Identification of Protein Complexes in Escherichia coli using Sequential Peptide Affinity Purification in Combination with Tandem Mass Spectrometry

JoVE 4057 11/12/2012

Mohan Babu^1,2, Olga Kagan¹, Hongbo Guo¹, Jack Greenblatt^1,3, Andrew Emili^1,3

¹Banting and Best Department of Medical Research, Donnelly Centre, University of Toronto, ²Deparment of Biochemistry, Research and Innovation Centre, University of Regina, ³Department of Medical Genetics and Microbiology, University of Toronto

Affinity purification of tagged proteins in combination with mass spectrometry (APMS) is a powerful method for the systematic mapping of protein interaction networks and for investigating the mechanistic basis of biological processes. Here, we describe an optimized sequential peptide affinity (SPA) APMS procedure developed for the bacterium Escherichia coli that can be used to isolate and characterize stable multi-protein complexes to near homogeneity even starting from low copy numbers per cell.

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.

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.

Isothermal Titration Calorimetry for Measuring Macromolecule-Ligand Affinity

JoVE 2796 9/07/2011

Michael R. Duff, Jr., Jordan Grubbs, Elizabeth E. Howell

Department of Biochemistry, Cellular and Molecular Biology, University of Tennessee

A general protocol for the use of isothermal titration calorimetry to monitor the binding thermodynamics for biological systems with moderate binding affinities is presented.

Quantifying Agonist Activity at G Protein-coupled Receptors

JoVE 3179 12/26/2011

Frederick J. Ehlert¹, Hinako Suga², Michael T. Griffin³

¹Department of Pharmacology, University of California, Irvine, ²Department of Pharmacology, University of California, ³Schmid College of Science, Chapman University

A method for estimating the affinity constant of an agonist for the active state (K_b) of a G protein-coupled receptor is described. The analysis provides absolute or relative measures of K_b depending on whether constitutive receptor activation is measurable. Our method applies to various responses downstream from receptor activation.

Improved Protocol For Laser Microdissection Of Human Pancreatic Islets From Surgical Specimens

JoVE 50231 1/06/2013

Dorothée Sturm^1,2, Lorella Marselli³, Florian Ehehalt^1,2, Daniela Richter¹, Marius Distler², Stephan Kersting^1,2, Robert Grützmann², Krister Bokvist⁴, Philippe Froguel⁵, Robin Liechti⁶, Anne Jörns⁷, Paolo Meda⁸, Gustavo Bruno Baretton⁹, Hans-Detlev Saeger², Anke M. Schulte¹⁰, Piero Marchetti³, Michele Solimena¹

¹Molecular Diabetology, Paul Langerhans Institute Dresden, ²Department of GI-, Thoracic- and Vascular Surgery, University Hospital Carl Gustav Carus, University of Technology Dresden, ³Department of Endocrinology and Metabolism, Metabolic Unit University of Pisa, ⁴Labs DC0522, Lilly Corporate Center, ⁵Genomics, Faculty of Medicine Imperial College London, ⁶Vital-IT, SIB Swiss Institute of Bioinformatics, ⁷Clinical Biochemistry, Hannover Medical School, ⁸Cell Physiology and Metabolism, Medical School, University of Geneva, ⁹Department of Pathology, University Hospital Carl Gustav Carus, University of Technology Dresden, ¹⁰R&D DIAB Division / Translational Medicine, Sanofi-Aventis

Laser microdissection is a technique that allows the recovery of selected cells from minute amounts of parenchyma. Here we describe a protocol for acquiring human pancreatic islets from surgical specimens to be used for transcriptomic studies. Our protocol improves the intrinsic autofluorescence of human beta cells, thus facilitating their collection.

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.

Profiling Changes in Receptor Tyrosine Kinase Phosphorylation using Antibody Arrays - ADVERTISEMENT

JoVE 4199 9/27/2012

Greta J. Wegner, David J. Finkel, Amy E. James, Richard A. Krzyzek

Array Group, Assay Department, R&D Systems, Inc.

Proteome Profiler antibody arrays are a convenient and cost efficient way to screen for changes in receptor tyrosine kinase (RTK) phosphorylation without performing numerous immunoprecipitation (IP) Westerns. The ARY001 Human RTK array allows for the qualitative measurement of multiple RTKs in a single sample using chemiluminescence detection.

