Generation of High Quality Chromatin Immunoprecipitation DNA Template for High-throughput Sequencing (ChIP-seq)

JoVE 50286 4/19/2013

Sandra Deliard¹, Jianhua Zhao¹, Qianghua Xia¹, Struan F.A. Grant^1,2

¹Division of Human Genetics, Children's Hospital of Philadelphia Research Institute, ²Department of Pediatrics, Perelman School of Medicine, University of Pennsylvania

The combination of chromatin immunoprecipitation and ultra-high-throughput sequencing (ChIP-seq) can identify and map protein-DNA interactions in a given tissue or cell line. Outlined is how to generate a high quality ChIP template for subsequent sequencing, using experience with the transcription factor TCF7L2 as an example.

Chromatin Isolation by RNA Purification (ChIRP)

JoVE 3912 3/25/2012

Ci Chu, Jeffrey Quinn, Howard Y. Chang

Howard Hughes Medical Institute and Program in Epithelial Biology, Stanford University School of Medicine

ChIRP is a novel and rapid technique to map genomic binding sites of long noncoding RNAs (lncRNAs). The method takes advantage of the specificity of anti-sense tiling oligonucleotides to allow the enumeration of lncRNA-bound genomic sites.

ReAsH/FlAsH Labeling and Image Analysis of Tetracysteine Sensor Proteins in Cells

JoVE 2857 8/31/2011

Sevgi Irtegun, Yasmin M. Ramdzan, Terrence D. Mulhern, Danny M. Hatters

Department of Biochemistry and Molecular Biology, Bio21 Molecular Science and Biotechnology Institute

The biarsenical dyes FlAsH and ReAsH bind specifically to tetracysteine motifs in proteins and can selectively label proteins in live cells. Recently this labeling strategy has been used to develop sensors for different protein conformations or oligomeric states. We describe the labeling approach and methods to quantitatively analyze binding.

Biosensor for Detection of Antibiotic Resistant Staphylococcus Bacteria

JoVE 50474 5/08/2013

Rajesh Guntupalli¹, Iryna Sorokulova¹, Eric Olsen², Ludmila Globa¹, Oleg Pustovyy¹, Vitaly Vodyanoy¹

¹Department of Anatomy, Physiology and Pharmacology, College of Veterinary Medicine, Auburn University, ²Clinical Research Laboratory, 81st Medical Group, Keesler Air Force Base

Lytic phage biosensors and antibody beads are able to discriminate between methicillin resistant (MRSA) and sensitive staphylococcus bacteria. The phages were immobilized by a Langmuir-Blodgett method onto a surface of a quartz crystal microbalance sensor and worked as broad range staphylococcus probes. Antibody beads recognize MRSA.

iCLIP - Transcriptome-wide Mapping of Protein-RNA Interactions with Individual Nucleotide Resolution

JoVE 2638 4/30/2011

Julian Konig¹, Kathi Zarnack², Gregor Rot³, Tomaz Curk³, Melis Kayikci¹, Blaz Zupan³, Daniel J. Turner⁴, Nicholas M. Luscombe², Jernej Ule¹

¹Laboratory of Molecular Biology, Medical Research Council - MRC, ²European Bioinformatics Institute, EMBL Heidelberg, ³Computer and Information Science, University of Ljubljana, ⁴Wellcome Trust Genome Campus, Wellcome Trust Sanger Institute

The spatial arrangement of RNA-binding proteins on a transcript is a key determinant of post-transcriptional regulation. Therefore, we developed individual-nucleotide resolution UV crosslinking and immunoprecipitation (iCLIP) that allows precise genome-wide mapping of the binding sites of an RNA-binding protein.

A Novel Bayesian Change-point Algorithm for Genome-wide Analysis of Diverse ChIPseq Data Types

JoVE 4273 12/10/2012

Haipeng Xing¹, Willey Liao^1,2, Yifan Mo^1,2, Michael Q. Zhang^2,3

¹Department of Applied Mathematics & Statistics, Stony Brook University, ²Computational Biology and Bioinformatics, Cold Spring Harbor Laboratory, ³Department of Molecular and Cell Biology, University of Texas at Dallas

Our Bayesian Change Point (BCP) algorithm builds on state-of-the-art advances in modeling change-points via Hidden Markov Models and applies them to chromatin immunoprecipitation sequencing (ChIPseq) data analysis. BCP performs well in both broad and punctate data types, but excels in accurately identifying robust, reproducible islands of diffuse histone enrichment.

