Non-invasive Optical Imaging of the Lymphatic Vasculature of a Mouse

JoVE 4326 3/08/2013

Holly A. Robinson, SunKuk Kwon, Mary A. Hall, John C. Rasmussen, Melissa B. Aldrich, Eva M. Sevick-Muraca

Center for Molecular Imaging (CMI), University of Texas Health Science Center-Houston

Recently developed imaging techniques using near-infrared fluorescence (NIRF) may help elucidate the role the lymphatic system plays in cancer metastasis, immune response, wound repair, and other lymphatic-associated diseases.

In vivo Near Infrared Fluorescence (NIRF) Intravascular Molecular Imaging of Inflammatory Plaque, a Multimodal Approach to Imaging of Atherosclerosis

JoVE 2257 8/04/2011

Marcella A. Calfon¹, Amir Rosenthal^1,2, Georgios Mallas^1,3, Adam Mauskapf¹, R. Nika Nudelman², Vasilis Ntziachristos², Farouc A. Jaffer¹

¹Cardiovascular Research Center and Cardiology Division, Massachusetts General Hospital, Harvard Medical School, ²Institute for Biological and Medical Imaging, Helmholtz Zentrum München und Technische Universität München, ³Department of Electrical and Computer Engineering, Northeastern University

We detail a new near-infrared fluorescence (NIRF) catheter for 2-dimensional intravascular molecular imaging of plaque biology in vivo. The NIRF catheter can visualize key biological processes such as inflammation by reporting on the presence of plaque-avid activatable and targeted NIR fluorochromes. The catheter utilizes clinical engineering and power requirements and is targeted for application in human coronary arteries. The following research study describes a multimodal imaging strategy that utilizes a novel in vivo intravascular NIRF catheter to image and quantify inflammatory plaque in proteolytically active inflamed rabbit atheromata.

March 2013: This Month in JoVE

JoVE 5066 3/01/2013

Wendy Chao¹, Aaron Kolski-Andreaco²

¹Department of Ophthalmology, Massachusetts Eye and Ear, ²JoVE Content Production

Here are some highlights from the March 2013 issue of Journal of Visualized Experiments (JoVE).

Fluorescent Nanoparticles for the Measurement of Ion Concentration in Biological Systems

JoVE 2896 7/04/2011

J. Matthew Dubach¹, Mary K. Balaconis¹, Heather A. Clark²

¹Bioengineering Department, Northeastern University, ²Department of Pharmaceutical Sciences, Northeastern University

Fluorescent nanoparticles produced in our lab are used for imaging ion concentrations and ion fluxes in biological systems such as cells during signaling and interstitial fluid during physiological homeostasis.

Tracking Dynamics of Muscle Engraftment in Small Animals by In Vivo Fluorescent Imaging

JoVE 1388 9/21/2009

Zhong Yang¹, Qing Zeng², Zhiyuan Ma¹, Yaming Wang¹, Xiaoyin Xu²

¹Department of Anesthesia, Brigham and Woman's Hospital, ²Department of Radiology, Brigham and Woman's Hospital

We describe an in vivo fluorescence imaging protocol to monitor muscle regeneration by GFP-labeled myoblasts after transplantation into skeletal muscles of both healthy and dystrophic mice. This protocol can be adapted to study muscle regeneration by transplantation of other types of cells and in other muscular conditions as well.

Labeling Stem Cells with Fluorescent Dyes for non-invasive Detection with Optical Imaging

JoVE 686 4/02/2008

Sophie Boddington, Tobias D. Henning, Elizabeth J. Sutton, Heike E. Daldrup-Link

Contrast Agent Research Group at the Center for Molecular and Functional Imaging, Department of Radiology, University of California San Francisco

This video shows techniques for labeling of human embryonic stem cells and mesenchymal stem cells with fluorescent dyes. This technique can be used for an in vivo tracking of transplanted stem cells with optical imaging and for histopathological correlations with fluorescence microscopy.

Viral Nanoparticles for In vivo Tumor Imaging

JoVE 4352 11/16/2012

Amy M. Wen¹, Karin L. Lee¹, Ibrahim Yildiz¹, Michael A. Bruckman¹, Sourabh Shukla¹, Nicole F. Steinmetz²

¹Department of Biomedical Engineering, Case Western Reserve University, ²Department of Biomedical Engineering, Radiology, and Materials Science and Engineering, Case Western Reserve University

Plant viral nanoparticles (VNPs) are promising platforms for applications in biomedicine. Here, we describe the procedures for plant VNP propagation, purification, characterization, and bioconjugation. Finally, we show the application of VNPs for tumor homing and imaging using a mouse xenograft model and fluorescence imaging.

