Your search keyword '"Immunology and Infection"' showing total 72 results

1. TurboID-Based Proximity Labeling for In Planta Identification of Protein-Protein Interaction Networks.

Author

Zhang, Yongliang, Li, Yuanyuan, Yang, Xinxin, Wen, Zhiyan, Nagalakshmi, Ugrappa, and Dinesh-Kumar, Savithramma P

Subjects

Biochemistry and Cell Biology, Biological Sciences, Animals, Plants, Protein Interaction Maps, Proteomics, Immunology and Infection, Issue 159, proximity labeling, TurboID, protein interactions, desalting, quantification, purification, TIR, Psychology, Cognitive Sciences, Biochemistry and cell biology

Abstract

Proximity labeling (PL) techniques using engineered ascorbate peroxidase (APEX) or Escherichia coli biotin ligase BirA (known as BioID) have been successfully used for identification of protein-protein interactions (PPIs) in mammalian cells. However, requirements of toxic hydrogen peroxide (H2O2) in APEX-based PL, longer incubation time with biotin (16-24 h), and higher incubation temperature (37 °C) in BioID-based PL severely limit their applications in plants. The recently described TurboID-based PL addresses many limitations of BioID and APEX. TurboID allows rapid proximity labeling of proteins in just 10 min under room temperature (RT) conditions. Although the utility of TurboID has been demonstrated in animal models, we recently showed that TurboID-based PL performs better in plants compared to BioID for labeling of proteins that are proximal to a protein of interest. Provided here is a step-by-step protocol for the identification of protein interaction partners using the N-terminal Toll/interleukin-1 receptor (TIR) domain of the nucleotide-binding leucine-rich repeat (NLR) protein family as a model. The method describes vector construction, agroinfiltration of protein expression constructs, biotin treatment, protein extraction and desalting, quantification, and enrichment of the biotinylated proteins by affinity purification. The protocol described here can be easily adapted to study other proteins of interest in Nicotiana and other plant species.

Published

2020

2. Rapid, Seamless Generation of Recombinant Poxviruses using Host Range and Visual Selection.

Author

Vipat, Sameera, Brennan, Greg, Park, Chorong, Haller, Sherry L, and Rothenburg, Stefan

Subjects

Biochemistry and Cell Biology, Biological Sciences, Biodefense, Rare Diseases, Prevention, Vaccine Related, Immunization, Infectious Diseases, Genetics, Biotechnology, Small Pox, Infection, Animals, Cells, Cultured, Genetic Vectors, Green Fluorescent Proteins, Host Specificity, Humans, Kidney, Poxviridae, Poxviridae Infections, Rabbits, Vaccinia virus, eIF-2 Kinase, Immunology and Infection, Issue 159, Recombination, Poxvirus, Host range, Protein kinase R, E3L-mCherry, Psychology, Cognitive Sciences, Biochemistry and cell biology

Abstract

Vaccinia virus (VACV) was instrumental in eradicating variola virus (VARV), the causative agent of smallpox, from nature. Since its first use as a vaccine, VACV has been developed as a vector for therapeutic vaccines and as an oncolytic virus. These applications take advantage of VACV's easily manipulated genome and broad host range as an outstanding platform to generate recombinant viruses with a variety of therapeutic applications. Several methods have been developed to generate recombinant VACV, including marker selection methods and transient dominant selection. Here, we present a refinement of a host range selection method coupled with visual identification of recombinant viruses. Our method takes advantage of selective pressure generated by the host antiviral protein kinase R (PKR) coupled with a fluorescent fusion gene expressing mCherry-tagged E3L, one of two VACV PKR antagonists. The cassette, including the gene of interest and the mCherry-E3L fusion is flanked by sequences derived from the VACV genome. Between the gene of interest and mCherry-E3L is a smaller region that is identical to the first ~150 nucleotides of the 3' arm, to promote homologous recombination and loss of the mCherry-E3L gene after selection. We demonstrate that this method permits efficient, seamless generation of rVACV in a variety of cell types without requiring drug selection or extensive screening for mutant viruses.

Published

2020

3. A Mouse Model to Assess Innate Immune Response to Staphylococcus aureus Infection.

Author

Anderson, Leif S, Reynolds, Mack B, Rivara, Kathryn R, Miller, Lloyd S, and Simon, Scott I

Subjects

Microbiology, Biological Sciences, Infectious Diseases, Emerging Infectious Diseases, Vaccine Related, Prevention, Biodefense, 2.2 Factors relating to the physical environment, Aetiology, 2.1 Biological and endogenous factors, Infection, Good Health and Well Being, Animals, Disease Models, Animal, Humans, Immunity, Innate, Mice, Staphylococcal Infections, Staphylococcus aureus, Immunology and Infection, Issue 144, innate immunity, neutrophils, wound healing, inflammation, whole-animal imaging, Biochemistry and Cell Biology, Psychology, Cognitive Sciences, Biochemistry and cell biology

Abstract

Staphylococcus aureus (S. aureus) infections, including methicillin resistant stains, are an enormous burden on the healthcare system. With incidence rates of S. aureus infection climbing annually, there is a demand for additional research in its pathogenicity. Animal models of infectious disease advance our understanding of the host-pathogen response and lead to the development of effective therapeutics. Neutrophils play a primary role in the innate immune response that controls S. aureus infections by forming an abscess to wall off the infection and facilitate bacterial clearance; the number of neutrophils that infiltrate an S. aureus skin infection often correlates with disease outcome. LysM-EGFP mice, which possess the enhanced green fluorescent protein (EGFP) inserted in the Lysozyme M (LysM) promoter region (expressed primarily by neutrophils), when used in conjunction with in vivo whole animal fluorescence imaging (FLI) provide a means of quantifying neutrophil emigration noninvasively and longitudinally into wounded skin. When combined with a bioluminescent S. aureus strain and sequential in vivo whole animal bioluminescent imaging (BLI), it is possible to longitudinally monitor both the neutrophil recruitment dynamics and in vivo bacterial burden at the site of infection in anesthetized mice from onset of infection to resolution or death. Mice are more resistant to a number of virulence factors produced by S. aureus that facilitate effective colonization and infection in humans. Immunodeficient mice provide a more sensitive animal model to examine persistent S. aureus infections and the ability of therapeutics to boost innate immune responses. Herein, we characterize responses in LysM-EGFP mice that have been bred to MyD88-deficient mice (LysM-EGFP×MyD88-/- mice) along with wild-type LysM-EGFP mice to investigate S. aureus skin wound infection. Multispectral simultaneous detection enabled study of neutrophil recruitment dynamics by using in vivo FLI, bacterial burden by using in vivo BLI, and wound healing longitudinally and noninvasively over time.

Published

2019

4. Isolation and Quantification of Zika Virus from Multiple Organs in a Mouse.

Author

Brien, James D, Hassert, Mariah, Stone, E Taylor, Geerling, Elizabeth, Cruz-Orengo, Lillian, and Pinto, Amelia K

Subjects

Biochemistry and Cell Biology, Biological Sciences, Emerging Infectious Diseases, Biotechnology, Infectious Diseases, Aetiology, 2.2 Factors relating to the physical environment, Infection, Good Health and Well Being, Animals, Genome, Viral, Limit of Detection, Mice, RNA, Viral, Real-Time Polymerase Chain Reaction, Viral Load, Viral Plaque Assay, Zika Virus, Zika Virus Infection, Immunology and Infection, Issue 150, Zika virus, brain, spinal cord, kidney, spleen, liver, viral titer, focus forming assay, quantitative real-time PCR, foot pad infection, Psychology, Cognitive Sciences, Biochemistry and cell biology

Abstract

The methods being presented demonstrate laboratory procedures for the isolation of organs from Zika virus infected animals and the quantification of viral load. The purpose of the procedure is to quantify viral titers in peripheral and CNS areas of the mouse at different time points post infection or under different experimental conditions to identify virologic and immunological factors that regulate Zika virus infection. The organ isolation procedures demonstrated allow for both focus forming assay quantification and quantitative PCR assessment of viral titers. The rapid organ isolation techniques are designed for the preservation of virus titer. Viral titer quantification by focus forming assay allows for the rapid throughput assessment of Zika virus. The benefit of the focus forming assay is the assessment of infectious virus, the limitation of this assay is the potential for organ toxicity reducing the limit of detection. Viral titer assessment is combined with quantitative PCR, and using a recombinant RNA copy control viral genome copy number within the organ is assessed with low limit of detection. Overall these techniques provide an accurate rapid high throughput method for the analysis of Zika viral titers in the periphery and CNS of Zika virus infected animals and can be applied to the assessment of viral titers in the organs of animals infected with most pathogens, including Dengue virus.

Published

2019

5. In Vitro Canine Neutrophil Extracellular Trap Formation: Dynamic and Quantitative Analysis by Fluorescence Microscopy.

Author

Li, Ronald HL and Tablin, Fern

Subjects

Neutrophils, Animals, Dogs, Humans, Microscopy, Fluorescence, Extracellular Traps, Hematology, Infection, Inflammatory and immune system, Immunology and Infection, Issue 138, Immunofluorescence microscopy, sepsis, granulocyte isolation, histone, citrullination, peptidylarginine deiminase, Biochemistry and Cell Biology, Psychology, Cognitive Sciences

Abstract

In response to invading pathogens, neutrophils release neutrophil extracellular traps (NETs), which are extracellular networks of DNA decorated with histones and antimicrobial proteins. Excessive NET formation (NETosis) and citH3 release during sepsis is associated with multiple organ dysfunction and mortality in mice and humans but its implications in dogs are unknown. Herein, we describe a technique to isolate canine neutrophils from whole blood for observation and quantification of NETosis. Leukocyte-rich plasma, generated by dextran sedimentation, is separated by commercially available density gradient separation media and granulocytes collected for cell count and viability testing. To observe real-time NETosis in live neutrophils, cell permeant and cell impermeant fluorescent nucleic acid stains are added to neutrophils activated either by lipopolysaccharide (LPS) or phorbol 12-myristate 13-acetate (PMA). Changes in nuclear morphology and NET formation are observed over time by fluorescence microscopy. In vitro NETosis is further characterized by co-colocalization of cell-free DNA (cfDNA), myeloperoxidase (MPO) and citrullinated histone H3 (citH3) using a modified double-immunolabelling protocol. To objectively quantify NET formation and citH3 expression using fluorescence microscopy, NETs and citH3-positive cells are quantified in a blinded manner using available software. This technique is a specific assay to evaluate the in vitro capacity of canine neutrophils to undergo NETosis.