Optimized Transfection Strategy for Expression and Electrophysiological Recording of Recombinant Voltage-Gated Ion Channels in HEK-293T Cells

JoVE 2314 1/19/2011

Adriano Senatore, Adrienne N. Boone, J. David Spafford

Department of Biology, University of Waterloo

Reliable method for highly efficient in vitro expression and subsequent electrophysiological recording of recombinant voltage-gated ion channels in cultured human embryonic kidney cells (HEK-293T).

Proteomics to Identify Proteins Interacting with P2X2 Ligand-Gated Cation Channels

JoVE 1178 5/18/2009

Harpreet Singh¹, Sarah Warburton², Thomas M. Vondriska³, Baljit S. Khakh¹

¹Department of Physiology, David Geffen School of Medicine, University of California, Los Angeles, ²Department of Anesthesiology, David Geffen School of Medicine, University of California, Los Angeles, ³Department of Anesthesiology, Medicine and Physiology, David Geffen School of Medicine, University of California, Los Angeles

We describe a simple protocol to identify brain proteins that bind to the full length C terminus of ATP-gated P2X2 receptors. The extension and systematic application of this approach to all P2X receptors is expected to lead to a better understanding of P2X receptor signaling.

Chromatin Interaction Analysis with Paired-End Tag Sequencing (ChIA-PET) for Mapping Chromatin Interactions and Understanding Transcription Regulation

JoVE 3770 4/30/2012

Yufen Goh*¹, Melissa J. Fullwood*^1,2,3, Huay Mei Poh¹, Su Qin Peh¹, Chin Thing Ong¹, Jingyao Zhang¹, Xiaoan Ruan¹, Yijun Ruan^1,3

¹Genome Institute of Singapore, Agency for Science, Technology and Research, Singapore, ²A*STAR-Duke-NUS Neuroscience Research Partnership, Singapore, ³Department of Biochemistry, National University of Singapore, Singapore

Chromatin Interaction Analysis by Paired-End Tag Sequencing (ChIA-PET) is a method for de novo detection of chromatin interactions, for better understanding of transcriptional control.

High-density EEG Recordings of the Freely Moving Mice using Polyimide-based Microelectrode

JoVE 2562 1/11/2011

Mina Lee^1,2, Dongwook Kim^1,2, Hee-Sup Shin^1,2, Ho-Geun Sung³, Jee Hyun Choi^1,2

¹Center for Neural Science , Korea Institute of Science and Technology (KIST), ²Department of Neuroscience, University of Science and Technology, ³Fab Service Department, Korea Advanced Nano Fab Center

In this article, we described the surgery procedure and handling tips for implantation of ultra-thin polyimide-based microelectrode array (PBM-array) on the mouse skull for acquisition of high-density encephalography (EEG) in a mouse model.

Development of an Audio-based Virtual Gaming Environment to Assist with Navigation Skills in the Blind

JoVE 50272 3/27/2013

Erin C. Connors¹, Lindsay A. Yazzolino¹, Jaime Sánchez², Lotfi B. Merabet¹

¹Laboratory for Visual Neuroplasticity, Department of Ophthalmology, Massachusetts Eye and Ear Infirmary, Harvard Medical School, ²Department of Computer Science and Center for Advanced Research in Education (CARE), University of Chile

Audio-based Environment Simulator (AbES) is virtual environment software designed to improve real world navigation skills in the blind.

Real-time Analyses of Retinol Transport by the Membrane Receptor of Plasma Retinol Binding Protein

JoVE 50169 1/28/2013

Riki Kawaguchi, Ming Zhong, Hui Sun

Department of Physiology, Jules Stein Eye Institute and Howard Hughes Medical Institute, University of California, Los Angeles

Here we describe an optimized technique to produce high-quality vitamin A/RBP complex and two real-time monitoring techniques to study vitamin A transport by STRA6, the RBP receptor.

