Cecal Ligation Puncture Procedure

JoVE 2860 5/07/2011

Miguel G. Toscano¹, Doina Ganea¹, Ana M. Gamero²

¹Department of Microbiology and Immunology School of Medicine, Temple University, ²Department of Biochemistry, School of Medicine, Temple University

The mouse model of cecal ligation and puncture as a valuable tool for the study of human sepsis.

On-Chip Endothelial Inflammatory Phenotyping

JoVE 4169 7/21/2012

J. Sherrod DeVerse*, Keith A. Bailey*, Greg A. Foster, Vaishali Mittal, Stuart M. Altman, Scott I. Simon, Anthony G. Passerini

Department of Biomedical Engineering, University of California, Davis

Microfluidic flow chambers etched by photolithography and fabricated from PDMS are applied to probe functional outcomes associated with EC dysfunction and inflammation. In a representative experiment, the ability of differential shear stress to modulate monocytic cell adhesion to cytokine activated EC monolayers is demonstrated.

A Quantitative Evaluation of Cell Migration by the Phagokinetic Track Motility Assay

JoVE 4165 12/04/2012

Maciej T. Nogalski^1,2, Gary C.T. Chan³, Emily V. Stevenson^1,2, Donna K. Collins-McMillen^1,2, Andrew D. Yurochko^1,2,4

¹Department of Microbiology and Immunology, Louisiana State University Health Sciences Center, ²Center for Molecular and Tumor Virology, Louisiana State University Health Sciences Center, ³Department of Microbiology and Immunology, SUNY Upstate Medical University, ⁴Feist-Weiller Cancer Center, Louisiana State University Health Sciences Center

The phagokinetic motility track assay is a method used to assess the movement of cells. Specifically, the assay measures chemokinesis (random cell motility) over time in a quantitative manner. The assay takes advantage of the ability of cells to create a measurable track of their movement on colloidal gold-coated coverslips.

Methods Development for Blood Borne Macrophage Carriage of Nanoformulated Antiretroviral Drugs

JoVE 2460 12/09/2010

Shantanu Balkundi*, Ari S. Nowacek*, Upal Roy, Andrea Martinez-Skinner, JoEllyn McMillan, Howard E. Gendelman

Department of Pharmacology and Experimental Neuroscience, University of Nebraska Medical Center

Nanoparticles of indinavir, ritonavir, efavirenz and atazanavir were manufactured using wet milling, homogenization and ultrasonication. These nanoformulations, collectively termed nanoformulated antiretroviral therapy (nanoART), assessed macrophage-based drug delivery. Monocyte-derived macrophage nanoART uptake, retention and sustained release were determined. These preliminary studies suggest the potential of nanoART for clinical use.

A Functional Whole Blood Assay to Measure Viability of Mycobacteria, using Reporter-Gene Tagged BCG or M.Tb (BCG lux/M.Tb lux)

JoVE 3332 9/14/2011

Sandra Newton¹, Adrian Martineau², Beate Kampmann¹

¹Department of Paediatrics, Imperial College London, ²Centre for Health Sciences, Barts & The London School of Medicine and Dentistry

We describe an alternative approach to the enumeration of mycobacteria in vitro, which uses reporter-gene tagged mycobacteria instead of colony-forming units (CFU). “Survival” of organisms as well as host response-markers are measured simultaneously, providing a low-cost, versatile and functional system for studies of host/pathogen interactions in the context of tuberculosis.

Isolation of Brain-infiltrating Leukocytes

JoVE 2747 6/13/2011

Reghann G. LaFrance-Corey*, Charles L. Howe*

Department of Neurology, Mayo Clinic College of Medicine

A rapid method to obtain infiltrating leukocytes from the murine brain is described. This method utilizes a continuous Percoll gradient and discontinuous Ficoll gradient to select and purify the leukocyte-enriched layer. Isolated leukocytes may then be characterized by flow cytometric measurements.

Enumeration of Major Peripheral Blood Leukocyte Populations for Multicenter Clinical Trials Using a Whole Blood Phenotyping Assay

JoVE 4302 9/16/2012

Tiffany R. Hensley, Austin B. Easter, Sarah E. Gerdts, Stephen C. De Rosa, Antje Heit, M. Juliana McElrath, Erica Andersen-Nissen

Vaccine and Infectious Disease Division, Fred Hutchinson Cancer Research Center

In this report, we demonstrate the staining and analysis steps of a phenotyping assay performed on fresh whole blood to enumerate major innate and adaptive leukocyte populations. We emphasize considerations for performing these procedures in the context of a multicenter clinical trial.