Near Infrared Optical Projection Tomography for Assessments of β-cell Mass Distribution in Diabetes Research

JoVE 50238 1/12/2013

Anna U. Eriksson*¹, Christoffer Svensson*¹, Andreas Hörnblad¹, Abbas Cheddad¹, Elena Kostromina¹, Maria Eriksson¹, Nils Norlin¹, Antonello Pileggi², James Sharpe³, Fredrik Georgsson⁴, Tomas Alanentalo¹, Ulf Ahlgren¹

¹Umeå Centre for Molecular Medicine, Umeå University, ²Cell Transplant Center, Diabetes Research Institute, University of Miami,, ³EMBL-CRG Systems Biology Program, Centre for Genomic Regulation, Catalan Institute of Research and Advanced Studies, ⁴Dept. of Computing Science, Umeå University

We describe the adaptation of optical projection tomography (OPT)¹ to imaging in the near infrared spectrum, and the implementation of a number of computational tools. These protocols enable assessments of pancreatic β-cell mass (BCM) in larger specimens, increase the multichannel capacity of the technique and increase the quality of OPT data.

Single Cell Fate Mapping in Zebrafish

JoVE 3172 10/05/2011

Vikram Kohli¹, Kira Rehn¹, Saulius Sumanas^1,2

¹Division of Developmental Biology, Cincinnati Children's Hospital Medical Center, ²Division of Hematology/Oncology, Cincinnati Children's Hospital Medical Center

A method is described to photoactivate single cells containing a caged fluorescent protein using two-photon absorption from a Ti:Sapphire femtosecond laser oscillator. To fate map the photoactivated cell, immunohistochemistry is used. This technique can be applied to any cell type.

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.

Nano-fEM: Protein Localization Using Photo-activated Localization Microscopy and Electron Microscopy

JoVE 3995 12/03/2012

Shigeki Watanabe, Jackson Richards, Gunther Hollopeter, Robert J. Hobson, Wayne M. Davis, Erik M. Jorgensen

Department of Biology, Howard Hughes Medical Institute, University of Utah

We describe a method to localize fluorescently tagged proteins in electron micrographs. Fluorescence is first localized using photo-activated localization microscopy on ultrathin sections. These images are then aligned to electron micrographs of the same section.

Computed Tomography-guided Time-domain Diffuse Fluorescence Tomography in Small Animals for Localization of Cancer Biomarkers

JoVE 4050 7/17/2012

Kenneth M. Tichauer¹, Robert W. Holt², Kimberley S. Samkoe³, Fadi El-Ghussein¹, Jason R. Gunn¹, Michael Jermyn¹, Hamid Dehghani⁴, Frederic Leblond¹, Brian W. Pogue^1,2

¹Thayer School of Engineering, Dartmouth College, ²Department of Physics and Astronomy, Dartmouth College, ³Darmouth Medical School, Dartmouth College, ⁴School of Computer Science, University of Birmingham

Diffuse fluorescence tomography offers a relatively low-cost and potentially high-throughout approach to preclinical in vivo tumor imaging. The methodology of optical data collection, calibration, and image reconstruction is presented for a computed tomography-guided non-contact time-domain system using fluorescent targeting of the tumor biomarker epidermal growth factor receptor in a mouse glioma model.

Multispectral Real-time Fluorescence Imaging for Intraoperative Detection of the Sentinel Lymph Node in Gynecologic Oncology

JoVE 2225 10/20/2010

Lucia M.A. Crane¹, George Themelis², K. Tim Buddingh¹, Niels J. Harlaar¹, Rick G. Pleijhuis¹, Athanasios Sarantopoulos², Ate G.J. van der Zee³, Vasilis Ntziachristos², Gooitzen M. van Dam¹

¹Department of Surgery, Division of Surgical Oncology, University Medical Center Groningen, ²Helmholtz Zentrum, Technical University Munich, ³Department of Obstetrics and Gynaecology, University Medical Center Groningen

Fluorescence imaging is a promising innovative modality for image-guided surgery in surgical oncology. In this video we describe the technical procedure for detection of the sentinel lymph node using fluorescence imaging as showcased in gynecologic oncologicy. A multispectral fluorescence camera system, together with the fluorescent agent indocyanine green, is applied.

In vivo Neuronal Calcium Imaging in C. elegans

JoVE 50357 4/10/2013

Samuel H. Chung*^1,2, Lin Sun*^1,2, Christopher V. Gabel^1,2

¹Department of Physiology and Biophysics, Boston University School of Medicine, ²Boston University Photonics Center

With its small transparent body, well-documented neuroanatomy and a host of amenable genetic techniques and reagents, C. elegans makes an ideal model organism for in vivo neuronal imaging using relatively simple, low-cost techniques. Here we describe single neuron imaging within intact adult animals using genetically encoded fluorescent calcium indicators.