Hi-C: A Method to Study the Three-dimensional Architecture of Genomes.

JoVE 1869 5/06/2010

Nynke L. van Berkum*¹, Erez Lieberman-Aiden*^2,3,4,5, Louise Williams*², Maxim Imakaev⁶, Andreas Gnirke², Leonid A. Mirny^3,6, Job Dekker¹, Eric S. Lander^2,7,8

¹Program in Gene Function and Expression, Department of Biochemistry and Molecular Pharmacology, University of Massachusetts Medical School, ²Broad Institute of Harvard and Massachusetts Institute of Technology, ³Division of Health Sciences and Technology, Massachusetts Institute of Technology, ⁴Program for Evolutionary Dynamics, Department of Organismic and Evolutionary Biology, Department of Mathematics, Harvard University, ⁵Department of Applied Mathematics, Harvard University, ⁶Department of Physics, Massachusetts Institute of Technology, ⁷Department of Systems Biology, Harvard Medical School, ⁸Department of Biology, Massachusetts Institute of Technology

The Hi-C method allows unbiased, genome-wide identification of chromatin interactions (1). Hi-C couples proximity ligation and massively parallel sequencing. The resulting data can be used to study genomic architecture at multiple scales: initial results identified features such as chromosome territories, segregation of open and closed chromatin, and chromatin structure at the megabase scale.

Identification of Protein Interacting Partners Using Tandem Affinity Purification

JoVE 3643 2/25/2012

Dalan Bailey*, Luis Urena*, Lucy Thorne, Ian Goodfellow

Section of Virology, Department of Medicine, Imperial College London

Tandem affinity purification is a robust approach for the identification of protein binding partners. As proof of concept, this methodology was applied to the well-characterized translation initiation factor eIF4E to co-precipitate the host cell factors involved in translation initiation. This method is easily adapted to any cellular or viral protein.

Purification of Pathogen Vacuoles from Legionella-infected Phagocytes

JoVE 4118 6/19/2012

Christine Hoffmann, Ivo Finsel, Hubert Hilbi

Max von Pettenkofer-Institut, Ludwig-Maximilians-Universität

This article describes a method for the isolation and purification of intact Legionella-containing vacuoles (LCVs) from amoeba and macrophages. The two-step protocol comprises LCV enrichment by immuno-magnetic separation using an antibody against a bacterial LCV marker and further purification by density gradient centrifugation.

The Importance of Correct Protein Concentration for Kinetics and Affinity Determination in Structure-function Analysis

JoVE 1746 3/17/2010

Ewa Pol

GE Healthcare Bio-Sciences AB

We apply label-free protein interaction analysis using Biacore X100 for structure-function analysis of the binding of several cystatin B mutants to papain through kinetic characterization. Calibration-free concentration analysis (CFCA) measures the concentration of protein with retained binding activity without the need for a standard curve. We show that confirmation of concentrations using CFCA increases the reliability of the kinetic analysis and that kinetic constants can reliably be determined even if the activity of a recombinant protein is reduced.

Direct Imaging of ER Calcium with Targeted-Esterase Induced Dye Loading (TED)

JoVE 50317 5/07/2013

Samira Samtleben¹, Juliane Jaepel^1,2, Caroline Fecher¹, Thomas Andreska¹, Markus Rehberg³, Robert Blum¹

¹Institute for Clinical Neurobiology, University of Wuerzburg, ²Department of Synapses - Circuits - Plasticity, Max Planck Institute of Neurobiology, Martinsried, ³Walter Brendel Centre of Experimental Medicine, Ludwig-Maximilians University of Munich

Targeted-esterase induced dye loading (TED) supports the analysis of intracellular calcium store dynamics by fluorescence imaging. The method bases on targeting of a recombinant Carboxylesterase to the endoplasmic reticulum (ER), where it improves the local unmasking of synthetic low-affinity Ca²⁺ indicator dyes in the ER lumen.

Lectin-based Isolation and Culture of Mouse Embryonic Motoneurons

JoVE 3200 9/15/2011

Rebecca Conrad¹, Sibylle Jablonka², Teresa Sczepan¹, Michael Sendtner², Stefan Wiese¹, Alice Klausmeyer¹

¹Institute for Cellmorphology and molecular Neurobiology, Group for Cellbiology, Ruhr-University Bochum, ²Institute for Clinical Neurobiology, University of Wuerzburg

An alternative way of isolating mouse embryonic motoneurons from the spinal cord is described. The method takes into account the fact that lectin can bind to the low affinity nerve growth factor receptor p75NTR. This lectin-based preplating allows a purification similar to that with a specific antibody against the p75NTR.