Collecting and Measuring Nociceptive and Inflammatory Mediators in Surgical Wounds

JoVE 962 10/29/2008

Brendan Carvalho, David J. Clark, David Yeomans, Martin S. Angst

Department of Anesthesiology, Stanford University School of Medicine

A technique to collect and measure surgical wound biochemical mediators at specific time points.

Optimized Protocol for Efficient Transfection of Dendritic Cells without Cell Maturation

JoVE 2766 7/08/2011

Robert Bowles*, Sonali Patil*, Hanna Pincas, Stuart C. Sealfon

Center for Translational Systems Biology and Department of Neurology, Mount Sinai School of Medicine

We present our optimized high-throughput nucleofection protocol as an efficient way of transfecting primary human monocyte-derived dendritic cells with either plasmid DNA or siRNA without causing cell maturation. We further provide evidence for successful siRNA silencing of targeted gene RIG-I at both the mRNA and protein levels.

Quantitative Imaging of Lineage-specific Toll-like Receptor-mediated Signaling in Monocytes and Dendritic Cells from Small Samples of Human Blood

JoVE 3741 4/16/2012

Feng Qian, Ruth R. Montgomery

Department of Internal Medicine, Yale University School of Medicine

We describe use of ImageStream technology (www.amnis.com), which combines quantitative flow cytometry with simultaneous high-resolution digital imaging, to quantify cellular mechanisms of primary immune cells from well-defined patient cohorts. Our studies provide a blueprint for translational investigations to quantify lineage specific cellular responses in small samples from subject cohorts.

Cholesterol Efflux Assay

JoVE 3810 3/06/2012

Hann Low, Anh Hoang, Dmitri Sviridov

Baker IDI Heart and Diabetes Institute

The cholesterol assay is designed to quantitate the rate of cholesterol efflux from cultured cells and the capacity of plasma acceptors to accept cholesterol released from cells. The assay consists of labelling cells with cholesterol, equilibration of cholesterol among intracellular pools and release of cholesterol to an extracellular acceptor.

CD4+ T-Lymphocyte Capture Using a Disposable Microfluidic Chip for HIV

JoVE 315 10/01/2007

Sang Jun Moon¹, Richard Lin², Utkan Demirci¹

¹Bio-Acoustic-MEMS Laboratory in Medicine (BAMM), HST-Center for Bioengineering, Brigham and Women's Hospital, ²Massachusetts Institute of Technology

An In vitro Co-infection Model to Study Plasmodium falciparum-HIV-1 Interactions in Human Primary Monocyte-derived Immune Cells

JoVE 4166 8/15/2012

Guadalupe Andreani, Dominic Gagnon, Robert Lodge, Michel J. Tremblay, Dave Richard

Infectious Disease Research Center, CHUL (CHUQ), Quebec City, Quebec, Canada

We have developed an in vitro malaria-HIV-1 co-infection model to study the impact of Plasmodium falciparum on the HIV-1 replicative cycle in human primary monocyte-derived macrophages. This versatile system can easily be adapted to other primary cell types susceptible to HIV-1 infection.

A Thin-skull Window Technique for Chronic Two-photon In vivo Imaging of Murine Microglia in Models of Neuroinflammation

JoVE 2059 9/19/2010

Daniel F. Marker*¹, Marie-Eve Tremblay*², Shao-Ming Lu¹, Ania K. Majewska², Harris A. Gelbard¹

¹Center for Neural Development and Disease, Department of Neurology, Child Neurology Division, University of Rochester, ²Department of Neurobiology and Anatomy, University of Rochester

We describe a method for repeatedly visualizing murine microglia and circulating monocytes in vivo over hours, days or weeks using transcranial two-photon microscopy. We demonstrate how to prepare a thinned-skull window that allows intermittent observation of quiescent microglia that can be activated by adjacent stereotactic injection of the HIV-1 regulatory protein Tat.

