3D Printing of Preclinical X-ray Computed Tomographic Data Sets

JoVE 50250 3/22/2013

Evan Doney¹, Lauren A. Krumdick¹, Justin M. Diener², Connor A. Wathen³, Sarah E. Chapman⁴, Brian Stamile⁵, Jeremiah E. Scott³, Matthew J. Ravosa⁶, Tony Van Avermaete⁴, W. Matthew Leevy^1,4,7

¹Department of Chemistry and Biochemistry, University of Notre Dame, ²Freimann Life Science Center, University of Notre Dame, ³Department of Biological Sciences, University of Notre Dame, ⁴Notre Dame Integrated Imaging Facility, University of Notre Dame, ⁵MakerBot Industries LLC, ⁶Departments of Biological Sciences, Aerospace and Mechanical Engineering, and Anthropology, University of Notre Dame, ⁷Harper Cancer Research Institute, University of Notre Dame

Using modern plastic extrusion and printing technologies, it is now possible to quickly and inexpensively produce physical models of X-ray CT data taken in a laboratory. The three -dimensional printing of tomographic data is a powerful visualization, research, and educational tool that may now be accessed by the preclinical imaging community.

Quantitatively Measuring In situ Flows using a Self-Contained Underwater Velocimetry Apparatus (SCUVA)

JoVE 2615 10/31/2011

Kakani Katija¹, Sean P. Colin^2,3, John H. Costello^3,4, John O. Dabiri⁵

¹Applied Ocean Physics and Engineering, Woods Hole Oceanographic Institution, ²Environmental Science and Marine Biology, Roger Williams University, ³Marine Biology Laboratory, Whitman Center, ⁴Department of Biology, Providence College, ⁵Departments of Aeronautics and Bioengineering, California Institute of Technology

This protocol provides instructions on how to use a self-contained underwater velocimetry apparatus (SCUVA), which is designed for quantification of in situ animal-generated flows. In addition, this protocol addresses challenges posed by field conditions, and includes operator motion, predicting position of animals, and orientation of SCUVA.

Testing Visual Sensitivity to the Speed and Direction of Motion in Lizards

JoVE 127 12/14/2006

Kevin L. Woo

Center for the Integrative Study of Animal Behaviour, Macquarie University

Testing visual sensitivity in lizards using an operant conditioning paradigm that employs video playback of random-dot kinematograms and computer-generated invertebrates.

Obtaining Eggs from Xenopus laevis Females

JoVE 890 8/20/2008

Marie K. Cross, Maureen Powers

Department of Cell Biology, Emory University

The eggs of Xenopus laevis intact, lysed, and/or fractionated are useful for a wide variety of experiments. This protocol shows how to induce egg laying, collect and dejelly the eggs, and sort the eggs to remove any damaged eggs.

Amide Hydrogen/Deuterium Exchange & MALDI-TOF Mass Spectrometry Analysis of Pak2 Activation

JoVE 3602 11/26/2011

Yuan-Hao Hsu¹, Jolinda A. Traugh²

¹Department of Chemistry, Tunghai University, ²Department of Biochemistry, University of California, Riverside

MALDI-TOF mass spectrometry was successfully utilized to monitor the amide hydrogen/deuterium exchange in protein kinase Pak2 activation.

Assessment of Motor Balance and Coordination in Mice using the Balance Beam

JoVE 2376 3/10/2011

Tinh N. Luong*, Holly J. Carlisle*, Amber Southwell, Paul H. Patterson

Department of Biology, California Institute of Technology

Deficits in fine motor coordination can be assessed with the balance beam test. Performance on the beam is quantified by the speed at which the beam is traversed and the number of times the mouse slips on the beam.

Spatio-Temporal Manipulation of Small GTPase Activity at Subcellular Level and on Timescale of Seconds in Living Cells

JoVE 3794 3/09/2012

Robert DeRose¹, Christopher Pohlmeyer¹, Nobuhiro Umeda^1,2, Tasuku Ueno^1,2, Tetsuo Nagano², Scot Kuo^1,3, Takanari Inoue¹

¹Department of Cell Biology, Center for Cell Dynamics, Johns Hopkins University, ²Graduate School of Pharmaceutical Sciences, University of Tokyo, ³Biomedical Engineering, Johns Hopkins University

A method for spatio-temporal control of small GTPase activity by light is described. This method is based on rapamycin-induced FKBP-FRB heterodimerization and photo-caging systems. Optimization of light-irradiation enables the spatio-temporally controlled activation of small GTPases at the subcellular level.