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.

A Cell Free Assay System Estimating the Neutralizing Capacity of GM-CSF Antibody using Recombinant Soluble GM-CSF Receptor

JoVE 2742 6/27/2011

Shinya Urano¹, Ryushi Tazawa¹, Takahito Nei¹, Natsuki Motoi¹, Masato Watanabe², Takenori Igarashi³, Masahiro Tomita³, Koh Nakata¹

¹Bioscience Medical Research Center, Niigata University Medical and Dental Hospital, ²First department of Internal Medicine, School of Medicine, Kyorin University, ³Neosilk Laboratory, Immuno Biological Laboratories Co., Ltd.

We designed a cell-free receptor binding assay in order to estimate the binding of granulocyte-macrophage colony-stimulating factor (GM-CSF) to the receptors. It enables us to evaluate competitive inhibition of biotinylated GM-CSF binding to soluble GM-CSF receptor alpha by GM-CSF autoantibody with excellent reproducibility.

Primer Extension Capture: Targeted Sequence Retrieval from Heavily Degraded DNA Sources

JoVE 1573 9/03/2009

Adrian W. Briggs, Jeffrey M. Good, Richard E. Green, Johannes Krause, Tomislav Maricic, Udo Stenzel, Svante Pääbo

Max-Planck Institute for Evolutionary Anthropology, Leipzig

We present a method of targeted ancient DNA sequence retrieval, which we used to reconstruct the complete mitochondrial genomes of five Neandertal individuals. Comparison of these sequences with present day humans suggests that Neandertals had a long term low effective population size.

Cellular Lipid Extraction for Targeted Stable Isotope Dilution Liquid Chromatography-Mass Spectrometry Analysis

JoVE 3399 11/17/2011

Stacy L. Gelhaus^1,2, A. Clementina Mesaros^1,2, Ian A. Blair^1,2

¹Centers for Cancer Pharmacology and Excellence in Environmental Toxicology, University of Pennsylvania, ²Department of Pharmacology, University of Pennsylvania

This protocol will demonstrate the extraction and analysis of free and esterified bioactive fatty acids from cells. Fatty acids are accurately quantified using stable isotope dilution, chiral liquid chromatography, electron capture atmospheric chemical ionization multiple reaction monitoring mass spectrometry (SID-LC-ECAPCI-MRM/MS).

Rapid Isolation of Viable Circulating Tumor Cells from Patient Blood Samples

JoVE 4248 6/15/2012

Andrew D. Hughes¹, Jeff Mattison¹, John D. Powderly^2,3, Bryan T. Greene^2,3, Michael R. King¹

¹Department of Biomedical Engineering, Cornell University, ²BioCytics, Inc., ³Carolina BioOncology Institute, PLLC

Circulating tumor cells are isolated from the blood of cancer patients without inflicting cellular damage. Isolation of tumor cells is accomplished using a bimolecular surface of E-selectin in addition to antibodies against epithelial markers. A nanotube coating specifically promotes cancer cell adhesion resulting in high capture purities.

Biomolecular Detection employing the Interferometric Reflectance Imaging Sensor (IRIS)

JoVE 2694 5/03/2011

Carlos A. Lopez¹, George G. Daaboul², Sunmin Ahn², Alexander P. Reddington¹, Margo R. Monroe², Xirui Zhang², Rostem J. Irani³, Chunxiao Yu^4,5, Caroline A. Genco^4,5, Marina Cretich⁶, Marcella Chiari⁶, Bennett B. Goldberg¹, John H. Connor⁵, M. Selim Ünlü^1,2

¹Department of Electrical and Computer Engineering, Boston University, ²Department of Biomedical Engineering, Boston University, ³Center for Advanced Genomics Technology, Boston University, ⁴Department of Medicine, Section of Infectious Diseases, Boston University School of Medicine, ⁵Department of Microbiology, Boston University School of Medicine, ⁶CNR (National Research Council), Istituto di Chimica del Riconoscimento Molecolare

Quantitative, high-throughput, real-time, and label-free biomolecular detection (DNA, protein, etc.) on SiO₂ surfaces can be achieved using a simple interferometric technique which relies on LED illumination, minimal optical components, and a camera. The Interferometric Reflectance Imaging Sensor (IRIS) is inexpensive, simple to use, and amenable to microarray formats.

