Visualization of Bacterial Toxin Induced Responses Using Live Cell Fluorescence Microscopy

JoVE 4227 10/01/2012

Peter A. Keyel¹, Michelle E. Heid¹, Simon C. Watkins², Russell D. Salter¹

¹Department of Immunology, University of Pittsburgh School of Medicine, ²Department of Cell Biology and Physiology, University of Pittsburgh School of Medicine

Methods for purifying the cholesterol binding toxin streptolysin O from recombinant E. coli and visualization of toxin binding to live eukaryotic cells are described. Localized delivery of toxin induces rapid and complex changes in targeted cells revealing novel aspects of toxin biology.

The Insect Galleria mellonella as a Powerful Infection Model to Investigate Bacterial Pathogenesis

JoVE 4392 12/11/2012

Nalini Ramarao, Christina Nielsen-Leroux, Didier Lereclus

INRA, Micalis UMR1319, France

Oral and intra haemocolic infection of larvae of the greater wax moth Galleria mellonella is described. This insect can be used to study virulence factors of entomopathogenic as well as mammalian opportunistic bacteria. Rearing of the insects, methods of infection and examples of in vivo analysis are described.

A Visual Assay to Monitor T6SS-mediated Bacterial Competition

JoVE 50103 3/20/2013

Abderrahman Hachani, Nadine S. Lossi, Alain Filloux

MRC Centre for Molecular Bacteriology and Infection, Division of Cell and Molecular Biology, Imperial College London

We describe a qualitative assay to monitor bacterial competition mediated by the Pseudomonas aeruginosa type VI secretion system (T6SS). The assay relies on the survival/killing of Escherichia coli target cells carrying a lacZ-reporter. This technique is adjustable to assess the bactericidal/bacteriostasis activity of T6SS-proficient microorganisms.

Electricity-Free, Sequential Nucleic Acid and Protein Isolation

JoVE 4202 5/15/2012

David R. Pawlowski^1,2, Richard J. Karalus^1,2

¹CUBRC, Inc., ²Department of Microbiology and Immunology, State University of New York at Buffalo, School of Medicine and Biomedical Sciences

A tool and chemistries are described to sequentially isolate nucleic acids followed by proteins from a sample without the need for electricity. The tool consists of a sorbent held within a transfer pipette while the isolation chemistries are based on solid-phase extraction principles. The isolated macromolecules can be analyzed by immuno-based and PCR-based assays.

ELIME (Enzyme Linked Immuno Magnetic Electrochemical) Method for Mycotoxin Detection

JoVE 1588 10/23/2009

Daniela Romanazzo, Francesco Ricci, Silvia Vesco, Silvia Piermarini, Giulia Volpe, Danila Moscone, Giuseppe Palleschi

Department of Sciences and Chemical Technologies, University of Rome, Tor Vergata

A protocol to detect trichothecenes (mycotoxins of concern for human health) using a newly developed screening method based on a competitive immunochemical method and a final electrochemical detection is demonstrated.

Ex utero Electroporation and Whole Hemisphere Explants: A Simple Experimental Method for Studies of Early Cortical Development

JoVE 50271 4/03/2013

Anna J. Nichols*, Ryan S. O'Dell*, Teresa A. Powrozek*, Eric C. Olson

Department of Neuroscience and Physiology, SUNY Upstate Medical University

This protocol describes an improved explant procedure that involves ex utero electroporation, dissection and culture of entire cerebral hemispheres from the embryonic mouse. The preparation facilitates pharmacological studies and assays of gene function during early cortical development.

Toxin Induction and Protein Extraction from Fusarium spp. Cultures for Proteomic Studies

JoVE 1690 2/16/2010

Matias Pasquali, Frédéric Giraud, Jean Paul Lasserre, Sebastien Planchon, Lucien Hoffmann, Torsten Bohn, Jenny Renaut

Department of Environment and Agro-Biotechnologies (EVA), Nutrition and Toxicology Unit (NuTox), Centre de Recherche Public-Gabriel Lippmann

Protein extraction for proteomic analyses in fungal species requires high levels of standardization to be accomplished according with the minimum information about a proteomic experiment (MIAPE) guidelines. We present a video-protocol that includes a procedure for minimizing experimental bias during toxin induction and protein extraction from Fusarium spp.