In vitro Reconstitution of the Active T. castaneum Telomerase

JoVE 2799 7/14/2011

Anthony P. Schuller, Michael J. Harkisheimer, Emmanuel Skordalakes

Gene Expression and Regulation, The Wistar Institute, University of Pennsylvania

Efforts to isolate the catalytic subunit of telomerase, TERT, in sufficient quantities for structural studies, have been met with limited success for more than a decade. Here, we present methods for the isolation of the recombinant Tribolium castaneum TERT (TcTERT) and the reconstitution of the active T. castaneum telomerase ribonucleoprotein (RNP) complex in vitro.

Growth Assays to Assess Polyglutamine Toxicity in Yeast

JoVE 3461 3/05/2012

Martin L. Duennwald

Boston Biomedical Research Institute

This manuscript describes three complementary protocols for assessing the toxicity of polyglutamine (polyQ)-expansion proteins in the yeast Saccharomyces cerevisiae. These protocols can easily be modified to monitor the toxicity of other misfolded proteins in yeast.

Protease- and Acid-catalyzed Labeling Workflows Employing ¹⁸O-enriched Water

JoVE 3891 2/20/2013

Diana Klingler, Markus Hardt

Boston Biomedical Research Institute

Stable isotope labeling workflows employing ¹⁸O-enriched water (LeO-workflows) are versatile tools for quantitative and qualitative proteomics studies. In protease-assisted (PALeO) workflows, ¹⁸O-atoms are introduced by proteolytic cleavage and carboxyl oxygen exchange reactions mediated by proteases. In the acid-catalyzed (ALeO) workflow, ¹⁸O-atoms are introduced by carboxyl oxygen exchange at low pH.

Ex vivo Expansion of Tumor-reactive T Cells by Means of Bryostatin 1/Ionomycin and the Common Gamma Chain Cytokines Formulation

JoVE 2381 1/14/2011

Maciej Kmieciak¹, Amir Toor², Laura Graham³, Harry D. Bear³, Masoud H. Manjili¹

¹Department of Microbiology & Immunology, Virginia Commonwealth University- Massey Cancer Center, ²Department of Internal Medicine, Virginia Commonwealth University- Massey Cancer Center, ³Department of Surgery, Virginia Commonwealth University- Massey Cancer Center

An efficient protocol for the ex vivo expansion of tumor-reactive T cells from tumor-draining lymph nodes or other secondary lymphoid tissues of tumor-bearing hosts is described. This protocol selectively expands tumor-specific T cells for use in adoptive immunotherapy of breast cancer.

Affinity Precipitation of Active Rho-GEFs Using a GST-tagged Mutant Rho Protein (GST-RhoA(G17A)) from Epithelial Cell Lysates

JoVE 3932 3/31/2012

Faiza Waheed^1,2, Pamela Speight^1,2, Qinghong Dan^1,2, Rafael Garcia-Mata³, Katalin Szaszi^1,2

¹Keenan Research Centre, Li Ka Shing Knowledge Institute, St. Michael's Hospital, ²Department of Surgery, University of Toronto, ³Department of Cell and Developmental Biology, University of North Carolina at Chapel Hill

The method presented here describes an assay to follow activation of RhoA specific GDP/GTP Exchange Factors (GEFs) in cultured cells by making use of a mutant RhoA GST fusion protein that has high affinity for activated GEFs. GEFs are precipitated from cell lysates, detected by Western blotting and quantified by densitometry.

Orthogonal Protein Purification Facilitated by a Small Bispecific Affinity Tag

JoVE 3370 1/16/2012

Johan Nilvebrant, Tove Alm, Sophia Hober

School of Biotechnology, Department of Proteomics, Royal Institute of Technology

A novel and highly efficient two-step affinity chromatography protocol has been developed and is described in detail. The method is based on a small purification tag with two inherent affinities and is applicable to a wide range of target proteins with different properties.