Blastomere Explants to Test for Cell Fate Commitment During Embryonic Development

JoVE 4458 1/26/2013

Paaqua A. Grant¹, Mona B. Herold¹, Sally A. Moody²

¹Department of Biological Sciences, The George Washington University, ²Department of Anatomy and Regenerative Biology, The George Washington University

The fate of an individual embryonic cell can be influenced by inherited molecules and/or by signals from neighboring cells. Utilizing fate maps of the cleavage stage Xenopus embryo, single blastomeres can be identified for culture in isolation to assess the contributions of inherited molecules versus cell-cell interactions.

Determination of Molecular Structures of HIV Envelope Glycoproteins using Cryo-Electron Tomography and Automated Sub-tomogram Averaging

JoVE 2770 12/01/2011

Joel R. Meyerson^1,2, Tommi A. White¹, Donald Bliss³, Amy Moran³, Alberto Bartesaghi¹, Mario J. Borgnia¹, M. Jason V. de la Cruz¹, David Schauder¹, Lisa M. Hartnell¹, Rachna Nandwani^1,4, Moez Dawood⁵, Brianna Kim⁶, Jun Hong Kim⁷, John Sununu⁸, Lisa Yang⁹, Siddhant Bhatia¹⁰, Carolyn Subramaniam¹, Darrell E. Hurt¹¹, Laurent Gaudreault¹², Sriram Subramaniam¹

¹Laboratory of Cell Biology, Center for Cancer Research, National Cancer Institute, National Institutes of Health, ²The Medical Research Council Mitochondrial Biology Unit, University of Cambridge, ³National Library of Medicine, National Institutes of Health, ⁴Massachusetts Institute of Technology, ⁵William Fremd High School, ⁶University of Virginia, ⁷Duke University, ⁸Yale University, ⁹University of Notre Dame, ¹⁰Washington University in St. Louis, ¹¹Bioinformatics and Computational Biosciences Branch, National Institute of Allergy and Infectious Diseases, National Institutes of Health, ¹²Thomas Jefferson High School for Science and Technology

The protocol describes a high-throughput approach to determining structures of membrane proteins using cryo-electron tomography and 3D image processing. It covers the details of specimen preparation, data collection, data processing and interpretation, and concludes with the production of a representative target for the approach, the HIV-1 Envelope glycoprotein. These computational procedures are designed in a way that enables researchers and students to work remotely and contribute to data processing and structural analysis.

Method for the Isolation and Identification of mRNAs, microRNAs and Protein Components of Ribonucleoprotein Complexes from Cell Extracts using RIP-Chip

JoVE 3851 9/29/2012

Garrett M. Dahm^1,2, Matthew M. Gubin^1,2, Joseph D. Magee², Patsharaporn Techasintana^1,2, Robert Calaluce², Ulus Atasoy^1,2,3

¹Molecular Microbiology and Immunology, University of Missouri, ²Department of Surgery, University of Missouri, ³Child Health, University of Missouri

A step by step protocol to isolating and identifying RNA associated complexes through RIP-Chip.

A Liquid Phase Affinity Capture Assay Using Magnetic Beads to Study Protein-Protein Interaction: The Poliovirus-Nanobody Example

JoVE 3937 5/29/2012

Lise Schotte, Bart Rombaut, Bert Thys

Department of Pharmaceutical Biotechnology and Molecular Biology, Centre for Pharmaceutical Research, Vrije Universiteit Brussel

In this article, a simple, quantitative, liquid phase affinity capture assay is presented. It is a reliable technique based on the interaction between magnetic beads and tagged proteins (e.g. nanobodies) on one hand and the affinity between the tagged protein and a second, labeled protein (e.g. poliovirus) on the other.