Murine Model of Hindlimb Ischemia

JoVE 1035 1/21/2009

Hiroshi Niiyama¹, Ngan F. Huang¹, Mark D. Rollins², John P. Cooke¹

¹Division of Cardiovascular Medicine, Stanford University, ²Department of Anesthesiology, University of California, San Francisco

The surgical procedure for induction of unilateral hindlimb ischemia is demonstrated, with confirmation of ischemia by laser Doppler perfusion imaging.

Collecting And Measuring Wound Exudate Biochemical Mediators In Surgical Wounds

JoVE 50133 10/20/2012

Brendan Carvalho, David J Clark, David Yeomans, Martin S Angst

Department of Anesthesia, Stanford University School of Medicine

This article provides a detailed and visual description of a methodology for collecting and measuring biochemical inflammatory and nociceptive mediators at the surgical wound site following cesarean delivery. This human bioassay has been used to determine correlations between wound and serum cytokine concentrations and drug-mediated changes in wound cytokines, chemokines and neuropetides.

Differentiating Functional Roles of Gene Expression from Immune and Non-immune Cells in Mouse Colitis by Bone Marrow Transplantation

JoVE 4208 10/01/2012

Hon Wai Koon, Samantha Ho, Michelle Cheng, Ryan Ichikawa, Charalabos Pothoulakis

Center for Inflammatory Bowel Diseases, Division of Digestive Diseases, David Geffen School of Medicine, The University of California Los Angeles, Los Angeles

Bone marrow transplantation provides a way to change the genotype of the bone marrow derived cells. If the gene of interest is expressed in both bone marrow derived cells and non-bone marrow derived cells, bone marrow transplantation can change the bone marrow derived cells to a different genotype without changing the non-bone marrow derived cell genotype.

Serial Enrichment of Spermatogonial Stem and Progenitor Cells (SSCs) in Culture for Derivation of Long-term Adult Mouse SSC Lines

JoVE 50017 2/25/2013

Laura A. Martin, Marco Seandel

Department of Surgery, Weill Cornell Medical College

A simple method to derive and maintain spermatogonial stem and progenitor cell lines from adult mice is presented here. The method utilizes feeder cells originating from the somatic cell compartment of the adult mouse testis. This technique is applicable to common mouse strains, including transgenic, knock-out, and knock-in mice.

Comprehensive & Cost Effective Laboratory Monitoring of HIV/AIDS: an African Role Model

JoVE 2312 10/31/2010

Denise Lawrie^1,2, George Janossy², Maarten Roos³, Deborah K. Glencross^1,2

¹National Health Laboratory Services (NHLS-SA), ²Department of Molecular Medicine and Haematology, University of Witwatersrand, ³Lightcurve Films

Anti-retroviral therapy to treat HIV/AIDS is monitored in South Africa on a large scale. Flow cytometry is combined for haematology (CD45), immunology (CD4) and viral-load linked CD38 assay. Recorded at NHLS-SA laboratories, Johannesburg, these modern methods are cost-efficient with heightened local internal quality control, serving as role-models for resource-limited diagnostics.

Isolation of Valvular Endothelial Cells

JoVE 2158 12/29/2010

Russell A. Gould, Jonathan T. Butcher

Department of Biomedical Engineering, Cornell University

We provide a method for isolating and culturing pure populations of heart valve endothelial cells (VEC). VEC can be isolated from either side of the cusp or leaflet and immediately following, underlying interstitial cell (VIC) isolation is straightforward.

Mouse Complete Stasis Model of Inferior Vena Cava Thrombosis

JoVE 2738 6/15/2011

Shirley K. Wrobleski, Diana M. Farris, José A. Diaz, Daniel D. Myers Jr., Thomas W. Wakefield

Conrad Jobst Vascular Research Laboratories, Section of Vascular Surgery, University of Michigan

The mouse complete stasis model of inferior vena cava thrombosis yields quantifiable amounts of vein wall tissue and thrombus. It has proven useful for evaluating interactions between the vein wall and the occlusive thrombus and in assessing the progression from acute to chronic inflammation.

Tractable Mammalian Cell Infections with Protozoan-primed Bacteria

JoVE 50300 4/02/2013

Samuel L. Drennan, Amrita Lama, Ben Doron, Eric D. Cambronne

Department of Molecular Microbiology & Immunology, Oregon Health & Science University

This technique provides a method to harvest, normalize and quantify intracellular growth of bacterial pathogens that are pre-cultivated in natural protozoan host cells prior to infections of mammalian cells. This method can be modified to accommodate a wide variety of host cells for the priming stage as well as target cell types.