Published

2018

6. The Lambda Select cII Mutation Detection System.

Author

Besaratinia, Ahmad and Tommasi, Stella

Subjects

Microbiology, Biological Sciences, Genetics, Biotechnology, Animals, Bacteriophage lambda, Mice, Mice, Transgenic, Mutagenicity Tests, Mutation, Rats, Rats, Transgenic, Transcription Factors, Viral Proteins, Immunology and Infection, Issue 134, Bacteriophage, cII Transgene, Embryonic Mouse Fibroblasts, EMF, Shuttle Vector, Biochemistry and Cell Biology, Psychology, Cognitive Sciences, Biochemistry and cell biology

Abstract

A number of transgenic animal models and mutation detection systems have been developed for mutagenicity testing of carcinogens in mammalian cells. Of these, transgenic mice and the Lambda (λ) Select cII Mutation Detection System have been employed for mutagenicity experiments by many research groups worldwide. Here, we describe a detailed protocol for the Lambda Select cII mutation assay, which can be applied to cultured cells of transgenic mice/rats or the corresponding animals treated with a chemical/physical agent of interest. The protocol consists of the following steps: (1) isolation of genomic DNA from the cells or organs/tissues of transgenic animals treated in vitro or in vivo, respectively, with a test compound; (2) recovery of the lambda shuttle vector carrying a mutational reporter gene (i.e., cII transgene) from the genomic DNA; (3) packaging of the rescued vectors into infectious bacteriophages; (4) infecting a host bacteria and culturing under selective conditions to allow propagation of the induced cII mutations; and (5) scoring the cII-mutants and DNA sequence analysis to determine the cII mutant frequency and mutation spectrum, respectively.

Published

2018

7. Rapid, Seamless Generation of Recombinant Poxviruses using Host Range and Visual Selection

Author

Sherry L. Haller, Stefan Rothenburg, Greg Brennan, Chorong Park, and Sameera Vipat

Subjects

0301 basic medicine, General Chemical Engineering, viruses, Poxviridae Infections, Kidney, Genome, law.invention, chemistry.chemical_compound, eIF-2 Kinase, 0302 clinical medicine, law, Psychology, Cells, Cultured, Immunology and Infection, Cultured, General Neuroscience, virus diseases, Infectious Diseases, Poxvirus, Recombinant DNA, Cognitive Sciences, Rabbits, Infection, Biotechnology, Protein kinase R, Cells, Genetic Vectors, Green Fluorescent Proteins, Antiviral protein, E3L-mCherry, Vaccinia virus, Computational biology, Biology, General Biochemistry, Genetics and Molecular Biology, Virus, Host Specificity, Article, Vaccine Related, 03 medical and health sciences, Rare Diseases, Biodefense, Issue 159, 030225 pediatrics, Genetics, Animals, Humans, Small Pox, Gene, General Immunology and Microbiology, Prevention, Poxviridae, Recombination, Oncolytic virus, 030104 developmental biology, chemistry, Host range, Immunization, Biochemistry and Cell Biology, Vaccinia, Homologous recombination

Abstract

Vaccinia virus (VACV) was instrumental in eradicating variola virus (VARV), the causative agent of smallpox, from nature. Since its first use as a vaccine, VACV has been developed as a vector for therapeutic vaccines and as an oncolytic virus. These applications take advantage of VACV's easily manipulated genome and broad host range as an outstanding platform to generate recombinant viruses with a variety of therapeutic applications. Several methods have been developed to generate recombinant VACV, including marker selection methods and transient dominant selection. Here, we present a refinement of a host range selection method coupled with visual identification of recombinant viruses. Our method takes advantage of selective pressure generated by the host antiviral protein kinase R (PKR) coupled with a fluorescent fusion gene expressing mCherry-tagged E3L, one of two VACV PKR antagonists. The cassette, including the gene of interest and the mCherry-E3L fusion is flanked by sequences derived from the VACV genome. Between the gene of interest and mCherry-E3L is a smaller region that is identical to the first ~150 nucleotides of the 3' arm, to promote homologous recombination and loss of the mCherry-E3L gene after selection. We demonstrate that this method permits efficient, seamless generation of rVACV in a variety of cell types without requiring drug selection or extensive screening for mutant viruses.

Published

2020

8. TurboID-Based Proximity Labeling for In Planta Identification of Protein-Protein Interaction Networks

Author

Ugrappa Nagalakshmi, Savithramma P. Dinesh-Kumar, Yuan-Yuan Li, Zhiyan Wen, Xinxin Yang, and Yongliang Zhang

Subjects

0106 biological sciences, Proteomics, Agroinfiltration, Protein family, purification, General Chemical Engineering, TurboID, 01 natural sciences, protein interactions, Article, General Biochemistry, Genetics and Molecular Biology, Protein–protein interaction, 03 medical and health sciences, chemistry.chemical_compound, Biotin, Affinity chromatography, Issue 159, Protein purification, Animals, Psychology, Protein Interaction Maps, 030304 developmental biology, Immunology and Infection, chemistry.chemical_classification, 0303 health sciences, DNA ligase, desalting, General Immunology and Microbiology, General Neuroscience, Plants, quantification, TIR, chemistry, Biochemistry, Biotinylation, Cognitive Sciences, Biochemistry and Cell Biology, 010606 plant biology & botany, proximity labeling

Abstract

Proximity labeling (PL) techniques using engineered ascorbate peroxidase (APEX) or Escherichia coli biotin ligase BirA (known as BioID) have been successfully used for identification of protein-protein interactions (PPIs) in mammalian cells. However, requirements of toxic hydrogen peroxide (H(2)O(2)) in APEX-based PL, longer incubation time with biotin (16–24 h), and higher incubation temperature (37 °C) in BioID-based PL severely limit their applications in plants. The recently described TurboID-based PL addresses many limitations of BioID and APEX. TurboID allows rapid proximity labeling of proteins in just 10 min under room temperature (RT) conditions. Although the utility of TurboID has been demonstrated in animal models, we recently showed that TurboID-based PL performs better in plants compared to BioID for labeling of proteins that are proximal to a protein of interest. Provided here is a step-by-step protocol for the identification of protein interaction partners using the N-terminal Toll/interleukin-1 receptor (TIR) domain of the nucleotide-binding leucine-rich repeat (NLR) protein family as a model. The method describes vector construction, agroinfiltration of protein expression constructs, biotin treatment, protein extraction and desalting, quantification, and enrichment of the biotinylated proteins by affinity purification. The protocol described here can be easily adapted to study other proteins of interest in Nicotiana and other plant species.

Published

2020

9. Visualization and Quantification of High-Dimensional Cytometry Data using Cytofast and the Upstream Clustering Methods FlowSOM and Cytosplore

Author

Ferry Ossendorp, Guillaume Beyrend, Ramon Arens, and Koen A. Stam

Subjects

0301 basic medicine, Computer science, medicine.medical_treatment, General Chemical Engineering, high-dimensional analysis, Cell, 02 engineering and technology, Computational biology, Lymphocyte Activation, visualization tool, B7-H1 Antigen, General Biochemistry, Genetics and Molecular Biology, Issue 154, Mice, 03 medical and health sciences, Single-cell analysis, Tumor Microenvironment, medicine, Animals, Cluster Analysis, single-cell analysis, Mass cytometry, Cluster analysis, Immunology and Infection, Tumor microenvironment, General Immunology and Microbiology, General Neuroscience, R package, Immunotherapy, data mining, flow and mass cytometry analysis, Flow Cytometry, 021001 nanoscience & nanotechnology, Visualization, Killer Cells, Natural, Mice, Inbred C57BL, 030104 developmental biology, medicine.anatomical_structure, 0210 nano-technology, Cytometry

Abstract

The complexity of data generated by mass cytometry has necessitated new tools to rapidly visualize analytic outcomes. Clustering methods like Cytosplore or FlowSOM are used for the visualization and identification of cell clusters. For downstream analysis, a newly developed R package, Cytofast, can generate a rapid visualization of results from clustering methods. Cytofast takes into account the phenotypic characterization of cell clusters, calculates the cell cluster abundance, then quantitatively compares groups. This protocol explains the applications of Cytofast to the use of mass cytometry data based on modulation of the immune system in the tumor microenvironment (i.e., the natural killer [NK] cell response) upon tumor challenge followed by immunotherapy (PD-L1 blockade). Demonstration of the usefulness of Cytofast with FlowSOM and Cytosplore is shown. Cytofast rapidly generates visual representations of group-related immune cell clusters and correlations with immune system composition. Differences are observed in the clustering analysis, but separation between groups are visible with both clustering methods. Cytofast visually shows the patterns induced by PD-L1 treatment that include a higher abundance of activated NK cell subsets, expressing a higher intensity of activation markers (i.e., CD54 or CD11c).