A Modified EPA Method 1623 that Uses Tangential Flow Hollow-fiber Ultrafiltration and Heat Dissociation Steps to Detect Waterborne Cryptosporidium and Giardia spp.

JoVE 4177 7/09/2012

Eric R. Rhodes¹, Leah Fohl Villegas², Nancy J. Shaw², Carrie Miller³, Eric N. Villegas¹

¹National Exposure Research Laboratory, Office of Research and Development, US Environmental Protection Agency, ²Shaw Environmental & Infrastructure, ³Office of Ground Water and Drinking Water, US Environmental Protection Agency

This protocol describes the use of a tangential flow hollow-fiber ultrafiltration sample concentration system and a heat dissociation as alternative steps for the detection of waterborne Cryptosporidium and Giardia species using EPA Method 1623.

Electrode Positioning and Montage in Transcranial Direct Current Stimulation

JoVE 2744 5/23/2011

Alexandre F. DaSilva¹, Magdalena Sarah Volz^2,3, Marom Bikson⁴, Felipe Fregni²

¹Headache & Orofacial Pain Effort (H.O.P.E.), Biologic & Material Sciences, School of Dentistry, University of Michigan, ²Laboratory of Neuromodulation, Department of Physical Medicine & Rehabilitation, Spaulding Rehabilitation Hospital and Massachusetts General Hospital, Harvard Medical School, ³Charité, University Medicine Berlin, ⁴Department of Biomedical Engineering, The City College of New York

Transcranial direct current stimulation (tDCS) is an established technique to modulate cortical excitability^1,2. It has been used as an investigative tool in neuroscience due to its effects on cortical plasticity, easy operation, and safe profile. One area that tDCS has been showing encouraging results is pain alleviation ^3-5.

Isolation of Human Islets from Partially Pancreatectomized Patients

JoVE 2962 7/30/2011

Gregor Bötticher¹, Dorothèe Sturm¹, Florian Ehehalt¹, Klaus P. Knoch², Stephan Kersting¹, Robert Grützmann¹, Gustavo B. Baretton³, Michele Solimena², Hans D. Saeger¹

¹Department of GI-, Thorax- and Vascular Surgery, University Hospital Carl Gustav Carus, University of Technology Dresden, ²Molecular Diabetology, Paul Langerhans Institute Dresden, ³Department of Pathology, University Hospital Carl Gustav Carus, University of Technology Dresden

The supply of type 2 diabetic islets for research is insufficient. Here we share our protocol for isolating islets from patients undergoing partial pancreatectomy. This approach represents a unique venue for obtaining islets from type 2 diabetic and clinically matched non-diabetic subjects in adequate numbers for basic and clinical studies.

DNA-based Fish Species Identification Protocol

JoVE 1871 4/28/2010

Rachel Formosa, Harini Ravi, Scott Happe, Danielle Huffman, Natalia Novoradovskaya, Robert Kincaid, Steve Garrett

Agilent Technologies

This publication describes how to use the Agilent Fish Species Identification System to identify the species of a fish by extracting DNA and performing PCR and RFLP analysis.

Deciphering Axonal Pathways of Genetically Defined Groups of Neurons in the Chick Neural Tube Utilizing in ovo Electroporation

JoVE 1792 5/02/2010

Oshri Avraham*, Sophie Zisman*, Yoav Hadas, Lilach Vald, Avihu Klar

Department of Medical Neurobiology, Institute for Medical Research Israel Canada, Hebrew University-Hadassah Medical School

This video demonstrates how to visualize axonal pathways of genetically defined groups of neurons in the embryonic chick spinal cord utilizing in ovo electroporation of reporter genes under the control of specific enhancer elements.

Compact Quantum Dots for Single-molecule Imaging

JoVE 4236 10/09/2012

Andrew M. Smith¹, Shuming Nie^1,2

¹Department of Biomedical Engineering, Emory University, ²Department of Chemistry, Georgia Institute of Technology

We describe the preparation of colloidal quantum dots with minimized hydrodynamic size for single-molecule fluorescence imaging. Compared to conventional quantum dots, these nanoparticles are similar in size to globular proteins and are optimized for single-molecule brightness, stability against photodegradation, and resistance to nonspecific binding to proteins and cells.