Visualization of Vascular Ca²⁺ Signaling Triggered by Paracrine Derived ROS

JoVE 3511 12/21/2011

Karthik Mallilankaraman¹, Rajesh Kumar Gandhirajan¹, Brian J. Hawkins², Muniswamy Madesh¹

¹Department of Biochemistry, Temple University, ²Department of Anesthesiology and Pain Medicine, University of Washington

An efficient method to gain insights into visualizing the paracrine-derived ROS induction of endothelial Ca2+ signaling is described. This method takes advantage of measuring paracrine derived ROS triggered Ca2+ mobilization in vascular endothelial cells in a co-culture model.

Registered Bioimaging of Nanomaterials for Diagnostic and Therapeutic Monitoring

JoVE 2459 12/09/2010

Michael Boska¹, Yutong Liu¹, Mariano Uberti¹, Balarininvasa R. Sajja¹, Shantanu Balkundi², JoEllyn McMillan², Howard E. Gendelman²

¹Department of Radiology, University of Nebraska Medical Center, ²Department of Pharmacology and Experimental Neuroscience, University of Nebraska Medical Center

Bioimaging methods used to assess cell biodistribution of nanoparticles are applicable for therapeutic and diagnostic monitoring of nanoformulated compounds. The methods described herein are sensitive and specific when assessed by histological coregistration. The methodologies provide a translational pathway from rodent to human applications.

A Simple and Efficient Method to Detect Nuclear Factor Activation in Human Neutrophils by Flow Cytometry

JoVE 50410 4/09/2013

Erick García-García¹, Eileen Uribe-Querol², Carlos Rosales³

¹Department of Biological Sciences, University of Alberta, ²División de Estudios de Posgrado e Investigación, Facultad de Odontología, Universidad Nacional Autónoma de México, ³Department of Immunology, Instituto de Investigaciones Biomédicas, Universidad Nacional Autónoma de México

Neutrophils are the most abundant leukocytes in blood. Neutrophils possess transcriptionally regulated functions such as production of proinflammatory cytokines and inhibition of apoptosis. These functions can be studied with the method presented here, which allows detection and quantification of nuclear factors by flow cytometry in isolated nuclei

Generation of Bone Marrow Derived Murine Dendritic Cells for Use in 2-photon Imaging

JoVE 773 7/09/2008

Melanie P. Matheu¹, Debasish Sen¹, Michael D Cahalan¹, Ian Parker²

¹Department of Physiology and Biophysics, University of California, Irvine (UCI), ²Department of Neurobiology and Behaviour, University of California, Irvine (UCI)

Antigen presentation in secondary lymphoid organs by dendritic cells is crucial for the initiation of the T cell mediated adaptive immune response. Here we demonstrate the culture of bone marrow derived murine dendritic cells, activation, and labeling for 2-photon imaging.

Imaging Leukocyte Adhesion to the Vascular Endothelium at High Intraluminal Pressure

JoVE 3221 8/23/2011

Danielle L. Michell, Karen L. Andrews, Kevin J. Woollard, Jaye P.F. Chin-Dusting

Vascular Pharmacology Laboratory, Baker IDI Heart and Diabetes Institute, Monash University

This is a method to visualise leukocyte adhesion to the endothelium in harvested pressurised vessels. The technique enables studying vascular adhesion under shear flow with differing intraluminal pressures up to 200 mmHg thus mimic-ing the pathophysiological conditions of high blood pressure.

Vaccinia Virus Infection & Temporal Analysis of Virus Gene Expression: Part 3

JoVE 1170 4/13/2009

Judy Yen, Ron Golan, Kathleen Rubins

Whitehead Institute for Biomedical Research, MIT - Massachusetts Institute of Technology

Protocol for Vaccinia infection of HeLa cells and analysis of host and viral gene expression. Part 3 describes the process of fluorescently labeling the amplified RNA from both host and viral samples by amino allyl coupling of dyes. Part 3 of 3.

Vaccinia Virus Infection & Temporal Analysis of Virus Gene Expression: Part 2

JoVE 1169 4/10/2009

Judy Yen, Ron Golan, Kathleen Rubins

Whitehead Institute for Biomedical Research, MIT - Massachusetts Institute of Technology

Protocol for Vaccinia infection of HeLa cells and analysis of host and viral gene expression. Part 2 of 3.