Published

2019

10. Inducing Meningococcal Meningitis Serogroup C in Mice via Intracisternal Delivery

Author

Elena Scaglione, Roberta Colicchio, Caterina Pagliarulo, Maria Michela Marino, Maria Virginia Pishbin, Chiara Pagliuca, Giuseppe Mantova, Paola Salvatore, Francesca Carraturo, Pagliuca, Chiara, Scaglione, Elena, Carraturo, Francesca, Mantova, Giuseppe, Marino, Maria Michela, Pishbin, Maria Virginia, Pagliarulo, Caterina, Colicchio, Roberta, and Salvatore, Paola

Subjects

Fulminant, General Chemical Engineering, Meningococcal meningiti, Spleen, Meningitis, Meningococcal, Neisseria meningitidis, Blood–brain barrier, medicine.disease_cause, Meningococcal disease, General Biochemistry, Genetics and Molecular Biology, Microbiology, Mouse model, Sepsis, Mice, medicine, Neisseria meningitidi, Animals, Humans, Immunology and Infection, Intra-cisternal injection, General Immunology and Microbiology, business.industry, General Neuroscience, Vaccination, Brain, medicine.disease, Brain tissue, Issue 153, Disease Models, Animal, medicine.anatomical_structure, Blood-Brain Barrier, Host-Pathogen Interactions, business, Infection, Meningitis, Isogenic mutant strain

Abstract

Neisseria meningitidis (meningococcus) is a narrow-host-range microorganism, globally recognized as the leading cause of bacterial meningitis. Meningococcus is a transient colonizer of human nasopharynx of approximately 10% of healthy subject. In particular circumstances, it acquires an invasive ability to penetrate the mucosal barrier and invades the bloodstream causing septicaemia. In the latest case, fulminating sepsis could arise even without the consequent development of meningitis. Conversely, bacteria could poorly multiply in the bloodstream, cross the blood brain barrier, reach the central nervous system, leading to fulminant meningitis. The murine models of bacterial meningitis represent a useful tool to investigate the host-pathogen interactions and to analyze the pathogenetic mechanisms responsible for this lethal disease. Although, several experimental model systems have been evaluated over the last decades, none of these were able to reproduce the characteristic pathological events of meningococcal disease. In this experimental protocol, we describe a detailed procedure for the induction of meningococcal meningitis in a mouse model based on the intracisternal inoculation of bacteria. The peculiar signs of human meningitis were recorded in the murine host through the assessment of clinical parameters (e.g., temperature, body weight), evaluation of survival rate, microbiological analysis and histological examination of brain injury. When using intracisternal (i.cist.) inoculum, meningococci complete delivery directly into cisterna magna, leading to a very efficient meningococcal replication in the brain tissue. A 1,000-fold increase of viable count of bacteria is observed in about 18 h. Moreover, meningococci are also found in the spleen, and liver of infected mice, suggesting that the liver may represent a target organ for meningococcal replication.

Published

2019

11. Isolation and Quantification of Zika Virus from Multiple Organs in a Mouse

Author

Lillian Cruz-Orengo, Amelia K. Pinto, Elizabeth Geerling, E. Taylor Stone, Mariah Hassert, and James D. Brien

Subjects

0301 basic medicine, viruses, General Chemical Engineering, Viral Plaque Assay, Dengue virus, medicine.disease_cause, Zika virus, law.invention, Mice, 0302 clinical medicine, Limit of Detection, law, viral titer, 2.2 Factors relating to the physical environment, Psychology, Viral, 030212 general & internal medicine, Aetiology, focus forming assay, Immunology and Infection, Genome, Zika Virus Infection, General Neuroscience, Viral Load, Titer, Infectious Diseases, Real-time polymerase chain reaction, medicine.anatomical_structure, Recombinant DNA, RNA, Viral, Cognitive Sciences, Infection, Viral load, Biotechnology, kidney, foot pad infection, brain, Spleen, Genome, Viral, Biology, Real-Time Polymerase Chain Reaction, liver, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, medicine, Animals, quantitative real-time PCR, General Immunology and Microbiology, spinal cord, Zika Virus, Issue 150, biology.organism_classification, Virology, Emerging Infectious Diseases, Good Health and Well Being, 030104 developmental biology, RNA, spleen, Biochemistry and Cell Biology

Abstract

The methods being presented demonstrate laboratory procedures for the isolation of organs from Zika virus infected animals and the quantification of viral load. The purpose of the procedure is to quantify viral titers in peripheral and CNS areas of the mouse at different time points post infection or under different experimental conditions to identify virologic and immunological factors that regulate Zika virus infection. The organ isolation procedures demonstrated allow for both focus forming assay quantification and quantitative PCR assessment of viral titers. The rapid organ isolation techniques are designed for the preservation of virus titer. Viral titer quantification by focus forming assay allows for the rapid throughput assessment of Zika virus. The benefit of the focus forming assay is the assessment of infectious virus, the limitation of this assay is the potential for organ toxicity reducing the limit of detection. Viral titer assessment is combined with quantitative PCR, and using a recombinant RNA copy control viral genome copy number within the organ is assessed with low limit of detection. Overall these techniques provide an accurate rapid high throughput method for the analysis of Zika viral titers in the periphery and CNS of Zika virus infected animals and can be applied to the assessment of viral titers in the organs of animals infected with most pathogens, including Dengue virus.

Published

2019

12. Immunological homeostasis at the ovine placenta may reflect the degree of maternal fetal interaction

Author

Sean R. Wattegedera, Laura E. Doull, Mariya I. Goncheva, Nicholas M. Wheelhouse, Donna M. Watson, Julian Pearce, Julio Benavides, Javier Palarea-Albaladejo, Colin J. McInnes, Keith Ballingall, Gary Entrican, Scottish Government's Rural and Environment Science and Analytical Services, European Commission, and Bio-Rad Laboratories

Subjects

0301 basic medicine, Biomedical Science Research Group, Placenta, Cell, Major histocompatibility complex, Gene Expression, 0302 clinical medicine, Pregnancy, Immunology and Allergy, Homeostasis, QR180 Immunology, Indoleamine 2,3 dioxygenase-1, Maternal-Fetal Exchange, Phylogeny, Original Research, MHC Class I Protein, biology, Trophoblast, Immunology and infection, 3. Good health, Cell biology, Trophoblasts, medicine.anatomical_structure, Health, Reproductive health, Female, lcsh:Immunologic diseases. Allergy, Ovine, Major Histocompatibility Complex, Indoleamine 2, 3 dioxygenase-1, synepitheliochorial placentation, trophoblast, Immunology, synepitheliochorial, rophoblast, Cell Line, Immunophenotyping, Applied microbiology, 03 medical and health sciences, 616 Diseases, MHC class I, medicine, Animals, Microbiology Research Group, Sheep, Synepitheliochorial placentation, Natural Cytotoxicity Triggering Receptor 1, Placentation, Sequence Analysis, DNA, Ovine, 030104 developmental biology, Cell culture, biology.protein, lcsh:RC581-607, Biomarkers, 030215 immunology

Abstract

10 páginas, 4 figuras., Successful mammalian pregnancies are a result of complex physiological, endocrinological, and immunological processes that combine to create an environment where the mother is tolerant to the semi-allogeneic fetus. Our knowledge of the mechanisms that contribute to maternal tolerance is derived mainly from human and murine studies of haemochorial placentation. However, as this is the most invasive type of placentation it cannot be assumed that identical mechanisms apply to the less invasive epitheliochorial placentation found in other species such as ruminants. Here, we examine three features associated with reproductive immune regulation in a transformed ovine trophoblast cell line and ex-vivo ovine reproductive tissues collected at term, namely: major histocompatibility complex (MHC) expression, Indoleamine 2,3 dioxygenase-1 (IDO-1) expression, and Natural Killer (NK) cell infiltration. High levels of MHC class I protein expression were detected at the surface of the trophoblast cell line using a pan-MHC class I specific monoclonal antibody. The majority of MHC class I transcripts isolated from the cell line clustered with classical MHC alleles. Transcriptional analysis of placental tissues identified only classical MHC class I transcripts. We found no evidence of constitutive transcription of IDO-1 in either the trophoblast cell line or placental tissues. Ex-vivo tissues collected from the materno-fetal interface were negative for cells expressing NKp46/NCR1. Collectively, these observations suggest that the relatively non-invasive synepitheliochorial placentation found in sheep has a more limited requirement for local immunoregulation compared to the more invasive haemochorial placentation of primates and rodents., SW, NW, CM, KB, JP-A, and GE were funded by the Scottish Government Rural and Environment Science and Analytical Services (RESAS) Strategic Research Programme (SRP). SW, CM, and GE also received funding from The route to identification of immunological correlates of protection in ruminants Industrial Partnership Award with Bio-Rad Laboratories (grant numbers BB/I019863/1; BB/I020519/1). KB and GE also receive funding the European Union’s Horizon 2020 research and innovation programme under grant agreement N◦731014 (VetBioNet).

