

Cell Co-culture Patterning Using Aqueous Two-phase Systems

JoVE 50304 3/26/2013

John P. Frampton¹, Joshua B. White¹, Abin T. Abraham¹, Shuichi Takayama^1,2

¹Department of Biomedical Engineering, University of Michigan, ²Department of Macromolecular Science and Engineering, University of Michigan

Aqueous two-phase systems were used to simultaneously pattern multiple populations of cells. This fast and easy method for cell patterning takes advantage of the phase separation of aqueous solutions of dextran and polyethylene glycol and the interfacial tension that exists between the two polymer solutions.

Quantitative Analysis of Cancer Metastasis using an Avian Embryo Model

JoVE 2815 5/30/2011

Trenis D. Palmer¹, John Lewis², Andries Zijlstra¹

¹Department of Pathology, Vanderbilt University, ²Departments of Oncology, Surgery and Medical Biophysics, London Regional cancer program

Using quantitative PCR, we demonstrate how the well-established chick CAM model can be used to quantitatively analyze the metastasis of human tumor cells to distant organs.

In vivo Dual Substrate Bioluminescent Imaging

JoVE 3245 10/11/2011

Michael K. Wendt, Joseph Molter, Christopher A. Flask, William P. Schiemann

Case Comprehensive Cancer Center, Case Western Reserve University

Herein we describe the methods to construct, visualize, and quantify the bioluminescent reactions of both firefly and renilla luciferase enzymes expressed in metastatic breast cancer cells during their growth and metastasis in vivo.

Isolation of Mammary Epithelial Cells from Three-dimensional Mixed-cell Spheroid Co-culture

JoVE 3760 4/30/2012

Kun Xu, Rachel J. Buchsbaum

Molecular Oncology Research Institute, Department of Medicine, Tufts Medical Center

A simple method is described for analyzing effects of tissue fibroblasts on associated epithelial cells. The combination of this method and three-dimensional tissue culture can facilitate analysis of cells after isolation from 3D. The technique is applicable to cells of varying malignant potential, allowing systematic study of effects of tumor-associated stroma on tumor cells.

A Galvanotaxis Assay for Analysis of Neural Precursor Cell Migration Kinetics in an Externally Applied Direct Current Electric Field

JoVE 4193 10/13/2012

Robart Babona-Pilipos¹, Milos R. Popovic², Cindi M. Morshead³

¹Institute for Biomaterials and Biomedical Engineering, University of Toronto, ²Lyndhurst Centre, Toronto Rehabilitation Institute, ³Department of Surgery, University of Toronto

In this protocol we demonstrate how to construct custom chambers that permit the application of a direct current electric field to enable time-lapse imaging of adult brain derived neural precursor cell translocation during galvanotaxis.

Assessing Neural Stem Cell Motility Using an Agarose Gel-based Microfluidic Device

JoVE 674 2/11/2008

Kevin Wong¹, Angel Ayuso-Sacido^2,3, Patrick Ahyow¹, Andrew Darling⁴, John A. Boockvar², Mingming Wu⁴

¹Biomedical Engineering Department, Cornell University, ²Neurosurgical Laboratory for Translational Stem Cell Research, Weill Cornell Brain Tumor Center, Weill Cornell Medical College of Cornell University, ³Cell Morphology Department, Instituto de Investigacion Principe Felipe, ⁴Department of Chemical and Biomolecular Engineering, Cornell University

We demonstrate that the over expression of epidermal growth factor receptors (EGFR) enhances the motility of neural stem cells(NSCs) using a novel agarose gel based microfluidic device. This technology can be readily adaptable to other mammalian cell systems where cell sources are scarce, such as human neural stem cells, and the turn around time is critical.

Primary Human Bronchial Epithelial Cells Grown from Explants

JoVE 1789 3/26/2010

Asma Yaghi, Aisha Zaman, Myrna Dolovich

Medicine, Faculty of Health Sciences, McMaster University

Here we describe a detailed method for growing primary human bronchial epithelial cells from explants of human bronchial airway tissue including differentiated growth on an air-liquid interface. This method provides an abundant source of primary cells for investigating the role of the airway epithelium in human lung health and disease.