Vaccinia Virus Infection & Temporal Analysis of Virus Gene Expression: Part 1

JoVE 1168 4/08/2009

Judy Yen, Ron Golan, Kathleen Rubins

Whitehead Institute for Biomedical Research, MIT - Massachusetts Institute of Technology

Protocol for Vaccinia infection of HeLa cells and analysis of host and viral gene expression. Part 1 of 3.

Embryonic Stem Cell-Derived Endothelial Cells for Treatment of Hindlimb Ischemia

JoVE 1034 1/23/2009

Ngan F. Huang¹, Hiroshi Niiyama¹, Abhijit De², Sanjiv S. Gambhir², John P. Cooke¹

¹Division of Cardiovascular Medicine, Stanford University, ²Department of Radiology, Stanford University

The surgical procedure for delivery of embryonic stem cell-derived endothelial cells to the ischemic hindlimb is demonstrated, with non-invasive tracking by bioluminescence imaging.

Live-cell Video Microscopy of Fungal Pathogen Phagocytosis

JoVE 50196 1/09/2013

Leanne E. Lewis¹, Judith M. Bain¹, Blessing Okai¹, Neil A.R. Gow², Lars Peter Erwig^1,2

¹Division of Applied Medicine, University of Aberdeen, ²Aberdeen Fungal Group, University of Aberdeen

We describe methods for live-cell video microscopy of Candida albicans phagocytosis by macrophages. These methods enable stage-specific analysis of macrophage migration, recognition, engulfment and phagosome maturation and reveal novel aspects of phagocytosis.

Intact Histological Characterization of Brain-implanted Microdevices and Surrounding Tissue

JoVE 50126 2/11/2013

Andrew J. Woolley¹, Himanshi A. Desai¹, Janak Gaire², Andrew L. Ready¹, Kevin J. Otto^1,2

¹Weldon School of Biomedical Engineering, Purdue University, ²Department of Biological Sciences, Purdue University

Here we present a histological method for capturing, labeling, optically clearing, and imaging the intact brain tissue interface around chronically implanted microdevices in rodent brain tissue. Results from the techniques comprising this method are useful for understanding the impact of various penetrating brain-implants on their surrounding tissue.

Generation and Labeling of Murine Bone Marrow-derived Dendritic Cells with Qdot Nanocrystals for Tracking Studies

JoVE 2785 6/02/2011

Maria Muccioli*¹, Michelle Pate*², Omowaleola Omosebi², Fabian Benencia^1,2,3

¹Molecular and Cell Biology Program, Ohio University, ²Department of Biomedical Sciences, College of Osteopathic Medicine, Ohio University, ³Department of Biomedical Engineering, Russ College of Engineering and Technology, Ohio University

Dendritic cells uptake antigens and migrate towards immune organs to present processed antigens to T cells. Qdot nanocrystal labeling provides a long-lasting and stable fluorescent signal. This allows tracking of dendritic cells to different organs by fluorescent microscopy.

Production and Detection of Reactive Oxygen Species (ROS) in Cancers

JoVE 3357 11/21/2011

Danli Wu, Patricia Yotnda

Center for Cell and Gene Therapy, Baylor College of Medicine

Here we propose simple methods to test and evaluate the presence of reactive oxygen species in cells.

Generation of Multivirus-specific T Cells to Prevent/treat Viral Infections after Allogeneic Hematopoietic Stem Cell Transplant

JoVE 2736 5/27/2011

Ulrike Gerdemann, Juan F. Vera, Cliona M. Rooney, Ann M. Leen

Center for Cell and Gene Therapy, Baylor College of Medicine

A rapid, simple and cost-effective protocol for the generation of donor-derived multivirus-specific CTLs (rCTL) for infusion to allogeneic hematopoietic stem cell transplant (HSCT) recipients at risk of developing CMV, Adv or EBV infections. This manufacturing process is GMP-compliant and should ensure the broader implementation of T-cell immunotherapy beyond specialized centers.