Published

2019

13. Rescue of recombinant zika virus from a bacterial artificial chromosome cdna clone

Author

Fernando Almazán, Jun-Gyu Park, Aitor Nogales, Ginés Ávila-Pérez, Luis Martinez-Sobrido, Ministerio de Economía y Competitividad (España), and National Institutes of Health (US)

Subjects

0301 basic medicine, Chromosomes, Artificial, Bacterial, DNA, Complementary, General Chemical Engineering, 030106 microbiology, Genome, Viral, Genome, General Biochemistry, Genetics and Molecular Biology, Zika virus, 03 medical and health sciences, cDNA transfection, Plasmid, Complementary DNA, Chlorocebus aethiops, Animals, Humans, Vero Cells, Immunology and Infection, Recombination, Genetic, Arbovirus, Bacterial artificial chromosome, General Immunology and Microbiology, biology, Zika Virus Infection, General Neuroscience, Flavivirus, Virion, biology.organism_classification, Bacterial artificial chromosomes, Virology, Reverse genetics, Full-length cDNA infectious clones, Clone Cells, 030104 developmental biology, Issue 148, Vero cell, Virus rescue

Abstract

© 2019 Journal of Visualized Experiments., The association of Zika virus (ZIKV) infection with neurological complications during the recent worldwide outbreak and the lack of approved vaccines and/or antivirals have underscored the urgent need to develop ZIKV reverse genetic systems to facilitate the study of ZIKV biology and the development of therapeutic and/or prophylactic approaches. However, like with other flaviviruses, the generation of ZIKV full-length infectious cDNA clones has been hampered due to the toxicity of viral sequences during its amplification in bacteria. To overcome this problem, we have developed a nontraditional approach based on the use of bacterial artificial chromosomes (BACs). Using this approach, the full-length cDNA copy of the ZIKV strain Rio Grande do Norte Natal (ZIKV-RGN) is generated from four synthetic DNA fragments and assembled into the single-copy pBeloBAC11 plasmid under the control of the human cytomegalovirus (CMV) immediate-early promoter. The assembled BAC cDNA clone is stable during propagation in bacteria, and infectious recombinant (r)ZIKV is recovered in Vero cells after transfection of the BAC cDNA clone. The protocol described here provides a powerful technique for the generation of infectious clones of flaviviruses, including ZIKV, and other positive-strand RNA viruses, particularly those with large genomes that have stability problems during bacterial propagation., This work was supported in part by grants from the Spanish Ministry of Economy and Competitiveness (MINECO, grant number BFU2016-79127-R) to F.A.T. and the National Institutes of Health (NIH, grant number 1R21AI120500) to L.M.S. and F.A.T.

Published

2019

14. Automated Behavioral Analysis of Large C. elegans Populations Using a Wide Field-of-view Tracking Platform

Author

Perni, Michele, Casford, Sam, Aprile, Francesco A, Nollen, Ellen A, Knowles, Tuomas PJ, Vendruscolo, Michele, Dobson, Christopher M, Perni, Michele [0000-0001-7593-8376], Aprile, Francesco [0000-0002-5040-4420], Knowles, Tuomas [0000-0002-7879-0140], Vendruscolo, Michele [0000-0002-3616-1610], and Apollo - University of Cambridge Repository

Subjects

GENES, IDENTIFICATION, Behavior, Animal, Drug discovery, large population analysis, nematode library, neurodegeneration, INHIBITION, Video Recording, amyloid formation, Alzheimer's disease, AGGREGATION, high-throughput screening, Issue 141, phenotype-based screening, MODEL, PROTEIN HOMEOSTASIS, C. elegans, Animals, Biological Assay, BETA-AMYLOID PEPTIDE, SCREEN, Caenorhabditis elegans, Immunology and Infection, LIFE-SPAN

Abstract

Caenorhabditis elegans is a well-established animal model in biomedical research, widely employed in functional genomics and ageing studies. To assess the health and fitness of the animals under study, one typically relies on motility readouts, such as the measurement of the number of body bends or the speed of movement. These measurements usually involve manual counting, making it challenging to obtain good statistical significance, as time and labor constraints often limit the number of animals in each experiment to 25 or less. Since high statistical power is necessary to obtain reproducible results and limit false positive and negative results when weak phenotypic effects are investigated, efforts have recently been made to develop automated protocols focused on increasing the sensitivity of motility detection and multi-parametric behavioral profiling. In order to extend the limit of detection to the level needed to capture the small phenotypic changes that are often crucial in genetic studies and drug discovery, we describe here a technological development that enables the study of up to 5,000 individual animals simultaneously, increasing the statistical power of the measurements by about 1,000-fold compared to manual assays and about 100-fold compared to other available automated methods.

Published

2018

15. Time-lapse 3D Imaging of Phagocytosis by Mouse Macrophages

Author

Janine J. Wilden, Markus Horsthemke, Peter J. Hanley, and Anne C. Bachg

Subjects

0301 basic medicine, Phagocytic cup, Phagocyte, General Chemical Engineering, Phagocytosis, Complement receptor, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Mice, Imaging, Three-Dimensional, Live cell imaging, medicine, Animals, Receptor, Opsonin, Immunology and Infection, Phagocytes, Microscopy, Confocal, General Immunology and Microbiology, Chemistry, General Neuroscience, Macrophages, Actin cytoskeleton, Cell biology, 030104 developmental biology, medicine.anatomical_structure

Abstract

Phagocytosis plays a key role in host defense, as well as in tissue development and maintenance, and involves rapid, receptor-mediated rearrangements of the actin cytoskeleton to capture, envelop and engulf large particles. Although phagocytic receptors, downstream signaling pathways, and effectors, such as Rho GTPases, have been identified, the dynamic cytoskeletal remodeling of specific receptor-mediated phagocytic events remain unclear. Four decades ago, two distinct mechanisms of phagocytosis, exemplified by Fcγ receptor (FcγR)- and complement receptor (CR)-mediated phagocytosis, were identified using scanning electron microscopy. Binding of immunoglobulin G (IgG)-opsonized particles to FcγRs triggers the protrusion of thin membrane extensions, which initially form a so-called phagocytic cup around the particle before it becomes completely enclosed and retracted into the cell. In contrast, complement opsonized particles appear to sink into the phagocyte following binding to complement receptors. These two modes of phagocytosis, phagocytic cup formation and sinking in, have become well established in the literature. However, the distinctions between the two modes have become blurred by reports that complement receptor-mediated phagocytosis may induce various membrane protrusions. With the availability of high resolution imaging techniques, phagocytosis assays are required that allow real-time 3D (three dimensional) visualization of how specific phagocytic receptors mediate the uptake of individual particles. More commonly used approaches for the study of phagocytosis, such as end-point assays, miss the opportunity to understand what is happening at the interface of particles and phagocytes. Here we describe phagocytic assays, using time-lapse spinning disk confocal microscopy, that allow 3D imaging of single phagocytic events. In addition, we describe assays to unambiguously image Fcγ receptor- or complement receptor-mediated phagocytosis.

Published

2018

16. Evaluation of Zika Virus-specific T-cell Responses in Immunoprivileged Organs of Infected Ifnar1-/- Mice

Author

Min Zhao, Hangjie Zhang, Xiangdong Li, Yingze Zhao, Kefang Liu, Yongli Zhang, Xuancheng Lu, Wenqiang Ma, Fuping Zhang, William J. Liu, and George F. Gao

Subjects

0301 basic medicine, antigen-specific T cell, General Chemical Engineering, T cell, T-Lymphocytes, Spleen, Inflammation, Receptor, Interferon alpha-beta, Biology, Immunofluorescence, Issue 140, General Biochemistry, Genetics and Molecular Biology, Virus, Epitope, 03 medical and health sciences, Mice, Immune system, immunoprivileged organs, medicine, Animals, Immunology and Infection, General Immunology and Microbiology, medicine.diagnostic_test, Zika Virus Infection, tetramer, General Neuroscience, Zika Virus, vaccination, Virology, 030104 developmental biology, medicine.anatomical_structure, Immunization, medicine.symptom

Abstract

The Zika virus (ZIKV) can induce inflammation in immunoprivileged organs (e.g., the brain and testis), leading to the Guillain-Barre syndrome and damaging the testes. During an infection with the ZIKV, immune cells have been shown to infiltrate into the tissues. However, the cellular mechanisms that define the protection and/or immunopathogenesis of these immune cells during a ZIKV infection are still largely unknown. Herein, we describe methods to evaluate the virus-specific T-cell functionality in these immunoprivileged organs of ZIKV-infected mice. These methods include a) a ZIKV infection and vaccine inoculation in Ifnar1-/- mice; b) histopathology, immunofluorescence, and immunohistochemistry assays to detect the virus infection and inflammation in the brain, testes, and spleen; c) the preparation of a tetramer of ZIKV-derived T-cell epitopes; d) the detection of ZIKV-specific T cells in the monocytes isolated from the brain, testes, and spleen. Using these approaches, it is possible to detect the antigen-specific T cells that have infiltrated into the immunoprivileged organs and to evaluate the functions of these T cells during the infection: potential immune protection via virus clearance and/or immunopathogenesis to exacerbate the inflammation. These findings may also help to clarify the contribution of T cells induced by the immunization against ZIKV.

Published

2018

17. Antigenic Liposomes for Generation of Disease-specific Antibodies

Author

Dharmendra Raghuwanshi, Lakeya C. Hardy, Shiteng Duan, Johanna Smeekens, Mike Kulis, Kyle J. Bednar, and Matthew S. Macauley

Subjects

0301 basic medicine, Immunogen, Arachis, T-Lymphocytes, General Chemical Engineering, medicine.medical_treatment, Peanut allergy, General Biochemistry, Genetics and Molecular Biology, Mice, 03 medical and health sciences, 0302 clinical medicine, Antigen, Calcium flux, medicine, Animals, Humans, Peanut Hypersensitivity, Anaphylaxis, Immunology and Infection, General Immunology and Microbiology, biology, General Neuroscience, Reproducibility of Results, Allergens, Immunoglobulin E, medicine.disease, Vaccination, 030104 developmental biology, Immunization, Liposomes, Immunology, biology.protein, Nanoparticles, Female, Antibody, Adjuvant, Food Hypersensitivity, 030215 immunology

Abstract

Antibody responses provide critical protective immunity to a wide array of pathogens. There remains a high interest in generating robust antibodies for vaccination as well as understand how pathogenic antibody responses develop in allergies and autoimmune disease. Generating robust antigen-specific antibody responses is not always trivial. In mouse models, it often requires multiple rounds of immunizations with adjuvant that leads to a great deal of variability in the levels of induced antibodies. One example is in mouse models of peanut allergies where more robust and reproducible models that minimize mouse numbers and the use of adjuvant would be beneficial. Presented here is a highly reproducible mouse model of peanut allergy anaphylaxis. This new model relies on two key factors: (1) antigen-specific splenocytes are adoptively transferred from a peanut-sensitized mouse into a naïve recipient mouse, normalizing the number of antigen-specific memory B- and T-cells across a large number of mice; and (2) recipient mice are subsequently boosted with a strong multivalent immunogen in the form of liposomal nanoparticles displaying the major peanut allergen (Ara h 2). The major advantage of this model is its reproducibility, which ultimately lowers the number of animals used in each study, while minimizing the number of animals receiving multiple injections of adjuvant. The modular assembly of these immunogenic liposomes provides relatively facile adaptability to other allergic or autoimmune models that involve pathogenic antibodies.