Determination of Lipid Raft Partitioning of Fluorescently-tagged Probes in Living Cells by Fluorescence Correlation Spectroscopy (FCS)

JoVE 3513 4/06/2012

Catherine Marquer¹, Sandrine Lévêque-Fort^2,3, Marie-Claude Potier¹

¹Centre de Recherche de l’Institut du Cerveau et de la Moelle Épinière, Hôpital de la Pitié-Salpêtrière, ²Institut des Sciences Moléculaires d'Orsay, Université Paris-Sud, ³Centre de Photonique Biomédicale du Centre Laser, Université Paris-Sud

A technique to probe the lipid raft partitioning of fluorescent proteins at the plasma membrane of living cells is described. It takes advantage of the disparity in diffusion times of proteins located inside or outside of lipid rafts. Acquisition can be performed dynamically in control conditions or after drug addition.

October 2012: This Month in JoVE

JoVE 5025 10/01/2012

Wendy Chao¹, Aaron Kolski-Andreaco²

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

Here are some highlights from the October 2012 Issue of Journal of Visualized Experiments (JoVE).

2012: A Year In Review

JoVE 5049 1/03/2013

Wendy Chao¹, Aaron Kolski-Andreaco²

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

Here's a look at some of the milestones and highlights of the year 2012 in Journal of Visualized Experiments (JoVE).

TransFLP — A Method to Genetically Modify Vibrio cholerae Based on Natural Transformation and FLP-recombination

JoVE 3761 10/08/2012

Melanie Blokesch

Global Health Institute, School of Life Sciences, Ecole Polytechnique Fédérale de Lausanne (EPFL)

A quick method to modify the genome of V. cholerae is described. These modifications include the deletion of single genes, gene clusters and genomic islands as well as the integration of short sequences (e.g. promoter elements or affinity-tag sequences). The method is based on the natural transformation and FLP-recombination.

High Content Screening in Neurodegenerative Diseases

JoVE 3452 1/06/2012

Shushant Jain¹, Ronald E. van Kesteren², Peter Heutink¹

¹Department of Clinical Genetics, VU University Medical Center, ²Center for Neurogenomics and Cognitive Research, Neuroscience Campus Amsterdam

We describe a methodology combining automated cell culturing with high-content imaging to visualize and quantify multiple cellular processes and structures, in a high-throughput manner. Such methods can aid in the further functional annotation of genomes as well as identify disease gene networks and potential drug targets.

In Vitro Analysis of PDZ-dependent CFTR Macromolecular Signaling Complexes

JoVE 4091 8/13/2012

Yanning Wu¹, Shuo Wang¹, Chunying Li^1,2,3

¹Department of Biochemistry & Molecular Biology, Wayne State University School of Medicine, ²Cardiovascular Research Institute, Wayne State University School of Medicine, ³Barbara Ann Karmanos Cancer Institute, Wayne State University School of Medicine

Cystic fibrosis transmembrane conductance regulator (CFTR), an epithelial chloride channel, has been reported to interact with various proteins and regulate important cellular processes; among them the CFTR PDZ motif-mediated interactions have been well documented. This protocol describes methods we developed to assemble a PDZ-dependent CFTR macromolecular signaling complex in vitro.

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.

Subcutaneous Infection of Methicillin Resistant Staphylococcus Aureus (MRSA)

JoVE 2528 2/09/2011

Ching Wen Tseng, Marisel Sanchez-Martinez, Andrea Arruda, George Y. Liu

Department of Pediatrics, Cedars-Sinai Medical Center

Murine skin and soft tissue infection model is utilized for assessing the virulence function of methicillin resistant Staphylococcus aureus (MRSA) and the host immunological responses. Here, we presented a subcutaneous infection model for skin and soft tissue infection.

Processing of Human Reduction Mammoplasty and Mastectomy Tissues for Cell Culture

JoVE 50011 1/03/2013

Mark A. LaBarge, James C. Garbe, Martha R. Stampfer

Life Science Division, Lawrence Berkeley National Laboratory

A method to process human mammary surgical discard material is described. Processed tissue, in the form of organoids, can be stored frozen indefinitely or placed in culture for long-term growth. This method enables experimental examination of normal human epithelial cell biology, and the effects of exogenous perturbations.