Efficient Recombinant Parvovirus Production with the Help of Adenovirus-derived Systems

JoVE 3518 4/23/2012

Nazim El-Andaloussi*^1,2, Barbara Leuchs*¹, Serena Bonifati^1,2, Jean Rommelaere^1,2, Antonio Marchini^1,2

¹Tumour Virology Division F010, German Cancer Research Center (DKFZ), ²Inserm Unit 701, German Cancer Research Center (DKFZ)

Here we describe a protocol based only on cell infection, which improves the efficiency of recombinant parvovirus production by more than 100 fold in comparison to other protocols in use. This protocol relies on the use of a novel adenovirus 5-based helper containing the parvovirus VP transcription unit (Ad-VP).

Introduction to Solid Supported Membrane Based Electrophysiology

JoVE 50230 5/11/2013

Andre Bazzone¹, Wagner Steuer Costa², Markus Braner¹, Octavian Călinescu¹, Lina Hatahet¹, Klaus Fendler¹

¹Department of Biophysical Chemistry, Max Planck Institute of Biophysics, ²Buchmann Institute for Molecular Life Sciences, Goethe University Frankfurt

Here we present an electrophysiological method based on solid supported membranes with focus on its applications for the characterization of electrogenic membrane transporters.

Transduction of Human Cells with Polymer-complexed Ecotropic Lentivirus for Enhanced Biosafety

JoVE 2822 7/24/2011

Bonnie Barrilleaux, Paul Knoepfler

Department of Cell Biology and Human Anatomy, School of Medicine, University of California, Davis

Lentiviruses are a valuable research tool for exploring gene function; however, researchers may wish to avoid production of pantropic lentivirus encoding known or suspected oncogenes. As an alternative, we present a safer protocol for use of ecotropic lentivirus on human cells modified to express the ecotropic receptor mSlc7a1.

Staphylococcus aureus Growth using Human Hemoglobin as an Iron Source

JoVE 50072 2/07/2013

Gleb Pishchany, Kathryn P. Haley, Eric P. Skaar

Department of Pathology, Microbiology and Immunology, Vanderbilt University Medical School

Here we describe a growth assay for Staphylococcus aureus using hemoglobin as the sole source of available nutrient iron. This assay establishes the role of bacterial factors involved in hemoglobin-derived iron acquisition.

Study of the DNA Damage Checkpoint using Xenopus Egg Extracts

JoVE 4449 11/05/2012

Jeremy Willis*, Darla DeStephanis*, Yogin Patel, Vrushab Gowda, Shan Yan

Department of Biology, University of North Carolina at Charlotte

Xenopus egg extract is a useful model system to investigate the DNA damage checkpoint. This protocol is for the preparation of Xenopus egg extracts and DNA damage checkpoint inducing reagents. These techniques are adaptable to a variety of DNA damaging approaches in the study of the DNA damage checkpoint signaling.

Odorant-induced Responses Recorded from Olfactory Receptor Neurons using the Suction Pipette Technique

JoVE 3862 4/05/2012

Samsudeen Ponissery Saidu*¹, Michele Dibattista*¹, Hugh R. Matthews², Johannes Reisert¹

¹Monell Chemical Senses Center, ²Department of Physiology, Development & Neuroscience, Physiological Laboratory, University of Cambridge

Olfactory receptor neurons (ORNs) convert odor signals first into a receptor current that in turn triggers action potentials that are conveyed to second order neurons in the olfactory bulb. Here we describe the suction pipette technique to record simultaneously the odorant-induced receptor current and action potentials from mouse ORNs.

Plastic Embedding and Sectioning of Xenopus laevis Embryos

JoVE 188 4/29/2007

Souichi Ogata¹, Shimako Kawauchi¹, Anne Calof², Ken W.Y. Cho¹

¹Department of Developmental and Cell Biology, University of California, Irvine (UCI), ²University of California, Irvine (UCI)

Plastic sections maintain true tissue morphology in thin sections of tissue that can be immunostained with fluorescent secondary antibodies, making this method more useful than paraffin-embedded or frozen sections for many types of tissue. The method for staining, plastic embedding, and sectioning is demonstrated in this video.