Development of Cell-type specific anti-HIV gp120 aptamers for siRNA delivery

JoVE 2954 6/23/2011

Jiehua Zhou¹, Haitang Li¹, Jane Zhang², Swiderski Piotr³, John Rossi¹

¹Department of Molecular and Cellular Biology, Beckman Research Institute of City of Hope, ²Graduate School of Biological Sciences, Beckman Research Institute of City of Hope, ³Shared Resource-DNA/RNA Peptide, Beckman Research Institute of City of Hope

Several 2’-Fluoro RNA aptamers against HIV-1Ba-L gp120 with nanomole affinity are isolated from a RNA library by in vitro SELEX procedure. A new dual inhibitory function anti-gp120 aptamer-siRNA chimera is created and shows considerable promise for systemic anti-HIV therapy.

Preparation of Acute Subventricular Zone Slices for Calcium Imaging

JoVE 4071 9/19/2012

Benjamin Lacar, Stephanie Z. Young, Jean-Claude Platel, Angélique Bordey

Department of Neurosurgery and Cellular & Molecular Physiology, Yale University School of Medicine

A method to load subventricular zone (SVZ) cells with calcium indicator dyes for recording calcium activity is described. The postnatal SVZ contains tightly packed cells including neural progenitor cells and neuroblasts. Rather than using bath loading we injected the dye by pressure inside the tissue allowing better dye diffusion.

Production of Disulfide-stabilized Transmembrane Peptide Complexes for Structural Studies

JoVE 50141 3/06/2013

Pooja Sharma^1,2, Mariam Kaywan-Lutfi¹, Logesvaran Krshnan^1,2, Eamon F. X. Byrne^1,2, Melissa Joy Call^1,2, Matthew Edwin Call^1,2

¹Structural Biology Division, The Walter and Eliza Hall Institute of Medical Research, ²The University of Melbourne

Biophysical and biochemical studies of interactions among membrane-embedded protein domains face many technical challenges, the first of which is obtaining appropriate study material. This article describes a protocol for producing and purifying disulfide-stabilized transmembrane peptide complexes that are suitable for structural analysis by solution nuclear magnetic resonance (NMR) and other analytical applications.

IP-FCM: Immunoprecipitation Detected by Flow Cytometry

JoVE 2066 12/02/2010

Tessa R. Davis, Adam G. Schrum

Department of Immunology, College of Medicine, Mayo Clinic

The IP-FCM method is presented, which allows a sensitive, robust, biochemical assessment of native protein-protein interactions, without requiring genetic engineering or large sample sizes.

Semi-automated Optical Heartbeat Analysis of Small Hearts

JoVE 1435 9/16/2009

Karen Ocorr¹, Martin Fink², Anthony Cammarato^1,3, Sanford I. Bernstein³, Rolf Bodmer¹

¹Development and Aging Program, The Sanford Burnham Institute for Medical Research, ²Cardiac Electrophysiology Group, Dept. of Physiology, Anatomy and Genetics, The Sanford Burnham Institute for Medical Research, ³Biology Department and Heart Institute, San Diego State University

We have developed a Semi-automated Optical Heartbeat Analysis method (SOHA) for analyzing high speed optical recordings from Drosophila, zebrafish and embryonic mouse hearts. We demonstrate the application of our methodology to the analysis of heart function in fruit fly and embryonic mouse hearts.

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.

Modified Annexin V/Propidium Iodide Apoptosis Assay For Accurate Assessment of Cell Death

JoVE 2597 4/24/2011

Aja M. Rieger¹, Kimberly L. Nelson¹, Jeffrey D. Konowalchuk¹, Daniel R. Barreda^1,2

¹Department of Biological Sciences, University of Alberta, ²Department of Agriculture, Food and Nutrition Sciences, University of Alberta

An accurate method for the assessment of cell death is described. The protocol improves upon conventional Annexin V/ propidium iodide (PI) protocols, which display up to 40% false- positive events in cell lines and primary cells from a broad range of animal models.