European Molecular Biology Laboratory

10 ARTICLES PUBLISHED IN JoVE

Immunology and Infection

Visualizing Cell-to-cell Transfer of HIV using Fluorescent Clones of HIV and Live Confocal Microscopy

Benjamin Dale¹, Gregory P. McNerney², Deanna L. Thompson², Wolfgang Hübner³, Thomas Huser², Benjamin K. Chen¹

¹Division of Infectious Diseases, Department of Medicine, Immunology Institute, Mount Sinai School of Medicine , ²NSF Center for Biophotonics, University of California, Davis, ³Structural and Computational Biology Unit, European Molecular Biology Laboratory

This visualized experiment is a guide for utilizing a fluorescent molecular clone of HIV for live confocal imaging experiments.

Biochemistry

Online Size-exclusion and Ion-exchange Chromatography on a SAXS Beamline

Martha E. Brennich¹, Adam R. Round^2,3, Stephanie Hutin⁴

¹Structural Biology Group, European Synchrotron Radiation Facility, ²European Molecular Biology Laboratory, ³School of Chemical and Physical Sciences, Keele University, ⁴Groupe de Microscopie Electronique et Méthodes, Institut de Biologie Structurale

The determination of the solution structure of a protein by small angle X-ray scattering (SAXS) requires monodisperse samples. Here, we present two possibilities to ensure minimal delays between sample preparation and data acquisition: online size-exclusion chromatography (SEC) and online ion-exchange chromatography (IEC).

Immunology and Infection

Fabricating Optical-quality Glass Surfaces to Study Macrophage Fusion

James J. Faust^1,2, Wayne Christenson^3,4,5, Kyle Doudrick⁶, John Heddleston⁷, Teng-Leong Chew⁷, Marko Lampe⁸, Arnat Balabiyev^1,2, Robert Ros^3,4,5, Tatiana P. Ugarova^1,2

¹Center for Metabolic and Vascular Biology, Mayo Clinic, ²Molecular and Cellular Biosciences, School of Life Sciences, Arizona State University, ³Department of Physics, Arizona State University, ⁴Center for Biological Physics, Arizona State University, ⁵Biodesign Institute, Arizona State University, ⁶Department of Civil and Environmental Engineering and Earth Sciences, University of Notre Dame, ⁷Advanced Imaging Center, HHMI Janelia Research Campus, ⁸Advanced Light Microscopy Facility, European Molecular Biology Laboratory

This protocol describes the fabrication of optical-quality glass surfaces adsorbed with compounds containing long-chain hydrocarbons that can be used to monitor macrophage fusion of living specimens and enables super-resolution microscopy of fixed specimens.

Bioengineering

Correlative Light Electron Microscopy (CLEM) for Tracking and Imaging Viral Protein Associated Structures in Cryo-immobilized Cells

Rachel Santarella-Mellwig¹, Uta Haselmann², Nicole L. Schieber¹, Paul Walther³, Yannick Schwab¹, Claude Antony¹, Ralf Bartenschlager^2,4, Inés Romero-Brey²

¹European Molecular Biology Laboratory, ²Department of Infectious Diseases, Molecular Virology, Heidelberg University, ³Central Facility for Electron Microscopy, Ulm University, ⁴Heidelberg Partner Site, German Center for Infection Research

A correlative light electron microscopy (CLEM) method is applied to image virus-induced intracellular structures via electron microscopy (EM) in cells that are previously selected by light microscopy (LM). LM and EM are combined as a hybrid imaging approach to achieve an integrated view of virus-host interactions.

Biochemistry

Structure Solution of the Fluorescent Protein Cerulean Using MeshAndCollect

Stephanie Hutin^*1, Gianluca Santoni^*1, Ulrich Zander², Nicolas Foos¹, Sylvain Aumonier¹, Guillaume Gotthard¹, Antoine Royant^1,3, Christoph Mueller-Dieckmann¹, Gordon Leonard¹

¹European Synchrotron Radiation Facility, Structural Biology Group, ²European Molecular Biology Laboratory, ³Univ. Grenoble Alpes, CNRS, CEA, IBS (Institut de Biologie Structurale)

We present the use of the MeshAndCollect protocol to obtain a complete diffraction data set, for use in subsequent structure determination, composed of partial diffraction data sets collected from many small crystals of the fluorescent protein Cerulean.

Chemistry

Exfoliation and Analysis of Large-area, Air-Sensitive Two-Dimensional Materials

Josh P. Thompson¹, M. Hasan Doha¹, Peter Murphy^1,2, Jin Hu^1,3, Hugh O.H. Churchill^1,3

¹Department of Physics, University of Arkansas, ²Department of Physics, SUNY Geneseo, ³Institute for Nanoscale Science and Engineering, University of Arkansas

A method for exfoliating large thin flakes of air sensitive two-dimensional materials and safely transporting them for analysis outside of a glovebox is presented.

Biochemistry

Fully Autonomous Characterization and Data Collection from Crystals of Biological Macromolecules

Stephanie Hutin¹, Bart Van Laer¹, Christoph Mueller-Dieckmann¹, Gordon Leonard¹, Didier Nurizzo¹, Matthew W. Bowler²

¹Structural Biology Group, European Synchrotron Radiation Facility, ²Grenoble Outstation, European Molecular Biology Laboratory

Here, we describe how to use the automated screening and data collection options available at some synchrotron beamlines. Scientists send cryocooled samples to the synchrotron, and the diffraction properties are screened, the data sets are collected and processed and, where possible, a structure solution is carried out—all without human intervention.

Biology

Strategies for Optimization of Cryogenic Electron Tomography Data Acquisition

Felix Weis¹, Wim J. H. Hagen¹, Martin Schorb², Simone Mattei^1,3

¹Structural and Computational Biology Unit, European Molecular Biology Laboratory, ²Electron Microscopy Core Facility, European Molecular Biology Laboratory, ³Imaging Centre, European Molecular Biology Laboratory

The increasing demand for large-scale data collection in cryogenic electron tomography requires high-throughput image acquisition routines. Described here is a protocol that implements the recent developments of advanced acquisition strategies aimed at maximizing the time-efficiency and throughput of tomographic data collection.

Biochemistry

The Automated Crystallography Pipelines at the EMBL HTX Facility in Grenoble

Irina Cornaciu^1,2, Raphael Bourgeas¹, Guillaume Hoffmann¹, Florine Dupeux^1,3, Anne-Sophie Humm¹, Vincent Mariaule¹, Andrea Pica^1,2, Damien Clavel^1,2, Gael Seroul^1,2, Peter Murphy¹, José Antonio Márquez^1,2

¹European Molecular Biology Laboratory, ²ALPX S.A.S., ³Institut de Biologie Structurale

Here, we describe how to use the automated macromolecular crystallography pipelines for protein-to-structure, rapid ligand-protein complex analysis and large-scale fragment screening based on the CrystalDirect technology at the HTX Laboratory in EMBL Grenoble.

Biology

Super-Resolution Microscopy of the Synaptonemal Complex Within the Caenorhabditis elegans Germline

Ivana Čavka^1,2, Rory M. Power³, Dietrich Walsh³, Timo Zimmermann^1,3, Simone Köhler¹

¹Cell Biology and Biophysics, European Molecular Biology Laboratory, ²Collaboration for joint PhD degree between EMBL and Heidelberg University, Faculty of Biosciences, ³EMBL Imaging Centre, European Molecular Biology Laboratory

Super-resolution microscopy can provide a detailed insight into the organization of components within the synaptonemal complex in meiosis. Here, we demonstrate a protocol to resolve individual proteins of the Caenorhabditis elegans synaptonemal complex.