Site-specific Bacterial Chromosome Engineering: ΦC31 Integrase Mediated Cassette Exchange (IMCE)

JoVE 3698 3/16/2012

John R. Heil, Jiujun Cheng, Trevor C. Charles

Biology, University of Waterloo

A quick and efficient method to integrate foreign DNA of interest into pre-made acceptor strains, termed landing pad strains, is described. The method allows site-specific integration of a DNA cassette into the engineered landing pad locus of a given strain, through conjugation and expression of the ΦC31 integrase.

Density Gradient Multilayered Polymerization (DGMP): A Novel Technique for Creating Multi-compartment, Customizable Scaffolds for Tissue Engineering

JoVE 50018 2/12/2013

Shivanjali Joshi-Barr¹, Jerome V. Karpiak², Yogesh Ner¹, Jessica H. Wen³, Adam J. Engler³, Adah Almutairi^1,2

¹Skaggs School of Pharmacy and Pharmaceutical Sciences, University of California, San Diego, ²Biomedical Sciences Program, University of California, San Diego, ³Department of Bioengineering, University of California, San Diego

Here we describe a unique strategy for creating biocompatible, layered matrices with continuous interfaces between distinct layers for tissue engineering. Such a scaffold could provide an ideal customizable environment to modulate cell behavior by various biological, chemical or mechanical cues

Developing Custom Chinese Hamster Ovary-host Cell Protein Assays using Acoustic Membrane Microparticle Technology

JoVE 2493 2/03/2011

Matthew Dickerson¹, Kristen Leong², Kate Sheldon², Lara Madison¹

¹Biomarker Division, BioScale, Inc., ²Bioprocessing Division, BioScale, Inc.

Development of custom assays on the ViBE platform for more sensitive, reproducible, automated results in complex matrices is described. The universal cartridge allows assays to be easily adapted for use with custom assays. This versatility enables rapid development and validation of novel assays or automated versions of existing manual assays, exemplified in this video.

Purification of the M. magneticum Strain AMB-1 Magnetosome Associated Protein MamAΔ41

JoVE 1844 3/25/2010

Natalie Zeytuni, Raz Zarivach

Department of Life Sciences and National Institute for Biotechnology in the Negev, Ben-Gurion University

MamA is a unique Magnetosome associated protein which was shown to be involved in magnetosome activation. Here we present the purification protocol of MamA deletion mutant (MamAΔ41) from M. magneticum AMB-1.

Quantitation and Analysis of the Formation of HO-Endonuclease Stimulated Chromosomal Translocations by Single-Strand Annealing in Saccharomyces cerevisiae

JoVE 3150 9/23/2011

Lauren Liddell^1,2, Glenn Manthey², Nicholas Pannunzio³, Adam Bailis²

¹Irell & Manella Graduate School of Biological Sciences, ²Department of Molecular and Cellular Biology, City of Hope Comprehensive Cancer Center and Beckman Research Institute, ³Department of Biochemistry and Molecular Biology, University of Southern California, Norris Comprehensive Cancer Center

The HO-stimulated translocation assay monitors single-strand annealing following the creation of DNA double-strand breaks at multiple loci in diploid Saccharomyces cerevisiae. This mechanism may model genome rearrangements in somatic cells of higher eukaryotes following exposure to high doses of ionizing radiation.

Differentiating Functional Roles of Gene Expression from Immune and Non-immune Cells in Mouse Colitis by Bone Marrow Transplantation

JoVE 4208 10/01/2012

Hon Wai Koon, Samantha Ho, Michelle Cheng, Ryan Ichikawa, Charalabos Pothoulakis

Center for Inflammatory Bowel Diseases, Division of Digestive Diseases, David Geffen School of Medicine, The University of California Los Angeles, Los Angeles

Bone marrow transplantation provides a way to change the genotype of the bone marrow derived cells. If the gene of interest is expressed in both bone marrow derived cells and non-bone marrow derived cells, bone marrow transplantation can change the bone marrow derived cells to a different genotype without changing the non-bone marrow derived cell genotype.