Time-lapse Imaging of Primary Preneoplastic Mammary Epithelial Cells Derived from Genetically Engineered Mouse Models of Breast Cancer

JoVE 50198 2/08/2013

Rebecca E. Nakles¹, Sarah L. Millman¹, M. Carla Cabrera¹, Peter Johnson^1,2, Susette Mueller^1,2, Philipp S. Hoppe³, Timm Schroeder³, Priscilla A. Furth^1,2,4,5

¹Department of Oncology, Georgetown University, ²Lombardi Comprehensive Cancer Center, Georgetown University, ³Stem Cell Dynamics, Helmholtz Zentrum München - German Research Center for Environmental Health, ⁴Department of Medicine, Georgetown University, ⁵Department of Nanobiomedical Science and WCU Research Center of Nanobiomedical Science, Dankook University

Time-lapse imaging is used to assess behavior of primary preneoplastic mammary epithelial cells derived from genetically engineered mouse models of breast cancer risk to determine if there are correlations between specific behavioral parameters and distinct genetic lesions.

Concurrent Quantitative Conductivity and Mechanical Properties Measurements of Organic Photovoltaic Materials using AFM

JoVE 50293 1/23/2013

Maxim P. Nikiforov¹, Seth B. Darling^1,2

¹Center for Nanoscale Materials, Argonne National Laboratory, ²Institute for Molecular Engineering, University of Chicago

Organic photovoltaic (OPV) materials are inherently inhomogeneous at the nanometer scale. Nanoscale inhomogeneity of OPV materials affects performance of photovoltaic devices. In this paper, we describe a protocol for quantitative measurements of electrical and mechanical properties of OPV materials with sub-100 nm resolution.

High-throughput Screening for Small-molecule Modulators of Inward Rectifier Potassium Channels

JoVE 4209 1/27/2013

Rene Raphemot^1,2, C. David Weaver^1,3, Jerod S. Denton^1,2

¹Department of Pharmacology, Vanderbilt University School of Medicine, ²Department of Anesthesiology, Vanderbilt University School of Medicine, ³Vanderbilt Institute of Chemical Biology, Vanderbilt University School of Medicine

Methods for developing and validating a quantitative fluorescence assay for measuring the activity of inward rectifier potassium (Kir) channels for high-throughput compound screening is presented.

Mapping Inhibitory Neuronal Circuits by Laser Scanning Photostimulation

JoVE 3109 10/06/2011

Taruna Ikrar¹, Nicholas D. Olivas¹, Yulin Shi¹, Xiangmin Xu^1,2

¹Department of Anatomy and Neurobiology, School of Medicine, University of California, Irvine, ²Department of Biomedical Engineering, School of Engineering, University of California, Irvine

This paper introduces an approach of combining laser scanning photostimulation with whole cell recordings in transgenic mice expressing GFP in limited inhibitory neuron populations. The technique allows for extensive mapping and quantitative analysis of local synaptic circuits of specific inhibitory cortical neurons.

Bacterial Immobilization for Imaging by Atomic Force Microscopy

JoVE 2880 8/10/2011

David P. Allison^1,2, Claretta J. Sullivan³, Ninell Pollas Mortensen^1,2, Scott T. Retterer^1,4, Mitchel Doktycz^1,4

¹Biological and Nanoscale Systems Group, Biosciences Division, Oak Ridge National Laboratory, ²Department of Biochemistry and Cellular and Molecular Biology, University of Tennessee, ³Department of Surgery, Eastern Virginia Medical School, ⁴Center for Nanophase Materials Sciences Division, Oak Ridge National Laboratory

Live Gram-negative and Gram-positive bacteria can be immobilized on gelatin-coated mica and imaged in liquid using Atomic Force Microscopy (AFM).

Targeted Labeling of Neurons in a Specific Functional Micro-domain of the Neocortex by Combining Intrinsic Signal and Two-photon Imaging

JoVE 50025 12/12/2012

Philip O'Herron, Zhiming Shen, Zhongyang Lu, Adrien E. Schramm, Manuel Levy, Prakash Kara

Department of Neuroscience, Medical University of South Carolina

A method is described for labeling neurons with fluorescent dyes in predetermined functional micro-domains of the neocortex. First, intrinsic signal optical imaging is used to obtain a functional map. Then two-photon microscopy is used to label and image neurons within a micro-domain of the map.