Isolation and Culture of Adult Epithelial Stem Cells from Human Skin

JoVE 2561 3/31/2011

Zhiru Guo, Kyle Draheim, Stephen Lyle

Department of Cancer Biology, University of Massachusetts Medical School

A rapid, robust way of isolating viable adult epithelial stem cells from human skin is described. The method utilizes enzymatic digestion of skin collagen matrix , followed by plucking of hair follicles and isolation of single cell suspensions or tissue fragments for cell culture.

Paired Patch Clamp Recordings from Motor-neuron and Target Skeletal Muscle in Zebrafish

JoVE 2351 11/20/2010

Hua Wen, Paul Brehm

Vollum Institute, Oregon Health and Sciences University

Larval zebrafish represent the first vertebrate model system to allow simultaneous patch clamp recording from a spinal motor-neuron and target skeletal muscle. This video demonstrates the microscopic methods used to identify a segmental CaP motor-neuron and target muscle cells as well as the methodologies for recording from each cell type.

Lentivirus-mediated Genetic Manipulation and Visualization of Olfactory Sensory Neurons in vivo

JoVE 2951 5/22/2011

Benjamin Sadrian, Huaiyang Chen, Qizhi Gong

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

We present a lentiviral technique for genetic manipulation and visualization of single olfactory sensory neuron axon and its terminal arborization in vivo.

Isolation of Basal Cells and Submucosal Gland Duct Cells from Mouse Trachea

JoVE 3731 9/14/2012

Ahmed E. Hegab, Vi Luan Ha, Yasser S. Attiga, Derek W. Nickerson, Brigitte N. Gomperts

Department of Pediatrics, David Geffen School of Medicine at UCLA

Here we demonstrate our protocol for isolation of basal and submucosal gland duct cells from mouse tracheas. We also demonstrate the method of injecting stem cells into the dorsal mouse fat pad to create an in vivo model of submucosal gland regeneration.

Use of Animal Model of Sepsis to Evaluate Novel Herbal Therapies

JoVE 3926 4/11/2012

Wei Li, Shu Zhu, Yusong Zhang, Jianhua Li, Andrew E. Sama, Ping Wang, Haichao Wang

The Feinstein Institute for Medical Research, North Shore – LIJ Health System

Sepsis refers to a systemic inflammatory response syndrome resulting from a microbial infection, and can be simulated by a surgical technique termed cecal ligation and puncture (CLP). Here we describe a method to use CLP-induced animal model to screen medicinal herbs for therapeutic agents.

Invasion of Human Cells by a Bacterial Pathogen

JoVE 2693 3/21/2011

Andrew M. Edwards, Ruth C. Massey

Department of Biology and Biochemistry, University of Bath

A general protocol for the study of invasion of host cells by a bacterial pathogen, focusing on Staphylococcus aureus and human endothelial cells.

Determination of Mitochondrial Membrane Potential and Reactive Oxygen Species in Live Rat Cortical Neurons

JoVE 2704 5/23/2011

Dinesh C. Joshi, Joanna C. Bakowska

Department of Molecular Pharmacology and Experimental Therapeutics, Loyola University Chicago

We demonstrate application of the fluorescence indicator, TMRM, in cortical neurons to determine the relative changes in TMRM fluorescence intensity before and after application of a specific stimulus. We also show application of the fluorescence probe H₂DCF-DA to assess the relative level of reactive oxygen species in cortical neurons.

Hyponeophagia: A Measure of Anxiety in the Mouse

JoVE 2613 5/17/2011

Rob M.J. Deacon

Department of Experimental Psychology, University of Oxford

Mice and rats, due to their innate cautiousness, are initially slow in consuming a novel food, particularly in a novel place. This hyponeophagia can readily be measured in the laboratory, even though laboratory animals are much less anxious than their wild counterparts

In Vitro Assay of Bacterial Adhesion onto Mammalian Epithelial Cells

JoVE 2783 5/16/2011

Jason Letourneau, Cynthia Levesque, Frederic Berthiaume, Mario Jacques, Michael Mourez

Universite de Montreal, Groupe de Recherche sur les Maladies Infectieuses du Porc GREMIP, Faculte de medecine veterinaire

This protocol is a simple bacterial adhesion assay consisting in counting the numbers of bacterial colony forming units that are adhered onto cultured cells. The assay is robust, independent of the adhesin studied, and numerous variations are used in most laboratories working on bacterial pathogenesis.