Isolation and Animal Serum Free Expansion of Human Umbilical Cord Derived Mesenchymal Stromal Cells (MSCs) and Endothelial Colony Forming Progenitor Cells (ECFCs)

JoVE 1525 10/08/2009

Andreas Reinisch, Dirk Strunk

Stem Cell Research Unit, Medical University of Graz, Austria

This protocol describes the isolation and subsequent expansion of mesenchymal stromal cells and endothelial colony forming cells without the use of animal serum to generate autologous pairs for experimental transplantation purposes.

Creating Defined Gaseous Environments to Study the Effects of Hypoxia on C. elegans

JoVE 4088 7/20/2012

Emily M. Fawcett^1,2, Joseph W. Horsman¹, Dana L. Miller¹

¹Department of Biochemistry, University of Washington, ²Molecular and Cellular Biology Program, University of Washington

This paper details how to use continuous-flow hypoxia chambers to generate atmospheres with defined concentrations of O₂ to understand biological responses to decreased O₂. This system is easy to setup and maintain, and flexible enough to suit a wide range of O₂ concentrations and model systems

Micro-particle Image Velocimetry for Velocity Profile Measurements of Micro Blood Flows

JoVE 50314 4/25/2013

Katie L. Pitts¹, Marianne Fenech^1,2

¹Department of Chemical and Biological Engineering, University of Ottawa, ²Department of Mechanical Engineering, University of Ottawa

Micro-particle image velocimetry (μPIV) is used to visualize paired images of micro particles seeded in blood flows which are cross-correlated to give an accurate velocity profile. Shear rate, maximum velocity, velocity profile shape, and flow rate, each of which has clinical applications, can be derived from these measurements.

The 2009 Lindau Nobel Laureate Meeting: Erwin Neher, Physiology or Medicine 1991

JoVE 1563 11/11/2009

Erwin Neher

German biophysicist Erwin Neher shared the 1991 Nobel Prize in Physiology or Medicine with Bert Sakmann for their pioneering work measuring the activity of single ion channels in cells.

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.

Quantification of γH2AX Foci in Response to Ionising Radiation

JoVE 1957 4/06/2010

Li-Jeen Mah^1,2, Raja S. Vasireddy^1,2,3, Michelle M. Tang^1,3, George T. Georgiadis¹, Assam El-Osta^2,3, Tom C. Karagiannis^1,2

¹Epigenomic Medicine, Baker IDI Heart and Diabetes Institute, The Alfred Medical Research and Education Precinct, ²Department of Pathology, The University of Melbourne, ³Epigenetics in Human Health and Disease, Baker IDI Heart and Diabetes Institute, The Alfred Medical Research and Education Precinct

Quantification of DNA double-strand streaks using γH2AX formation as a molecular marker has become an invaluable tool in radiation biology. Here we demonstrate the use of an immunofluorescence assay for quantification of γH2AX foci after exposure of cells to radiation.

Transfection and Mutagenesis of Target Genes in Mosquito Cells by Locked Nucleic Acid-modified Oligonucleotides

JoVE 2355 12/26/2010

Nazzy Pakpour¹, Kong Wai Cheung¹, Lattha Souvannaseng¹, Jean-Paul Concordet², Shirley Luckhart¹

¹Department of Medical Microbiology and Immunology, University of California, Davis, ²Département Génétique et Développement, Institut Cochin, Université Paris Descartes

Oligonucleotides can be used to site specifically substitute a single nucleotide of transfected target genes in both Anopheles gambiae and Anopheles stephensi cells.