Angle-resolved Photoemission Spectroscopy At Ultra-low Temperatures

JoVE 50129 10/09/2012

Sergey V. Borisenko¹, Volodymyr B. Zabolotnyy¹, Alexander A. Kordyuk^1,2, Danil V. Evtushinsky¹, Timur K. Kim^1,3, Emanuela Carleschi⁴, Bryan P. Doyle⁴, Rosalba Fittipaldi⁵, Mario Cuoco⁵, Antonio Vecchione⁵, Helmut Berger⁶

¹Institute for Solid State Research, IFW-Dresden, ²Institute of Metal Physics of National Academy of Sciences of Ukraine, ³Diamond Light Source LTD, ⁴Department of Physics, University of Johannesburg, ⁵CNR-SPIN, and Dipartimento di Fisica "E. R. Caianiello", Università di Salerno, ⁶Institute of Physics of Complex Matter, École Polytechnique Fédérale de Lausanne

The overall goal of this method is to determine the low-energy electronic structure of solids at ultra-low temperatures using Angle-Resolved Photoemission Spectroscopy with synchrotron radiation.

IonFlux: Automated Patch Clamp System with Plate Reader Simplicity - ADVERTISEMENT

JoVE 2392 9/15/2010

The IonFlux Automated Patch Clamp System provides high throughput, cost-effective ion channel screening for a wide range of electrophysiology applications. Fast compound exchange, low cost per data point, and convenient well plate formats make the system ideal for both ligand- and voltage-gated ion channel targets. The IonFlux HT provides an industry-leading 10,000 data points per day, while the IonFlux 16 provides true automated patch clamp performance for about the cost of a manual patch clamp rig.

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).

Fluorescence-microscopy Screening and Next-generation Sequencing: Useful Tools for the Identification of Genes Involved in Organelle Integrity

JoVE 3809 4/13/2012

Giovanni Stefano, Luciana Renna, Federica Brandizzi

DOE Plant Research Laboratory, Michigan State University

A fundamental quest in cell biology is to define the mechanisms that underlie the identity of the organelles that make eukaryotic cells. Here we propose a method to identify the genes responsible for the morphological and functional integrity of plant organelles using fluorescence microscopy and next-generation sequencing tools.

High-Resolution Endocardial and Epicardial Optical Mapping in a Sheep Model of Stretch-Induced Atrial Fibrillation

JoVE 3103 7/29/2011

David Filgueiras-Rama, Raphael Pedro Martins, Steven R. Ennis, Sergey Mironov, Jiang Jiang, Masatoshi Yamazaki, Jérôme Kalifa, Josè Jalife, Omer Berenfeld

Center for Arrhythmia Research. Internal Medicine, University of Michigan

This report provides a detailed description of the methodology and results of simultaneous endocardial and epicardial optical mapping of electrical excitation in the intact left atrium of a Langendorff-perfused sheep heart during stretch-induced atrial fibrillation.

A Microfluidic Device for Studying Multiple Distinct Strains

JoVE 4257 11/09/2012

Guy Aidelberg*, Yifat Goldshmidt*, Iftach Nachman

Department of Biochemistry and Molecular Biology, George S. Wise Faculty of Life Sciences, Tel Aviv University

We present a simple method to produce microfluidic devices capable of applying similar dynamic conditions to multiple distinct strains, without the need for a clean room or soft lithography.

Multiparametric Optical Mapping of the Langendorff-perfused Rabbit Heart

JoVE 3160 9/13/2011

Qing Lou, Wenwen Li, Igor R. Efimov

Department of Biomedical Engineering, Washington University in St. Louis

This article describes the basic procedures for conducting optical mapping experiments in the Langendorff-perfused rabbit heart using the panoramic imaging system, and the dual (voltage and calcium) imaging modality.

A High-content Imaging Workflow to Study Grb2 Signaling Complexes by Expression Cloning

JoVE 4382 10/30/2012

Jamie Freeman¹, Janos Kriston-Vizi¹, Brian Seed², Robin Ketteler¹

¹MRC LMCB, University College London, ²Center for Computational and Integrative Biology, Massachusetts General Hospital

A high-content screening method for the identification of novel signaling competent transmembrane receptors is described. This method is amenable to large-scale automation and allows predictions about in vivo protein binding and the sub-cellular localization of protein complexes in mammalian cells.