A New High Sensitivity Tandem Quadrupole Mass Spectrometer for Quantitative LC/MS/MS Analysis of Low Exposure Pharmaceuticals - ADVERTISEMENT

JoVE 2266 6/15/2010

Robert S. Plumb

Pharmaceutical Business Operations, Waters Corporation

Assessing Neurodegenerative Phenotypes in Drosophila Dopaminergic Neurons by Climbing Assays and Whole Brain Immunostaining

JoVE 50339 4/24/2013

Maria Cecilia Barone, Dirk Bohmann

Department of Biomolecular Genetics, University of Rochester Medical Center

Here we describe two assays that have been established to study age-dependent neurodegeneration of dopaminergic (DA) neurons in Drosophila: the climbing/startle-induced negative geotaxis assay which allows to study the functional effects of DA neurons degeneration and the tyrosine hydroxylase immunostaining which is used to identify and count DA neurons in whole brain mounts.

A Neuronal and Astrocyte Co-Culture Assay for High Content Analysis of Neurotoxicity

JoVE 1173 5/05/2009

Janet L Anderl, Stella Redpath, Andrew J Ball

Bioscience Division, High Content Analysis Research and Development, Millipore Inc

This article describes a novel protocol and reagent set designed for sensitive measurement of neurotoxic effects of compounds and treatments on co-cultures of neurons and astrocytes using high content analysis. Results demonstrate that high content analysis represents an exciting novel technology for neurotoxicity assessment.

Subcutaneous Administration of Muscarinic Antagonists and Triple-Immunostaining of the Levator Auris Longus Muscle in Mice

JoVE 3124 9/08/2011

Megan Wright¹, Amy Kim², Young-Jin Son³

¹Biology Department, Arcadia University, ²Shriners Hospitals Pediatric Research Center, Temple University School of Medicine, ³Shriners Hospitals Pediatric Research Center and Department of Anatomy and Cell Biology, Temple University School of Medicine

We describe procedures for repeated administration of inhibitors of muscarinic signaling to the levator auris longus (LAL) muscle of young adult mice and for subsequent immunostaining of its neuromuscular junctions (NMJs) in wholemounts. The LAL muscle has unique advantages for revealing in vivo pharmacological effects on NMJs.

On-chip Isotachophoresis for Separation of Ions and Purification of Nucleic Acids

JoVE 3890 3/02/2012

Giancarlo Garcia-Schwarz, Anita Rogacs, Supreet S. Bahga, Juan G. Santiago

Mechanical Engineering, Stanford University

Isotachophoresis (ITP) is a robust electrokinetic separation and preconcentration technique with applications ranging from toxin detection to sample preparation. We review the physical principles of ITP and the methodology of applying this technique to two specific example applications: separation and detection of small molecules and purification of nucleic acids from cell culture lysate.

Isolation of Mouse Respiratory Epithelial Cells and Exposure to Experimental Cigarette Smoke at Air Liquid Interface

JoVE 2513 2/21/2011

Hilaire C. Lam^1,2, Augustine M.K. Choi¹, Stefan W. Ryter¹

¹Department of Medicine, Pulmonary and Critical Care Medicine, Brigham and Women’s Hospital, Harvard Medical School, ²Cellular and Molecular Pathology, School of Medicine, University of Pittsburgh

Pulmonary epithelial cells can be isolated from the respiratory tract of mice and cultured at air-liquid interface as a model of differentiated respiratory epithelium. A protocol is described for isolating, culturing and exposing these cells to mainstream cigarette smoke, in order to study molecular responses to this environmental toxin.