Non-surgical Intratracheal Instillation of Mice with Analysis of Lungs and Lung Draining Lymph Nodes by Flow Cytometry

JoVE 2702 5/02/2011

Manira Rayamajhi¹, Elizabeth F. Redente², Tracy V. Condon¹, Mercedes Gonzalez-Juarrero³, David W.H. Riches^1,2,4, Laurel L. Lenz^1,4

¹Department of Immunology, University of Colorado School of Medicine, ²Division of Cell Biology, Department of Pediatrics, National Jewish Health, ³Department of Microbiology, Immunology, and Pathology, Colorado State University, ⁴Department of Immunology, National Jewish Health

We illustrate non-surgical delivery of test materials into the lungs of anesthetized mice via the trachea. This method permits lung exposure to bacterial and viral pathogens, cytokines, antibodies, beads, chemicals, or dyes. We further describe harvesting and processing of lungs and lung draining lymph nodes (LDLNs) for flow cytometry.

A Microfluidic Device for Quantifying Bacterial Chemotaxis in Stable Concentration Gradients

JoVE 1779 4/19/2010

Derek L. Englert¹, Michael D. Manson², Arul Jayaraman^1,3

¹McFerrin Department of Chemical Engineering, Texas A&M University, ²Department of Biology, Texas A&M University, ³Department of Biomedical Engineering, Texas A&M University

This protocol describes the development of a microfluidic device for investigating bacterial chemotaxis in stable concentration gradients of chemoeffectors.

Analysis of Pulmonary Dendritic Cell Maturation and Migration during Allergic Airway Inflammation

JoVE 4014 7/23/2012

Rahul Kushwah¹, Jim Hu²

¹Stem Cell and Cancer Research Institute, McMaster University, Hamilton, ²Physiology and Experimental Medicine Research Program, Hospital for Sick Children, University of Toronto

We describe a strategy to monitor maturation and migration of pulmonary dendritic cells in response to ovalbumin in the setting of ovalbumin induced allergic airway inflammation. This strategy can be modified to assess migration of pulmonary dendritic cells in settings of infection.

A Cre-Lox P Recombination Approach for the Detection of Cell Fusion In Vivo

JoVE 3581 1/04/2012

Anthony J. Sprangers¹, Brian T. Freeman¹, Nicholas A. Kouris¹, Brenda M. Ogle²

¹Department of Biomedical Engineering, University of Wisconsin-Madison, ²Department of Biomedical Engineering, Materials Science Program, Laboratory for Optical and Computational Instrumentation, University of Wisconsin-Madison

A method to track cell fusion in living organisms over time is described. The approach utilizes Cre-LoxP recombination to induce luciferase expression upon cell fusion. The luminescent signal generated can be detected in living organisms using biophotonic imaging systems with a sensitivity of detection of ˜1,000 cells in peripheral tissues.

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.

Study of the Actin Cytoskeleton in Live Endothelial Cells Expressing GFP-Actin

JoVE 3187 11/18/2011

Travis M. Doggett, Jerome W. Breslin

Department of Physiology, Louisiana State University Health Sciences Center

Microscopic imaging of live endothelial cells expressing GFP-actin allows characterization of dynamic changes in cytoskeletal structures. Unlike techniques that use fixed specimens, this method provides a detailed assessment of temporal changes in the actin cytoskeleton in the same cells before, during, and after various physical, pharmacological, or inflammatory stimuli.

Analysis of Trunk Neural Crest Cell Migration using a Modified Zigmond Chamber Assay

JoVE 3330 1/19/2012

Christopher C. Walheim¹, Juan Pablo Zanin², Maria Elena de Bellard¹

¹Department of Biology, California State University, Northridge, ²Centro de Biología Celular y Molecular, Universidad Nacional de Córdoba

An approach to analyze the migration of explanted cells (trunk neural crest cells) is described. This method is inexpensive, gentle, and capable of distinguishing chemotaxis from both chemokinesis and other influences on migratory polarity such as those derived from cell-cell interactions within the primary trunk neural crest cell culture.

An Analytical Tool that Quantifies Cellular Morphology Changes from Three-dimensional Fluorescence Images

JoVE 4233 8/31/2012

Carolina L. Haass-Koffler^1,2, Mohammad Naeemuddin¹, Selena E. Bartlett^1,3

¹Medications Development, Ernest Gallo Clinic and Research Center, University of California, San Francisco, ²Clinical Pharmacology and Experimental Therapeutics, University of California, San Francisco, ³Translational Research Institute and the Institute for Health and Biomedical Innovation, Queensland University of Technology, Brisbane, Australia

We developed a software platform that utilizes Imaris Neuroscience, ImarisXT and MATLAB to measure the changes in morphology of an undefined shape taken from three-dimensional confocal fluorescence of single cells. This novel approach can be used to quantify changes in cell shape following receptor activation and therefore represents a possible additional tool for drug discovery.