Phenotypic Analysis and Isolation of Murine Hematopoietic Stem Cells and Lineage-committed Progenitors

JoVE 3736 7/08/2012

Michela Frascoli¹, Michele Proietti¹, Fabio Grassi^1,2

¹Institute for Research in Biomedicine, Bellinzona (Switzerland), ²Dipartimento di Biologia e Genetica per le Scienze Mediche, Universitá degli Studi di Milano

A method to analyse the distribution of bone marrow hematopoietic progenitors in flow cytometry as well as to efficiently isolate highly purified hematopoietic stem cells (HSCs) is described. The isolation procedure is essentially based on magnetic enrichment of c-Kit+ cells and cell sorting to purify HSCs for cellular and molecular studies.

Chick ex ovo Culture and ex ovo CAM Assay: How it Really Works

JoVE 1620 11/30/2009

Daniel S. Dohle¹, Susanne D. Pasa¹, Sebastian Gustmann², Markus Laub³, Josef H. Wissler⁴, Herbert P. Jennissen¹, Nicole Dünker²

¹Institute for Physiological Chemistry, Department of Biochemical Endocrinology, University of Duisburg-Essen, ²Institute for Anatomy, Department of Neuroanatomy, University of Duisburg-Essen, ³Morphoplant GmbH, ⁴ARCONS Institute for Applied Research and Didactics

The chick chorioallantoic membrane (CAM) is a unique, naturally immunodeficient supportive culture environment to study angiogenesis and tumorigenesis. This video article demonstrates the different steps in chick ex ovo culture, application of potentially angiogenic substances and successful inoculation of tumor cells and tissues on the surface of the CAM.

Harvesting Murine Alveolar Macrophages and Evaluating Cellular Activation Induced by Polyanhydride Nanoparticles

JoVE 3883 6/08/2012

Ana V. Chavez-Santoscoy¹, Lucas M. Huntimer², Amanda E. Ramer-Tait², Michael Wannemuehler², Balaji Narasimhan¹

¹Department of Chemical and Biological Engineering, Iowa State University, ²Department of Veterinary Microbiology and Preventive Medicine, Iowa State University

Herein, we describe protocols for harvesting murine alveolar macrophages, which are resident innate immune cells in the lung, and examining their activation in response to co-culture with polyanhydride nanoparticles.

A Parasite Rescue and Transformation Assay for Antileishmanial Screening Against Intracellular Leishmania donovani Amastigotes in THP1 Human Acute Monocytic Leukemia Cell Line

JoVE 4054 12/30/2012

Surendra K. Jain¹, Rajnish Sahu¹, Larry A. Walker^1,2, Babu L. Tekwani^1,2

¹National Center for Natural Products Research, School of Pharmacy, University of Mississippi, ²Department of Pharmacology, University of Mississippi

A parasite-rescue and transformation assay with THP1 cells infected in vitro with Leishmania donovani has been optimized for anti-leishmanial drug screening. The assay involves differentiation of THP1 cells, infection with promastigotes, treatment with test drugs, controlled lysis of the infected macrophages, rescue of amastigotes, transformation to promastigotes and monitoring promastigote growth and proliferation with a fluorometric assay.

Parasite Induced Genetically Driven Autoimmune Chagas Heart Disease in the Chicken Model

JoVE 3716 7/29/2012

Antonio R. L. Teixeira, Nadjar Nitz, Francisco M. Bernal, Mariana M. Hecht

Chagas Disease Multidisciplinary Research Laboratory, University of Brasilia

The inoculation of Trypanosoma cruzi in fertile eggs prior to incubation renders the parasite kDNA minicircle integration in embryo cells genome. Crossbreeding reveals the vertical transfer of the mutations to progeny. The kDNA integrates into coding regions at several chromosomes and the chickens die with an inflammatory autoimmune heart disease.

Propagating and Detecting an Infectious Molecular Clone of Maedi-visna Virus that Expresses Green Fluorescent Protein

JoVE 3483 10/09/2011

Stefán R. Jónsson, Valgerdur Andrésdóttir

Institute for Experimental Pathology, University of Iceland

We describe a molecular clone of maedi-visna virus that expresses GFP and is fully infectious. Replication of this virus can be detected by using fluorescence microscopy and flow cytometry.