Published

2018

18. Listeria monocytogenes Infection of the Brain

Author

Pallab, Ghosh and Darrren E, Higgins

Subjects

Disease Models, Animal, Mice, Animals, Brain, Listeriosis, Listeria monocytogenes, Immunology and Infection

Abstract

Listeria monocytogenes is an intracellular bacterial pathogen that is frequently associated with food-borne infection. The ability of L. monocytogenes to cross the blood-brain barrier (BBB) is concerning as it can lead to life-threatening meningitis and encephalitis. The BBB protects the brain microenvironment from various toxic metabolites and microbial pathogens found in the blood following infection, and therefore supports brain homeostasis. The mechanisms by which L. monocytogenes present in the bloodstream cross the BBB to cause brain infections are not fully understood and there is also a lack of a robust model system to study brain infections by L. monocytogenes. Here, we present a simple mouse infection model to determine whether bacteria have crossed the BBB and to quantitate the burden of bacteria that have colonized the brain in vivo. In this method, animals were infected intravenously with L. monocytogenes and were humanely euthanized by exposure to CO(2) followed by cervical dislocation. Cardiac perfusion of the animals was performed prior to harvesting infected organs. Blood was collected before perfusion and the number of bacteria per organ or mL of blood was determined by plating dilutions of the blood or organ homogenates on agar plates and counting the number of colonies formed. This method can be used to study novel receptor-ligand interactions that enhance infection of the brain by L. monocytogenes and can be easily adapted for the study of multiple bacterial pathogens.

Published

2018

19. Modeling Tuberculosis in Mycobacterium marinum Infected Adult Zebrafish

Author

Hanna, Luukinen, Milka Marjut, Hammarén, Leena-Maija, Vanha-Aho, and Mataleena, Parikka

Subjects

Disease Models, Animal, Host-Pathogen Interactions, Mycobacterium marinum, Animals, Gene Expression, Mycobacterium Infections, Nontuberculous, Real-Time Polymerase Chain Reaction, Zebrafish, Immunology and Infection

Abstract

Mycobacterium tuberculosis is currently the deadliest human pathogen causing 1.7 million deaths and 10.4 million infections every year. Exposure to this bacterium causes a wide disease spectrum in humans ranging from a sterilized infection to an actively progressing deadly disease. The most common form is the latent tuberculosis, which is asymptomatic, but has the potential to reactivate into a fulminant disease. Adult zebrafish and its natural pathogen Mycobacterium marinum have recently proven to be an applicable model to study the wide disease spectrum of tuberculosis. Importantly, spontaneous latency and reactivation as well as adaptive immune responses in the context of mycobacterial infection can be studied in this model. In this article, we describe methods for the experimental infection of adult zebrafish, the collection of internal organs for the extraction of nucleic acids for the measurement of mycobacterial loads and host immune responses by quantitative PCR. The in-house-developed, M. marinum-specific qPCR assay is more sensitive than the traditional plating methods as it also detects DNA from non-dividing, dormant or recently dead mycobacteria. As both DNA and RNA are extracted from the same individual, it is possible to study the relationships between the diseased state, and the host and pathogen gene-expression. The adult zebrafish model for tuberculosis thus presents itself as a highly applicable, non-mammalian in vivo system to study host-pathogen interactions.

Published

2018

20. Mouse Models Of Helicobacter Infection And Gastric Pathologies

Author

D'Costa, Kimberley, Chonwerawong, Michelle, Tran, Le Son, and Ferrero, Richard L.

Subjects

Disease Models, Animal, Mice, Helicobacter pylori, Gastric Mucosa, Animals, Humans, Immunology and Infection, Helicobacter Infections

Abstract

Helicobacter pylori is a gastric pathogen that is present in half of the global population and is a significant cause of morbidity and mortality in humans. Several mouse models of gastric Helicobacter infection have been developed to study the molecular and cellular mechanisms whereby H. pylori bacteria colonize the stomach of human hosts and cause disease. Herein, we describe protocols to: 1) prepare bacterial suspensions for the in vivo infection of mice via intragastric gavage; 2) determine bacterial colonization levels in mouse gastric tissues, by polymerase chain reaction (PCR) and viable counting; and 3) assess pathological changes, by histology. To establish Helicobacter infection in mice, specific pathogen-free (SPF) animals are first inoculated with suspensions (containing ≥10(5) colony-forming units, CFUs) of mouse-colonizing strains of either Helicobacter pylori or other gastric Helicobacter spp. from animals, such as Helicobacter felis. At the appropriate time-points post-infection, stomachs are excised and dissected sagittally into two equal tissue fragments, each comprising the antrum and body regions. One of these fragments is then used for either viable counting or DNA extraction, while the other is subjected to histological processing. Bacterial colonization and histopathological changes in the stomach may be assessed routinely in gastric tissue sections stained with Warthin-Starry, Giemsa or Haematoxylin and Eosin (H&E) stains, as appropriate. Additional immunological analyses may also be undertaken by immunohistochemistry or immunofluorescence on mouse gastric tissue sections. The protocols described below are specifically designed to enable the assessment in mice of gastric pathologies resembling those in human-related H. pylori diseases, including inflammation, gland atrophy and lymphoid follicle formation. The inoculum preparation and intragastric gavage protocols may also be adapted to study the pathogenesis of other enteric human pathogens that colonize mice, such as Salmonella Typhimurium or Citrobacter rodentium.

Published

2018

21. Isolation, Fixation, and Immunofluorescence Imaging of Mouse Adrenal Glands

Author

Isabella Finco and Gary D. Hammer

Subjects

0301 basic medicine, Pathology, medicine.medical_specialty, Cell type, medicine.diagnostic_test, General Immunology and Microbiology, Chemistry, Adrenal gland, Adrenal cortex, General Chemical Engineering, General Neuroscience, Immunofluorescence, General Biochemistry, Genetics and Molecular Biology, Staining, 03 medical and health sciences, Mice, 030104 developmental biology, medicine.anatomical_structure, Adrenal Glands, medicine, Endocrine system, Animals, Adrenal medulla, Hormone, Immunology and Infection

Abstract

Immunofluorescence is a well-established technique for detection of antigens in tissues with the employment of fluorochrome-conjugated antibodies and has a broad spectrum of applications. Detection of antigens allows for characterization and identification of multiple cell types. Located above the kidneys and encapsulated by a layer of mesenchymal cells, the adrenal gland is an endocrine organ composed by two different tissues with different embryological origins, the mesonephric intermediate mesoderm-derived outer cortex and the neural crest-derived inner medulla. The adrenal cortex secretes steroids (i.e., mineralocorticoids, glucocorticoids, sex hormones), whereas the adrenal medulla produces catecholamines (i.e., adrenaline, noradrenaline). While conducting adrenal research, it is important to be able to distinguish unique cells with different functions. Here we provide a protocol developed in our laboratory that describes a series of sequential steps required for obtaining immunofluorescence staining to characterize the cell types of the adrenal gland. We focus first on the dissection of the mouse adrenal glands, the microscopic removal of periadrenal fat followed by the fixation, processing and paraffin embedding of the tissue. We then describe sectioning of the tissue blocks with a rotary microtome. Lastly, we detail a protocol for immunofluorescent staining of adrenal glands that we have developed to minimize both non-specific antibody binding and autofluorescence in order to achieve an optimal signal.

Published

2018

22. An Ex Vivo Chicken Primary Bursal-cell Culture Model to Study Infectious Bursal Disease Virus Pathogenesis

Author

Dulwich, Katherine L., Asfor, Amin S., Gray, Alice G., Nair, Venugopal, and Broadbent, Andrew J.

Subjects

IBDV, B cells, B-Lymphocytes, animal structures, infectious bursal disease virus, Cell Survival, Primary Cell Culture, primary cells, virus, Birnaviridae Infections, Virus Replication, Issue 140, Chicken, Bursa of Fabricius, Animals, Chickens, Poultry Diseases, Immunology and Infection

Abstract

Infectious bursal disease virus (IBDV) is a birnavirus of economic importance to the poultry industry. The virus infects B cells, causing morbidity, mortality, and immunosuppression in infected birds. In this study, we describe the isolation of chicken primary bursal cells from the bursa of Fabricius, the culture and infection of the cells with IBDV, and the quantification of viral replication. The addition of chicken CD40 ligand significantly increased cell proliferation fourfold over six days of culture and significantly enhanced cell viability. Two strains of IBDV, a cell-culture adapted strain, D78, and a very virulent strain, UK661, replicated well in the ex vivo cell cultures. This model will be of use in determining how cells respond to IBDV infection and will permit a reduction in the number of infected birds used in IBDV pathogenesis studies. The model can also be expanded to include other viruses and could be applied to different species of birds.

