Seven Steps to Stellate Cells

JoVE 2710 5/10/2011

Patrick Maschmeyer, Melanie Flach, Florian Winau

Immune Disease Institute, Program in Cellular and Molecular Medicine at Children's Hospital, Department of Pathology, Harvard Medical School

Here we describe a method for the isolation of hepatic stellate cells from mouse liver. For stellate cell purification, mouse livers are digested in situ and in vitro by pronase-collagenase treatment prior to density gradient centrifugation. This technique yields highly pure hepatic stellate cells.

May 2011: This Month in JoVE

JoVE 3449 5/04/2011

Aaron Kolski-Andreaco

The main highlights for our May issue include methods for measuring cognition in zero gravity, isolating mosquito immune cells, engineering recombinant SARS vaccines, and detecting tumors with thermal imaging. In addition, procedures for isolating neural stem cells from human fetal brain and culturing antigen-presenting liver cells will also be released.

Preparation of Parasagittal Slices for the Investigation of Dorsal-ventral Organization of the Rodent Medial Entorhinal Cortex

JoVE 3802 3/28/2012

Hugh Pastoll¹, Melanie White², Matthew Nolan²

¹Neuroinformatics DTC, University of Edinburgh, ²Centre for Integrative Physiology, University of Edinburgh

We describe procedures for preparation and electrophysiological recording from brain slices that maintain the dorsal-ventral axis of the medial entorhinal cortex (MEC). Because neural encoding of location follows a dorsal-ventral organization within the MEC, these procedures facilitate investigation of cellular mechanisms important for navigation and memory.

Isolation of Rat Portal Fibroblasts by In situ Liver Perfusion

JoVE 3669 6/29/2012

Jessica W. Wen¹, Abby L. Olsen², Maryna Perepelyuk², Rebecca G. Wells²

¹Division of Gastroenterology, Hepatology & Nutrition, Department of Pediatrics, The Children's Hospital of Philadelphia, ²Department of Medicine, University of Pennsylvania

A technique for isolating portal fibroblasts from rat liver is described. Livers are perfused and digested in situ with collagenase, followed by ex vivo digestion of the liver slurry and size selection of cells. This method provides a pure population of portal fibroblasts without the need for passage in culture.

In vivo Liver Endocytosis Followed by Purification of Liver Cells by Liver Perfusion

JoVE 3138 11/10/2011

Sandhya Gopalakrishnan, Edward N. Harris

Department of Biochemistry, University of Nebraska, Lincoln

The study of liver sinusoidal endothelial cells (SECs) must be performed with primary cells obtained from the animal as no cell lines exist. This method relies on liver digestion and differential centrifugation for SEC purification for subsequent culturing and experimentation.

Isolation of CD133+ Liver Stem Cells for Clonal Expansion

JoVE 3183 10/10/2011

C. Bart Rountree¹, Wei Ding¹, Hein Dang¹, Colleen VanKirk², Gay M. Crooks³

¹Department of Pediatrics and Pharmacology, Pennsylvania State College of Medicine, ²Department of Pharmacology, Pennsylvania State College of Medicine, ³Department of Pediatrics, University of California Los Angeles, School of Medicine

Here we describe the isolation of CD133 expressing liver stem cells and cancer stem cells from whole murine liver, a process that requires tissue digestion, cell enrichment, and flow cytometry isolation. We include methods for advanced single cell isolation and clonal expansion.

Mouse Epidermal Neural Crest Stem Cell (EPI-NCSC) Cultures

JoVE 772 5/09/2008

Maya Sieber-Blum^1,2, Yaofei Hu²

¹Institute of Human Genetics and Northeast England Stem Cell Institute, Newcastle University, ²Department of Cell Biology, Neurobiology and Anatomy, Medical College of Wisconsin

Here we show our method to isolate mouse epidermal neural crest stem cells (EPI-NCSC). Technique involves micro-dissecting whisker follicles, isolating the bulge and placeing it into tissue culture. EPI-NCSC start to emigrate from bulge explants onto the substratum within 3 - 4 days.

Isolation and Culture of Mouse Cortical Astrocytes

JoVE 50079 1/19/2013

Sebastian Schildge¹, Christian Bohrer¹, Kristina Beck², Christian Schachtrup¹

¹Institute of Anatomy and Cell Biology, University of Freiburg, ²Centre of Chronic Immunodeficiency (CCI), University Medical Centre Freiburg, University of Freiburg

Astrocytes have been recognized to be versatile cells participating in fundamental biological processes that are essential for normal brain development and function, and central nervous system repair. Here we present a rapid procedure to obtain pure mouse astrocyte cultures to study the biology of this major class of central nervous system cells.