Accurate and Simple Measurement of the Pro-inflammatory Cytokine IL-1β using a Whole Blood Stimulation Assay

JoVE 2662 3/01/2011

Barbara Yang*¹, Tuyet-Hang Pham*², Raphaela Goldbach-Mansky², Massimo Gadina¹

¹Translational Immunology Section, Office of Science and Technology, National Institute of Arthritis and Musculoskeletal and Skin Diseases, ²Translational Autoinflammatory Disease Section, Office of the Clinical Director, National Institute of Arthritis and Musculoskeletal and Skin Diseases

We describe a simple immunoassay to measure the production of pro-inflammatory cytokines, such as IL-1 beta production, in patients presenting with autoinflammatory phenotypes. By activating cells in whole blood cultures with pathogen-associated molecular patterns, specifically with lipopolysaccharide, cytokine secretion can be conveniently evaluated in whole blood supernatants.

IgY Technology: Extraction of Chicken Antibodies from Egg Yolk by Polyethylene Glycol (PEG) Precipitation

JoVE 3084 5/01/2011

Diana Pauly¹, Pablo A. Chacana², Esteban G. Calzado³, Björn Brembs⁴, Rüdiger Schade⁵

¹Center for Biological Security, Robert Koch-Institute, ²CICVyA - INTA Castelar, Instituto de Virología, ³Center of Molecular Immunology, Ciudad de la Habana, Cuba, ⁴Department of Biology, Chemistry, Pharmacy, Institute of Biology-Neurobiology, Free University of Berlin, ⁵Institut of Pharmacology, Charité-University Medicine of Berlin

This protocol describes in particular the extraction of total IgY from egg yolk by means of polyethylene glycol precipitation and gives general information about IgY technology.

Catheterization of Intestinal Loops in Ruminants

JoVE 1301 6/11/2009

Richard R. E. Uwiera¹, John P. Kastelic², G. Douglas Inglis²

¹Department of Agricultural, Food and Nutritional Science, University of Alberta, ²Agriculture and Agri-Food Canada, Lethbridge Research Centre, Lethbridge

We describe a novel surgical method for catheterizing 'intestinal loops' within the ileum of sheep. Once animals have recovered from surgery and have cleared antibiotics and analgesics, multiple treatments can be deposited directly in loops via the catheters.

Rearing and Injection of Manduca sexta Larvae to Assess Bacterial Virulence

JoVE 4295 12/11/2012

Elizabeth Hussa, Heidi Goodrich-Blair

Department of Bacteriology, University of Wisconsin-Madison

The method described here utilizes direct injection of entomopathogenic bacteria into the hemocoel of Manduca sexta insect larvae. M. sexta is a commercially available and well-studied insect. Thus, this method represents a simple approach to analyzing host-bacterial interactions from the perspective of one or both partners.

Microgavage of Zebrafish Larvae

JoVE 4434 2/20/2013

Jordan L. Cocchiaro, John F. Rawls

Department of Cell and Molecular Physiology, University of North Carolina at Chapel Hill

We present a novel method for microgavage of larval zebrafish utilizing standard embryo microinjection and stereomicroscopy equipment. We demonstrate that microgavage is a safe and efficient technique useful for delivering controlled amounts of diverse materials specifically into the larval zebrafish intestinal lumen.

December 2012: This Month in JoVE

JoVE 5047 12/03/2012

Wendy Chao¹, Aaron Kolski-Andreaco²

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

Here are some highlights from the December 2012 Issue of Journal of Visualized Experiments (JoVE).

A Fluorescent Screening Assay for Identifying Modulators of GIRK Channels

JoVE 3850 4/24/2012

Maribel Vazquez, Charity A. Dunn, Kenneth B. Walsh

Department of Pharmacology, Physiology & Neuroscience, University of South Carolina, School of Medicine

A real-time screening procedure for identifying drugs that interact with G protein-gated inward rectifier K⁺ (GIRK) channels is described. The assay utilizes membrane potential-sensitive fluorescent dyes to measure GIRK channel activity. This technique is adaptable for use on a number of cell lines.

Bioluminescent Bacterial Imaging In Vivo

JoVE 4318 11/04/2012

Chwanrow K. Baban*, Michelle Cronin*, Ali R. Akin, Anne O'Brien, Xuefeng Gao, Sabin Tabirca, Kevin P. Francis, Mark Tangney

Cork Cancer Research Centre, BioSciences Institute, University College Cork

This article describes the administration of lux-tagged bacteria to mice and subsequent in vivo analysis using IVIS bioluminescence imaging.