Published

2018

23. Oral Intubation of Adult Zebrafish: A Model for Evaluating Intestinal Uptake of Bioactive Compounds

Author

Nerea Roher, Rosemary Thwaite, and Jie Ji

Subjects

0301 basic medicine, General Chemical Engineering, Administration, Oral, Pharmacology, General Biochemistry, Genetics and Molecular Biology, Flow cytometry, 03 medical and health sciences, chemistry.chemical_compound, Immune system, Intestinal mucosa, Adjuvants, Immunologic, In vivo, medicine, Water environment, Animals, Intestinal Mucosa, Intubation, Gastrointestinal, Zebrafish, Immunology and Infection, Lamina propria, medicine.diagnostic_test, General Immunology and Microbiology, business.industry, General Neuroscience, Biological Transport, Bioactive compound, 030104 developmental biology, medicine.anatomical_structure, Real-time polymerase chain reaction, chemistry, business

Abstract

Most pathogens invade organisms through their mucosa. This is particularly true in fish as they are continuously exposed to a microbial-rich water environment. Developing effective methods for oral delivery of immunostimulants or vaccines, which activate the immune system against infectious diseases, is highly desirable. In devising prophylactic tools, good experimental models are needed to test their performance. Here, we show a method for oral intubation of adult zebrafish and a set of procedures to dissect and prepare the intestine for cytometry, confocal microscopy and quantitative polymerase chain reaction (qPCR) analysis. With this protocol, we can precisely administer volumes up to 50 µL to fish weighing approximately 1 g simply and quickly, without harming the animals. This method allows us to explore the direct in vivo uptake of fluorescently labelled compounds by the intestinal mucosa and the immunomodulatory capacity of such biologics at the local site after intubation. By combining downstream methods such as flow cytometry, histology, qPCR and confocal microscopy of the intestinal tissue, we can understand how immunostimulants or vaccines are able to cross the intestinal mucosal barriers, pass through the lamina propria, and reach the muscle, exerting an effect on the intestinal mucosal immune system. The model could be used to test candidate oral prophylactics and delivery systems or the local effect of any orally administered bioactive compound.

Published

2018

24. Single-cell Quantitation of mRNA and Surface Protein Expression in Simian Immunodeficiency Virus-infected CD4(+) T Cells Isolated from Rhesus macaques

Author

Tokarev, Andrey, Creegan, Matthew, Eller, Michael A., Roederer, Mario, and Bolton, Diane L.

Subjects

CD4-Positive T-Lymphocytes, Simian Acquired Immunodeficiency Syndrome, Animals, Membrane Proteins, Simian Immunodeficiency Virus, RNA, Messenger, Macaca mulatta, Immunology and Infection

Abstract

Single-cell analysis is an important tool for dissecting heterogeneous populations of cells. The identification and isolation of rare cells can be difficult. To overcome this challenge, a methodology combining indexed flow cytometry and high-throughput multiplexed quantitative polymerase chain reaction (qPCR) was developed. The objective was to identify and characterize simian immunodeficiency virus (SIV)-infected cells present within rhesus macaques. Through quantitation of surface protein by fluorescence-activated cell sorting (FACS) and mRNA by qPCR, virus-infected cells are identified by viral gene expression, which is combined with host gene and protein measurements to create a multidimensional profile. We term the approach, targeted Single-Cell Proteo-transcriptional Evaluation, or tSCEPTRE. To perform the method, viable cells are stained with fluorescent antibodies specific for surface markers used for FACS isolation of a cell subset and/or downstream phenotypic analysis. Single cells are sorted followed by immediate lysis, multiplex reverse transcription (RT), PCR pre-amplification, and high throughput qPCR of up to 96 transcripts. FACS measurements are recorded at the time of sorting and subsequently linked to the gene expression data by well position to create a combined protein and transcriptional profile. To study SIV-infected cells directly ex vivo, cells were identified by qPCR detection of multiple viral RNA species. The combination of viral transcripts and the quantity of each provide a framework for classifying cells into distinct stages of the viral life cycle (e.g., productive versus non-productive). Moreover, tSCEPTRE of SIV(+) cells were compared to uninfected cells isolated from the same specimen to assess differentially expressed host genes and proteins. The analysis revealed previously unappreciated viral RNA expression heterogeneity among infected cells as well as in vivo SIV-mediated post-transcriptional gene regulation with single-cell resolution. The tSCEPTRE method is relevant for the analysis of any cell population amenable to identification by expression of surface protein marker(s), host or pathogen gene(s), or combinations thereof.

Published

2018

25. In Vitro Differentiation of Mouse Granulocyte-macrophage-colony-stimulating Factor (GM-CSF)-producing T Helper (THGM) Cells

Author

Yi, Lu, Xin-Yuan, Fu, and Yongliang, Zhang

Subjects

Mice, Interleukin-17, Animals, Granulocyte-Macrophage Colony-Stimulating Factor, Interferon-alpha, Cell Differentiation, T-Lymphocytes, Helper-Inducer, Immunology and Infection

Abstract

The granulocyte-macrophage-colony-stimulating factor (GM-CSF)-producing T helper (T(H)GM) cell is a newly identified T helper cell subset that predominantly secretes GM-CSF without producing interferon (IFN)γ or interleukin (IL)-17 and is found to play an essential role in the autoimmune neuroinflammation. A method of isolation of naive CD4+ T cells from a single-cell suspension of splenocytes and T(H)GM cell generation from naive CD4+ T cells would be a useful technique in the study of T cell-mediated immunity and autoimmune diseases. Here we describe a method that differentiates mouse naive CD4+ T cells into T(H)GM cells promoted by IL-7. The outcome of the differentiation was assessed by the analysis of the cytokines expression using different techniques, including intracellular cytokine staining combined with flow cytometry, a quantitative real-time polymerase chain reaction (PCR), and enzyme-linked immunosorbent assays (ELISA). Using the T(H)GM differentiation protocol as described here, about 55% of the cells expressed GM-CSF with a minimal expression of IFNα or IL-17. The predominant expression of GM-CSF by T(H)GM cells was further confirmed by the analysis of the expression of GM-CSF, IFNα, and IL-17 at both mRNA and protein levels. Thus, this method can be used to differentiate naive CD4+ T cells to T(H)GM cells in vitro, which will be useful in the study of T(H)GM cell biology.

Published

2018

26. Mouse Body Temperature Measurement Using Infrared Thermometer During Passive Systemic Anaphylaxis and Food Allergy Evaluation

Author

Yu Kawakami, Toshiaki Kawakami, and Rachel Sielski

Subjects

0301 basic medicine, Materials science, Infrared Rays, Thermometers, General Chemical Engineering, Body temperature measurement, Temperature measurement, General Biochemistry, Genetics and Molecular Biology, Degree (temperature), Mice, 03 medical and health sciences, Systemic anaphylaxis, Food allergy, Body surface, medicine, Animals, Humans, Anaphylaxis, Immunology and Infection, General Immunology and Microbiology, General Neuroscience, Temperature, medicine.disease, 030104 developmental biology, Infrared thermometer, Female, Temperature drop, Food Hypersensitivity, Biomedical engineering

Abstract

Mouse body temperature measurement is of paramount importance for investigating allergies and anaphylactic symptoms. Rectal probes for temperature readings is common, and they have been proven to be accurate and invaluable in this regard. However, this method of temperature measurement requires the mice to be anesthetized in order to insert the probe without injury to the animal. This limits the ability to observe other phenotypes of the mouse simultaneously. In order to investigate other phenotypes while measuring temperatures, rectal probes are not ideal, and another method is desired. Here, we introduce a noninvasive method of temperature measurement that foregoes the requirement for mouse anesthesia while maintaining equal reliability to rectal probes in measuring body temperature. We use an infrared thermometer that detects body surface temperatures at ranges between 2 and 150 mm. This method of body temperature measurement is successful in reliably replicating temperature change trends during passive system anaphylaxis experiments in mice. We show that body surface temperatures are about 2.0 °C lower than rectal probe measurements, but the degree of temperature drop follows the same trend. Furthermore, we use the same technique to observe mice in a food allergy model to evaluate temperature and activity levels simultaneously.

Published

2018

27. Arbovirus Infections As Screening Tools for the Identification of Viral Immunomodulators and Host Antiviral Factors

Author

Emily A. Rex, Dahee Seo, and Don B. Gammon

Subjects

General Immunology and Microbiology, biology, Arbovirus Infections, viruses, General Chemical Engineering, General Neuroscience, Virus Replication, biology.organism_classification, medicine.disease, Antiviral Agents, Arbovirus, Virology, General Biochemistry, Genetics and Molecular Biology, Virus, Viral replication, Genome editing, Vesicular stomatitis virus, RNA interference, medicine, Animals, Immunologic Factors, Mass Screening, Mass screening, Immunology and Infection

Abstract

RNA interference- and genome editing-based screening platforms have been widely used to identify host cell factors that restrict virus replication. However, these screens are typically conducted in cells that are naturally permissive to the viral pathogen under study. Therefore, the robust replication of viruses in control conditions may limit the dynamic range of these screens. Furthermore, these screens may be unable to easily identify cellular defense pathways that restrict virus replication if the virus is well-adapted to the host and capable of countering antiviral defenses. In this article, we describe a new paradigm for exploring virus-host interactions through the use of screens that center on naturally abortive infections by arboviruses such as vesicular stomatitis virus (VSV). Despite the ability of VSV to replicate in a wide range of dipteran insect and mammalian hosts, VSV undergoes a post-entry, abortive infection in a variety of cell lines derived from lepidopteran insects, such as the gypsy moth (Lymantria dispar). However, these abortive VSV infections can be "rescued" when host cell antiviral defenses are compromised. We describe how VSV strains encoding convenient reporter genes and restrictive L. dispar cell lines can be paired to set-up screens to identify host factors involved in arbovirus restriction. Furthermore, we also show the utility of these screening tools in the identification of virally encoded factors that rescue VSV replication during coinfection or through ectopic expression, including those encoded by mammalian viruses. The natural restriction of VSV replication in L. dispar cells provides a high signal-to-noise ratio when screening for the conditions that promote VSV rescue, thus enabling the use of simplistic luminescence- and fluorescence-based assays to monitor the changes in VSV replication. These methodologies are valuable for understanding the interplay between host antiviral responses and viral immune evasion factors.