Artificial Antigen Presenting Cell (aAPC) Mediated Activation and Expansion of Natural Killer T Cells

JoVE 4333 12/29/2012

James E. East*, Wenji Sun*, Tonya J. Webb

Department of Microbiology and Immunology, University of Maryland

Here we describe a method for activating and expanding human NKT cells from bulk T cell populations using artificial antigen presenting cells (aAPC). The use of CD1d-based aAPC provides a standardized method for generating high numbers of functional NKT cells.

High-throughput Synthesis of Carbohydrates and Functionalization of Polyanhydride Nanoparticles

JoVE 3967 7/06/2012

Brenda R. Carrillo-Conde*¹, Rajarshi Roychoudhury*², Ana V. Chavez-Santoscoy*¹, Balaji Narasimhan¹, Nicola L.B. Pohl^1,2

¹Department of Chemical and Biological Engineering, Iowa State University, ²Department of Chemistry, Iowa State University

In this article, a high throughput method is presented for the synthesis of oligosaccharides and their attachment to the surface of polyanhydride nanoparticles for further use in targeting specific receptors on antigen presenting cells.

Flow Cytometric Isolation of Primary Murine Type II Alveolar Epithelial Cells for Functional and Molecular Studies

JoVE 4322 12/26/2012

Marcus Gereke^1,2, Andrea Autengruber^1,2, Lothar Gröbe³, Andreas Jeron², Dunja Bruder^1,2, Sabine Stegemann-Koniszewski¹

¹Research Group Immune Regulation, Helmholtz Centre for Infection Research, ²Research Group Infection Immunology, Institute of Medical Microbiology, Otto-von-Guericke University, ³Department of Experimental Immunology, Helmholtz Centre for Infection Research

We describe the rapid isolation of primary murine type II alveolar epithelial cells (AECII) by flow cytometric negative selection. These AECII show high viability and purity and are suitable for a wide range of functional and molecular studies regarding their role in respiratory conditions such as autoimmune or infectious diseases.

Establishing a Liquid-covered Culture of Polarized Human Airway Epithelial Calu-3 Cells to Study Host Cell Response to Respiratory Pathogens In vitro

JoVE 50157 2/07/2013

Jennifer L. Harcourt, Lia M. Haynes

National Center for Immunization and Respiratory Diseases, Division of Viral Diseases, Gastroenteritis and Respiratory Viruses Laboratory Branch, Centers for Disease Control and Prevention (CDC)

The findings and conclusions in this report are those of the authors and do not necessarily represent the views of the Centers for Disease Control and Prevention.

Parallel-plate Flow Chamber and Continuous Flow Circuit to Evaluate Endothelial Progenitor Cells under Laminar Flow Shear Stress

JoVE 3349 1/17/2012

Whitney O. Lane¹, Alexandra E. Jantzen², Tim A. Carlon², Ryan M. Jamiolkowski³, Justin E. Grenet¹, Melissa M. Ley¹, Justin M. Haseltine², Lauren J. Galinat², Fu-Hsiung Lin¹, Jason D. Allen⁴, George A. Truskey², Hardean E. Achneck¹

¹Department of Surgery, Duke University Medical Center, ²Department of Biomedical Engineering, Duke University, ³School of Medicine, University of Pennsylvania, ⁴Department of Medicine, Division of Cardiology, Duke University Medical Center

We are describing a method to subject adherent cells to laminar flow shear stress in a sterile continuous flow circuit. The cells' adhesion, morphology can be studied through the transparent chamber, samples obtained from the circuit for metabolite analysis and cells harvested after shear exposure for future experiments or culture.

Optimized Staining and Proliferation Modeling Methods for Cell Division Monitoring using Cell Tracking Dyes

JoVE 4287 12/13/2012

Joseph D. Tario Jr.¹, Kristen Humphrey¹, Andrew D. Bantly², Katharine A. Muirhead³, Jonni S. Moore⁴, Paul K. Wallace¹

¹Department of Flow and Image Cytometry, Roswell Park Cancer Institute, ²Flow Cytometry & Cell Sorting Resource Laboratory, University of Pennsylvania, ³SciGro, Inc., ⁴Department of Pathology and Laboratory Medicine, University of Pennsylvania

Successful use of cell tracking dyes to monitor immune cell function and proliferation involves several critical steps. We describe methods for: 1) obtaining bright, uniform, reproducible label-ing with membrane dyes; 2) selecting fluorochromes and data acquisition conditions; and 3) choosing a model to quantify cell proliferation based on dye dilution.