Quantification of dsDNA using the Hitachi F-7000 Fluorescence Spectrophotometer and PicoGreen Dye

JoVE 2465 11/05/2010

Luis A. Moreno, Kendra L. Cox

Life Sciences Group, Hitachi High Technologies America

Demonstration of quantification of dsDNA using Molecular Probes PicoGreen dye and Hitachi F-7000 Fluorescence Spectrophotometer equipped with a microplate reader accessory.

Cut-loading: A Useful Tool for Examining the Extent of Gap Junction Tracer Coupling Between Retinal Neurons

JoVE 3180 1/12/2012

Hee Joo Choi¹, Christophe P. Ribelayga², Stuart C. Mangel¹

¹Department of Neuroscience, Ohio State University College of Medicine, ²Department of Ophthalmology and Visual Science, University of Texas Medical School

An easy and convenient method to determine the extent of gap junction tracer coupling between retinal neurons is described. This technique enables one to investigate the function of the electrical synapses between neurons in the intact retina under different illumination conditions and at different times of the day and night.

Rejection of Fluorescence Background in Resonance and Spontaneous Raman Microspectroscopy

JoVE 2592 5/18/2011

Zachary J. Smith*¹, Florian Knorr*¹, Cynthia V. Pagba¹, Sebastian Wachsmann-Hogiu^1,2

¹Center for Biophotonics Science and Technology, University of California, Davis, ²Department of Pathology and Laboratory Medicine, University of California, Davis

We discuss the construction and operation of a complex nonlinear optical system that uses ultrafast all-optical switching to isolate Raman from fluorescence signals. Using this system we are able to successfully separate Raman and fluorescence signals utilizing pulse energies and average powers that remain biologically safe.

Voltage-sensitive Dye Recording from Axons, Dendrites and Dendritic Spines of Individual Neurons in Brain Slices

JoVE 4261 11/29/2012

Marko Popovic, Xin Gao, Dejan Zecevic

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

An imaging technique for monitoring of membrane potential changes with sub-micrometer spatial and sub-millisecond temporal resolution is described. The technique, based on laser excitation of voltage-sensitive dyes, allows measurements of signals in axons and axon collaterals, terminal dendritic branches, and individual dendritic spines.

Transplantation into the Anterior Chamber of the Eye for Longitudinal, Non-invasive In vivo Imaging with Single-cell Resolution in Real-time

JoVE 50466 3/10/2013

Midhat H. Abdulreda^1,2, Alejandro Caicedo^1,3,4, Per-Olof Berggren^1,5

¹Diabetes Research Institute, University of Miami Miller School of Medicine, ²Department of Surgery, University of Miami Miller School of Medicine, ³Department of Medicine, University of Miami Miller School of Medicine, ⁴Department of Physiology & Biophysics, University of Miami Miller School of Medicine, ⁵The Rolf Luft Research Center for Diabetes and Endocrinology, Karolinska Institutet

A new approach combining intraocular transplantation and confocal microscopy enables longitudinal, non-invasive real-time imaging with single-cell resolution within grafted tissues in vivo. We demonstrate how to transplant pancreatic islets into the anterior chamber of the mouse eye.

Live Cell Imaging of F-actin Dynamics via Fluorescent Speckle Microscopy (FSM)

JoVE 1325 8/05/2009

James Lim, Gaudenz Danuser

Department of Cell Biology, Scripps Institute

Selection, microinjection, and imaging of fluorescently-labeled F-actin via fluorescent speckle microscopy (FSM).

The 2009 Lindau Nobel Laureate Meeting: Roger Y. Tsien, Chemistry 2008

JoVE 1575 1/13/2010

Roger Y. Tsien

American biochemist Roger Tsien shared the 2008 Nobel Prize in Chemistry with Martin Chalfie and Osamu Shimomura for their discovery and development of the Green Fluorescent Protein (GFP). Tsien dramatically improved the wild-type GFP resulting in increased fluorescence, increased photostability, and a shift in the major excitation peak to 488 nm (matching FITC).

Patch-clamp Capacitance Measurements and Ca²⁺ Imaging at Single Nerve Terminals in Retinal Slices

JoVE 3345 1/19/2012

Mean-Hwan Kim, Evan Vickers, Henrique von Gersdorff

The Vollum Institute, Oregon Health and Science University

Here we describe a protocol for the preparation of agar-embedded retinal slices that are suitable for electrophysiology and Ca²⁺ imaging. This method allows one to study ribbon-type synapses in retinal microcircuits using direct patch-clamp recordings of single presynaptic nerve terminals.