Published

2018

28. An In Vivo Mouse Model to Measure Naïve CD4 T Cell Activation, Proliferation and Th1 Differentiation Induced by Bone Marrow-derived Dendritic Cells

Author

Raquel, Toribio-Fernandez, Virginia, Zorita, Beatriz, Herrero-Fernandez, and Jose M, Gonzalez-Granado

Subjects

CD4-Positive T-Lymphocytes, Disease Models, Animal, Mice, Animals, Bone Marrow Cells, Cell Differentiation, Dendritic Cells, Th1 Cells, Cell Proliferation, Immunology and Infection

Abstract

Quantification of naïve CD4 T cell activation, proliferation, and differentiation to T helper 1 (Th1) cells is a useful way to assess the role played by T cells in an immune response. This protocol describes the in vitro differentiation of bone marrow (BM) progenitors to obtain granulocyte macrophage colony-stimulating factor (GM-CSF) derived-dendritic cells (DCs). The protocol also describes the adoptive transfer of ovalbumin peptide (OVAp)-loaded GM-CSF-derived DCs and naïve CD4 T cells from OTII transgenic mice in order to analyze the in vivo activation, proliferation, and Th1 differentiation of the transferred CD4 T cells. This protocol circumvents the limitation of purely in vivo methods imposed by the inability to specifically manipulate or select the studied cell population. Moreover, this protocol allows studies in an in vivo environment, thus avoiding alterations to functional factors that may occur in vitro and including the influence of cell types and other factors only found in intact organs. The protocol is a useful tool for generating changes in DCs and T cells that modify adaptive immune responses, potentially providing important results to understand the origin or development of numerous immune associated diseases.

Published

2018

29. In Vitro Canine Neutrophil Extracellular Trap Formation: Dynamic and Quantitative Analysis by Fluorescence Microscopy

Author

Ronald H L, Li and Fern, Tablin

Subjects

Dogs, Microscopy, Fluorescence, Neutrophils, Animals, Humans, Extracellular Traps, Immunology and Infection

Abstract

In response to invading pathogens, neutrophils release neutrophil extracellular traps (NETs), which are extracellular networks of DNA decorated with histones and antimicrobial proteins. Excessive NET formation (NETosis) and citH3 release during sepsis is associated with multiple organ dysfunction and mortality in mice and humans but its implications in dogs are unknown. Herein, we describe a technique to isolate canine neutrophils from whole blood for observation and quantification of NETosis. Leukocyte-rich plasma, generated by dextran sedimentation, is separated by commercially available density gradient separation media and granulocytes collected for cell count and viability testing. To observe real-time NETosis in live neutrophils, cell permeant and cell impermeant fluorescent nucleic acid stains are added to neutrophils activated either by lipopolysaccharide (LPS) or phorbol 12-myristate 13-acetate (PMA). Changes in nuclear morphology and NET formation are observed over time by fluorescence microscopy. In vitro NETosis is further characterized by co-colocalization of cell-free DNA (cfDNA), myeloperoxidase (MPO) and citrullinated histone H3 (citH3) using a modified double-immunolabelling protocol. To objectively quantify NET formation and citH3 expression using fluorescence microscopy, NETs and citH3-positive cells are quantified in a blinded manner using available software. This technique is a specific assay to evaluate the in vitro capacity of canine neutrophils to undergo NETosis.

Published

2018

30. Characterization of Thymus-dependent and Thymus-independent Immunoglobulin Isotype Responses in Mice Using Enzyme-linked Immunosorbent Assay

Author

Sining Zhu, Ping Xie, and Almin I. Lalani

Subjects

0301 basic medicine, T-Lymphocytes, medicine.medical_treatment, General Chemical Engineering, Enzyme-Linked Immunosorbent Assay, chemical and pharmacologic phenomena, Biology, Immunoglobulin E, General Biochemistry, Genetics and Molecular Biology, Mice, 03 medical and health sciences, Antigen, medicine, Animals, Antigen-presenting cell, Immunology and Infection, General Immunology and Microbiology, General Neuroscience, Antigens, T-Independent, Isotype, Immunoglobulin Isotypes, 030104 developmental biology, Immunization, Antibody Formation, Humoral immunity, Immunology, biology.protein, Antibody, Adjuvant

Abstract

Antibodies, also termed as immunoglobulins (Ig), secreted by differentiated B lymphocytes, plasmablasts/plasma cells, in humoral immunity provide a formidable defense against invading pathogens via diverse mechanisms. One major goal of vaccination is to induce protective antigen-specific antibodies to prevent life-threatening infections. Both thymus-dependent (TD) and thymus-independent (TI) antigens can elicit robust antigen-specific IgM responses and can also induce the production of isotype-switched antibodies (IgG, IgA and IgE) as well as the generation of memory B cells with the help provided by antigen presenting cells (APCs). Here, we describe a protocol to characterize TD and TI Ig isotype responses in mice using enzyme-linked immunosorbent assay (ELISA). In this protocol, TD and TI Ig responses are elicited in mice by intraperitoneal (i.p.) immunization with hapten-conjugated model antigens TNP-KLH (in alum) and TNP-polysaccharide (in PBS), respectively. To induce TD memory response, a booster immunization of TNP-KLH in alum is given at 3 weeks after the first immunization with the same antigen/adjuvant. Mouse sera are harvested at different time points before and after immunization. Total serum Ig levels and TNP-specific antibodies are subsequently quantified using Ig isotype-specific Sandwich and indirect ELISA, respectively. In order to correctly quantify the serum concentration of each Ig isotype, the samples need to be appropriately diluted to fit within the linear range of the standard curves. Using this protocol, we have consistently obtained reliable results with high specificity and sensitivity. When used in combination with other complementary methods such as flow cytometry, in vitro culture of splenic B cells and immunohistochemical staining (IHC), this protocol will allow researchers to gain a comprehensive understanding of antibody responses in a given experimental setting.

Published

2018

31. Stereotactic Adoptive Transfer of Cytotoxic Immune Cells in Murine Models of Orthotopic Human Glioblastoma Multiforme Xenografts

Author

Cynthia Chauvin, Ulrich Jarry, Claire Pecqueur, Emmanuel Scotet, Béatrice Clémenceau, Noémie Joalland, Immunobiology of Human αβ and γδ T Cells and Immunotherapeutic Applications (CRCINA-ÉQUIPE 1), Centre de Recherche en Cancérologie et Immunologie Nantes-Angers (CRCINA), Institut National de la Santé et de la Recherche Médicale (INSERM)-Université de Nantes - UFR de Médecine et des Techniques Médicales (UFR MEDECINE), Université de Nantes (UN)-Université de Nantes (UN)-Centre hospitalier universitaire de Nantes (CHU Nantes)-Centre National de la Recherche Scientifique (CNRS)-Université d'Angers (UA)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Université de Nantes - UFR de Médecine et des Techniques Médicales (UFR MEDECINE), Université de Nantes (UN)-Université de Nantes (UN)-Centre hospitalier universitaire de Nantes (CHU Nantes)-Centre National de la Recherche Scientifique (CNRS)-Université d'Angers (UA), LabEx IGO 'Immunotherapy, Graft, Oncology' [Nantes], Unité de Thérapie Cellulaire et Génique [CHU Nantes] (UTCG), Hôtel-Dieu-Centre hospitalier universitaire de Nantes (CHU Nantes), Apoptosis and Tumor Progression (CRCINA-ÉQUIPE 9), Université d'Angers (UA)-Université de Nantes (UN)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS)-Centre hospitalier universitaire de Nantes (CHU Nantes)-Université d'Angers (UA)-Université de Nantes (UN)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS)-Centre hospitalier universitaire de Nantes (CHU Nantes), LabEX IGO Immunothérapie Grand Ouest, Nantes Université (Nantes Univ), and Bernardo, Elizabeth

Subjects

Adult, lymphocytes, Adoptive cell transfer, adoptive transfer, General Chemical Engineering, medicine.medical_treatment, Cell, [SDV.CAN]Life Sciences [q-bio]/Cancer, General Biochemistry, Genetics and Molecular Biology, Mice, 03 medical and health sciences, 0302 clinical medicine, Immune system, [SDV.CAN] Life Sciences [q-bio]/Cancer, Cell Line, Tumor, Issue 139, medicine, Animals, Humans, Cytotoxic T cell, Primary Brain Tumors, Immunology and Infection, Cancer, 030304 developmental biology, 0303 health sciences, General Immunology and Microbiology, Brain Neoplasms, business.industry, General Neuroscience, glioblastoma, Immunotherapy, stereotaxy, medicine.disease, Xenograft Model Antitumor Assays, 3. Good health, medicine.anatomical_structure, Cancer research, Heterografts, immunotherapy, business, 030217 neurology & neurosurgery, Glioblastoma

Abstract

International audience; Glioblastoma multiforme (GBM), the most frequent and aggressive primary brain cancer in adults, is generally associated with a poor prognosis, and scarce efficient therapies have been proposed over the last decade. Among the promising candidates for designing novel therapeutic strategies, cellular immunotherapies have been targeted to eliminate highly invasive and chemo-radioresistant tumor cells, likely involved in a rapid and fatal relapse of this cancer. Thus, administration(s) of allogeneic GBM-reactive immune cell effectors, such as human Vϒ9Vδ2 T lymphocytes, in the vicinity of the tumor would represents a unique opportunity to deliver efficient and highly concentrated therapeutic agents directly into the site of brain malignancies. Here, we present a protocol for the preparation and the stereotaxic administration of allogeneic human lymphocytes in immunodeficient mice carrying orthotopic human primary brain tumors. This study provides a preclinical proof-of-concept for both the feasibility and the antitumor efficacy of these cellular immunotherapies that rely on stereotactic injections of allogeneic human lymphocytes within intrabrain tumor beds.