Oral Administration of Rotenone using a Gavage and Image Analysis of Alpha-synuclein Inclusions in the Enteric Nervous System

JoVE 2123 10/26/2010

Francisco J. Pan-Montojo, Richard H.W. Funk

Institute of Anatomy, Technische Universität Dresden

Parkinson's disease has been related to the exposure to pesticides. Here we show a method to deliver pesticides using a gastric tube at the desired concentration and a method to analyze their effect in alpha-synuclein accumulation in the enteric nervous system.

Analysis of SNARE-mediated Membrane Fusion Using an Enzymatic Cell Fusion Assay

JoVE 4378 10/19/2012

Nazarul Hasan, David Humphrey, Krista Riggs, Chuan Hu

Department of Biochemistry and Molecular Biology, University of Louisville School of Medicine

We have developed a cell fusion assay that quantifies SNARE-mediated membrane fusion events by activated expression of β-galactosidase.

Analysis of Gene Expression in Emerald Ash Borer (Agrilus planipennis) Using Quantitative Real Time-PCR

JoVE 1974 5/04/2010

Binny Bhandary, Swapna Priya Rajarapu, Loren Rivera-Vega, Omprakash Mittapalli

Department of Entomology, The Ohio State University

Quantitative real-time PCR (qRT-PCR) is an effective tool to diagnose mRNA levels in different insect tissues and developmental stages. In this report we show the use of qRT-PCR to ascertain mRNA levels in different larval tissues and developmental stages of the invasive insect species, emerald ash borer.

Revealing Neural Circuit Topography in Multi-Color

JoVE 3371 11/14/2011

Stacey L. Reeber, Samrawit A. Gebre, Nika Filatova, Roy V. Sillitoe

Dominick P. Purpura Department of Neuroscience, Albert Einstein College of Medicine, Yeshiva University

We provide a practical guide for delivering tracers in vivo and use the spinocerebellar pathway as a model system to demonstrate essential steps for successful neuronal circuit analysis in mice. We describe in detail our versatile tracing protocol that exploits wheat germ agglutinin (WGA) conjugated to Alexa fluorophores.

FSL Constructs: A Simple Method for Modifying Cell/Virion Surfaces with a Range of Biological Markers Without Affecting their Viability

JoVE 3289 8/05/2011

Deborah A. Blake¹, Nicolai V. Bovin², Dan Bess¹, Stephen M. Henry¹

¹Biotechnology Research Institute, AUT University and KODE Biotech Ltd, ²Shemyakin Institute of Bioorganic Chemistry RAS, Moscow, Russia

Function-Spacer-Lipid (FSL) constructs allow the surface characteristics of living cells and virions to be modified without loss of vitality. The method requires only simple contact of an FSL construct solution with a cell/virion and spontaneous and stable surface incorporation occurs.

Demonstrating the Uses of the Novel Gravitational Force Spectrometer to Stretch and Measure Fibrous Proteins

JoVE 2624 3/19/2011

James W. Dunn, Douglas D. Root

Department of Biological Sciences, University of North Texas

This is a step-by step guide showing the purpose, operation, and representative results from the novel gravitational force spectrometer.

Non-surgical Intratracheal Instillation of Mice with Analysis of Lungs and Lung Draining Lymph Nodes by Flow Cytometry

JoVE 2702 5/02/2011

Manira Rayamajhi¹, Elizabeth F. Redente², Tracy V. Condon¹, Mercedes Gonzalez-Juarrero³, David W.H. Riches^1,2,4, Laurel L. Lenz^1,4

¹Department of Immunology, University of Colorado School of Medicine, ²Division of Cell Biology, Department of Pediatrics, National Jewish Health, ³Department of Microbiology, Immunology, and Pathology, Colorado State University, ⁴Department of Immunology, National Jewish Health

We illustrate non-surgical delivery of test materials into the lungs of anesthetized mice via the trachea. This method permits lung exposure to bacterial and viral pathogens, cytokines, antibodies, beads, chemicals, or dyes. We further describe harvesting and processing of lungs and lung draining lymph nodes (LDLNs) for flow cytometry.