The CYP2D6 Animal Model: How to Induce Autoimmune Hepatitis in Mice

JoVE 3644 2/03/2012

Edith Hintermann, Janine Ehser, Urs Christen

Pharmazentrum Frankfurt / ZAFES, Goethe University Hospital Frankfurt

Infection of mice with an Adenovirus expressing the major human autoantigen cytochrome P450 2D6 (hCYP2D6) recognized by sera of patients suffering from type 2 autoimmune hepatitis results in a persistent form of autoimmune-mediated liver disease characterized by extensive hepatitis, fibrosis and generation of a CYP2D6-specific immune response.

Dual Electrophysiological Recordings of Synaptically-evoked Astroglial and Neuronal Responses in Acute Hippocampal Slices

JoVE 4418 11/26/2012

Ulrike Pannasch*¹, Jérémie Sibille*^1,2, Nathalie Rouach¹

¹Neuroglial Interactions in Cerebral Physiopathology, Center for Interdisciplinary Research in Biology, CNRS UMR 7241, INSERM U1050, Collège de France, ²Paris Diderot University

The preparation of acute brain slices from isolated hippocampi, as well as the simultaneous electrophysiological recordings of astrocytes and neurons in stratum radiatum during stimulation of schaffer collaterals is described. The pharmacological isolation of astroglial potassium and glutamate transporter currents is demonstrated.

Optic Nerve Transection: A Model of Adult Neuron Apoptosis in the Central Nervous System

JoVE 2241 5/12/2011

Mark M. Magharious*, Philippe M. D'Onofrio*, Paulo D. Koeberle

Department of Surgery, University of Toronto

Optic Nerve transection is a widely used model of adult CNS injury. Ninety percent of retinal ganglion cells (RGCs) whose axons are completely transected (axotomy) die within 14 days after axotomy. This model is easily amenable to experimental manipulations and highly reproducible.

Patterning Cells on Optically Transparent Indium Tin Oxide Electrodes

JoVE 259 8/20/2007

Sunny Shah, Alexander Revzin

Department of Biomedical Engineering, University of California, Davis

Non-fouling PEG silane monolayer was desorbed from individually addressable ITO electrodes on glass by application of a reductive potential. Electrochemical stripping of PEG-silane layer from ITO microelectrodes allowed for cell adhesion to take place in a spatially defined fashion, with cellular patterns corresponding closely to electrode patterns.

Dechorionation of Medaka Embryos and Cell Transplantation for the Generation of Chimeras

JoVE 2055 12/22/2010

Sean R. Porazinski, Huijia Wang, Makoto Furutani-Seiki

Centre for Regenerative Medicine, Department of Biology and Biochemistry, University of Bath

Due to the hard chorion and soft embryos, manipulation of medaka embryos is more involved than in zebrafish. This video shows step-by-step procedures for how to manipulate medaka embryos, including dechorionation, mounting in agarose for imaging and cell transplantation for the production of chimeras. These procedures are essential to use medaka and zebrafish in a laboratory to take full advantage of their complementary features for the genetic dissection of vertebrate genome functions.

An Introduction to Parasitic Wasps of Drosophila and the Antiparasite Immune Response

JoVE 3347 5/07/2012

Chiyedza Small*^1,2, Indira Paddibhatla*^1,2, Roma Rajwani¹, Shubha Govind^1,2

¹Biology Department, The City College of New York, CUNY, ²The Graduate Center, The City University of New York

Parasitoid (parasitic) wasps constitute a major class of natural enemies of many insects including Drosophila melanogaster. We will introduce the techniques to propagate these parasites in Drosophila spp. and demonstrate how to analyze their effects on immune tissues of Drosophila larvae.

Ex Vivo Culture of Patient Tissue & Examination of Gene Delivery

JoVE 2378 12/20/2010

Simon Rajendran¹, Slawomir Salwa¹, Xuefeng Gao², Sabin Tabirca², Deirdre O'Hanlon², Gerald C. O'Sullivan¹, Mark Tangney¹

¹Cork Cancer Research Centre, Mercy University Hospital and Leslie C. Quick Jnr. Laboratory, University College Cork, ²Department of Computer Science, University College Cork

This article describes the culture of patient tissue slices for gene delivery studies and subsequent analysis of gene expression using IVIS bioluminescence imaging.

An Explant Assay for Assessing Cellular Behavior of the Cranial Mesenchyme

JoVE 4245 1/20/2013

Anjali A. Sarkar, Irene E. Zohn

Center for Neuroscience Research, Children's Research Institute, Children's National Medical Center

The cranial mesenchyme undergoes dramatic morphogenic movements that likely provides a driving force for elevation of the neural folds^1,2. Here we describe a simple ex vivo explant assay to characterize the cellular behaviors of the cranial mesenchyme during neurulation. This assay has numerous applications including being amenable to pharmacological manipulations and live imaging analyses.