Lipid Vesicle-mediated Affinity Chromatography using Magnetic Activated Cell Sorting (LIMACS): a Novel Method to Analyze Protein-lipid Interaction

JoVE 2657 4/26/2011

Erhard Bieberich

Institute of Molecular Medicine and Genetics, Georgia Health Sciences University

To test the interaction of a protein with its target lipid we used MACS and Annexin V-conjugated magnetic beads and lipid vesicles synthesized from the target lipid and Annexin V-binding phosphatidylserine. Proteins bound to the target lipid are co-purified and analyzed after elution from the beads.

ampliPHOX Colorimetric Detection on a DNA Microarray for Influenza

JoVE 2682 6/09/2011

Kevin R. Moulton, Amber W. Taylor, Kathy L. Rowlen, Erica D. Dawson

InDevR, Inc.

ampliPHOX colorimetric detection technology is presented as an inexpensive alternative to fluorescence detection for microarrays. Based on photopolymerization, ampliPHOX produces solid polymer spots visible to the naked eye in just a few minutes. Results are then imaged and automatically interpreted with a simple yet powerful software package.

Whole-Body Nanoparticle Aerosol Inhalation Exposures

JoVE 50263 5/07/2013

Jinghai Yi^1,2, Bean T. Chen³, Diane Schwegler-Berry³, Dave Frazer³, Vince Castranova³, Carroll McBride¹, Travis L. Knuckles^1,2, Phoebe A. Stapleton^1,2, Valerie C. Minarchick^1,2, Timothy R. Nurkiewicz^1,2

¹Department of Physiology and Pharmacology, School of Medicine, West Virginia University, ²Center for Cardiovascular and Respiratory Sciences, West Virginia University, ³National Institute for Occupational Safety and Health

A whole-body nanoparticle aerosol inhalation exposure facility was constructed for nano-sized titanium dioxide (TiO₂) inhalation toxicology studies. This system provides nano-TiO₂ aerosol test atmospheres that have: 1) a steady mass concentration; 2) a homogenous composition free of contaminants; and 3) a stable particle size distribution during aerosol generation.

Closed System Cell Culture Protocol Using HYPERStack Vessels with Gas Permeable Material Technology

JoVE 2499 11/29/2010

Kim Titus*¹, Vitaly Klimovich*², Mark Rothenberg², Pilar Pardo*², Allison Tanner*³, Greg Martin³

¹Business Development, Corning Life Science, ²Applications, Corning Life Science, ³Product Development, Corning Life Science

An Introduction into the technology, protocol and handling of the Corning HYPERStack Vessels and accessories used for high yield adherent cell culture. The protocol will show how to use the closed system vessels for increasing cell harvesting over current stacked plate products.

Purification of Hsp104, a Protein Disaggregase

JoVE 3190 9/30/2011

Elizabeth A. Sweeny, Morgan E. DeSantis, James Shorter

Department of Biochemistry and Biophysics, University of Pennsylvania

Here, we describe a protocol for the purification of highly active Hsp104, a hexameric AAA+ protein from yeast, which couples ATP hydrolysis to protein disaggregation. This scheme exploits a His6-tagged construct for affinity purification from E. coli followed by anion-exchange chromatography, His6-tag removal with TEV protease, and size-exclusion chromatography.

In-vivo Detection of Protein-protein Interactions on Micro-patterned Surfaces

JoVE 1969 3/19/2010

Julian Weghuber, Stefan Sunzenauer, Mario Brameshuber, Birgit Plochberger, Clemens Hesch, Gerhard J. Schutz

Institute of Biophysics, Johannes Kepler Universitat Linz

This video shows experiments with subsequent analysis of protein-protein interactions by the use of micro-patterned surfaces. The approach offers the possibility to detect protein interactions in living cells and combines high throughput capabilities with the possibility to extract quantitative information.

Preparation of embryos for Electron Microscopy of the Drosophila embryonic heart tube

JoVE 1630 12/21/2009

Nadine H. Soplop^1,2, Rajesh Patel¹, Sunita G. Kramer^1,2

¹Joint Graduate Program in Cell and Developmental Biology, UMDNJ-Graduate School of Biomedical Sciences and Rutgers: The State University of New Jersey, ²Department of Pathology and Laboratory Medicine, Robert Wood Johnson Medical School, University of Medicine and Dentistry of New Jersey

We describe a process for fixation, embedding, sectioning, and imaging of late stage Drosophila embryos for Trasmission Electron Microscopy of the embryonic heart tube. This technique allows for the visualization of the heart tube lumen as well as the basement membrane, which lines the lumen of the heart.