Published

2018

32. Isolation and Identification of Extravascular Immune Cells of the Heart

Author

Xavier Clemente-Casares, Laura Aronoff, and Slava Epelman

Subjects

0301 basic medicine, General Chemical Engineering, Population, Inflammation, General Biochemistry, Genetics and Molecular Biology, Flow cytometry, 03 medical and health sciences, Mice, Immune system, medicine, Macrophage, Animals, Humans, education, Immunology and Infection, education.field_of_study, biology, medicine.diagnostic_test, General Immunology and Microbiology, Chemistry, General Neuroscience, Macrophages, Heart, Dendritic cell, Dendritic Cells, Cell sorting, Flow Cytometry, Cell biology, 030104 developmental biology, biology.protein, Antibody, medicine.symptom

Abstract

The immune system is an essential component of a healthy heart. The myocardium is home to a rich population of different immune cell subsets with functional compartmentalization both during steady state and during different forms of inflammation. Until recently, the study of immune cells in the heart required the use of microscopy or poorly developed digestion protocols, which provided enough sensitivity during severe inflammation but were unable to confidently identify small - but key - populations of cells during steady state. Here, we discuss a simple method combining enzymatic (collagenase, hyaluronidase and DNAse) and mechanical digestion of murine hearts preceded by intravascular administration of fluorescently-labelled antibodies to differentiate small but unavoidable intravascular cell contaminants. This method generates a suspension of isolated viable cells that can be analyzed by flow cytometry for identification, phenotyping and quantification, or further purified with fluorescence-activated cell sorting or magnetic bead separation for transcriptional analysis or in vitro studies. We include an example of a step-by-step flow cytometric analysis to differentiate the key macrophage and dendritic cell populations of the heart. For a medium sized experiment (10 hearts) the completion of the procedure requires 2-3 h.

Published

2018

33. Quantification of Efferocytosis by Single-cell Fluorescence Microscopy

Author

Bryan Heit, Daniel G. Wootton, Kyle Taruc, and Charles Yin

Subjects

0301 basic medicine, Cell signaling, Cellular differentiation, General Chemical Engineering, Cell, Apoptosis, General Biochemistry, Genetics and Molecular Biology, Flow cytometry, Mice, 03 medical and health sciences, Phagocytosis, Fluorescence microscope, medicine, Animals, Humans, Macrophage, Efferocytosis, Immunology and Infection, medicine.diagnostic_test, General Immunology and Microbiology, Chemistry, Macrophages, General Neuroscience, Cell Differentiation, Cell biology, 030104 developmental biology, medicine.anatomical_structure, Microscopy, Fluorescence, Biotinylation

Abstract

Studying the regulation of efferocytosis requires methods that are able to accurately quantify the uptake of apoptotic cells and to probe the signaling and cellular processes that control efferocytosis. This quantification can be difficult to perform as apoptotic cells are often efferocytosed piecemeal, thus necessitating methods which can accurately delineate between the efferocytosed portion of an apoptotic target versus residual unengulfed cellular fragments. The approach outlined herein utilizes dual-labeling approaches to accurately quantify the dynamics of efferocytosis and efferocytic capacity of efferocytes such as macrophages. The cytosol of the apoptotic cell is labeled with a cell-tracking dye to enable monitoring of all apoptotic cell-derived materials, while surface biotinylation of the apoptotic cell allows for differentiation between internalized and non-internalized apoptotic cell fractions. The efferocytic capacity of efferocytes is determined by taking fluorescent images of live or fixed cells and quantifying the amount of bound versus internalized targets, as differentiated by streptavidin staining. This approach offers several advantages over methods such as flow cytometry, namely the accurate delineation of non-efferocytosed versus efferocytosed apoptotic cell fractions, the ability to measure efferocytic dynamics by live-cell microscopy, and the capacity to perform studies of cellular signaling in cells expressing fluorescently-labeled transgenes. Combined, the methods outlined in this protocol serve as the basis for a flexible experimental approach that can be used to accurately quantify efferocytic activity and interrogate cellular signaling pathways active during efferocytosis.

Published

2018

34. Imaging Cell Interaction in Tracheal Mucosa During Influenza Virus Infection Using Two-photon Intravital Microscopy

Author

Diego Morone, Diego Ulisse Pizzagalli, Santiago F. Gonzalez, Tommaso Virgilio, and Miguel Palomino-Segura

Subjects

0301 basic medicine, Pathology, medicine.medical_specialty, Intravital Microscopy, General Chemical Engineering, Motility, Cell Communication, General Biochemistry, Genetics and Molecular Biology, Virus, Mice, 03 medical and health sciences, Immune system, Two-photon excitation microscopy, In vivo, Animals, Medicine, Respiratory system, Immunology and Infection, Photons, Mucous Membrane, General Immunology and Microbiology, business.industry, General Neuroscience, Dendritic cell, Trachea, 030104 developmental biology, business, Intravital microscopy

Abstract

The analysis of cell-cell or cell-pathogen interaction in vivo is an important tool to understand the dynamics of the immune response to infection. Two-photon intravital microscopy (2P-IVM) allows the observation of cell interactions in deep tissue in living animals, while minimizing the photobleaching generated during image acquisition. To date, different models for 2P-IVM of lymphoid and non-lymphoid organs have been described. However, imaging of respiratory organs remains a challenge due to the movement associated with the breathing cycle of the animal. Here, we describe a protocol to visualize in vivo immune cell interactions in the trachea of mice infected with influenza virus using 2P-IVM. To this purpose, we developed a custom imaging platform, which included the surgical exposure and intubation of the trachea, followed by the acquisition of dynamic images of neutrophils and dendritic cells (DC) in the mucosal epithelium. Additionally, we detailed the steps needed to perform influenza intranasal infection and flow cytometric analysis of immune cells in the trachea. Finally, we analyzed neutrophil and DC motility as well as their interactions during the course of a movie. This protocol allows for the generation of stable and bright 4D images necessary for the assessment of cell-cell interactions in the trachea.

Published

2018

35. Generation of Large Numbers of Myeloid Progenitors and Dendritic Cell Precursors from Murine Bone Marrow Using a Novel Cell Sorting Strategy

Author

Peter B. Rogers and Elizabeth Hiltbold Schwartz

Subjects

0301 basic medicine, Cell type, Myeloid, General Chemical Engineering, Cellular differentiation, Population, Bone Marrow Cells, Cell Separation, Monocytes, General Biochemistry, Genetics and Molecular Biology, Mice, 03 medical and health sciences, medicine, Animals, education, Myeloid Progenitor Cells, Immunology and Infection, MHC class II, education.field_of_study, General Immunology and Microbiology, biology, General Neuroscience, Monocyte, Cell Differentiation, Dendritic Cells, Dendritic cell, Cell sorting, Cell biology, 030104 developmental biology, medicine.anatomical_structure, biology.protein

Abstract

Cultures of monocyte-derived dendritic cells (moDC) generated from mouse bone marrow using Granulocyte-Macrophage Colony Stimulating Factor (GM-CSF) have recently been recognized to be more heterogeneous than previously appreciated. These cultures routinely contain moDC as well monocyte-derived macrophages (moMac), and even some less developed cells such as monocytes. The goal of this protocol is to provide a consistent method for identification and separation of the many cell types present in these cultures as they develop, so that their specific functions may be further investigated. The sorting strategy presented here separates cells first into four populations based on expression of Ly6C and CD115, both of which are expressed transiently by cells as they develop in GM-CSF-driven culture. These four populations include Common myeloid progenitors or CMP (Ly6C-, CD115-), granulocyte/macrophage progenitors or GMP (Ly6C+, CD115-), monocytes (Ly6C+, CD115+), and monocyte-derived macrophages or moMac (Ly6C-, CD115+). CD11c is also added to the sorting strategy to distinguish two populations within the Ly6C-, CD115- population: CMP (CD11c-) and moDC (CD11c+). Finally, two populations may be further distinguished within the Ly6C-, CD115+ population based on the level of MHC class II expression. MoMacs express lower levels of MHC class II, while a monocyte-derived DC precursor (moDP) expresses higher MHC class II. This method allows for the reliable isolation of several developmentally distinct populations in numbers sufficient for a variety of functional and developmental analyses. We highlight one such functional readout, the differential responses of these cell types to stimulation with Pathogen-Associated Molecular Patterns (PAMPs).

Published

2018

36. Quantifying Vibrio cholerae Colonization and Diarrhea in the Adult Zebrafish Model

Author

Dhrubajyoti, Nag, Kristie, Mitchell, Paul, Breen, and Jeffrey H, Withey

Subjects

Diarrhea, Disease Models, Animal, animal structures, fungi, Animals, Humans, Vibrio cholerae, Zebrafish, Immunology and Infection

Abstract

Vibrio cholerae is best known as the infectious agent that causes the human disease cholera. Outside the human host, V. cholerae primarily exists in the aquatic environment, where it interacts with a variety of higher aquatic species. Vertebrate fish are known to be an environmental host and are a potential V. cholerae reservoir in nature. Both V. cholerae and the teleost fish species Danio rerio, commonly known as zebrafish, originate from the Indian subcontinent, suggesting a long-standing interaction in aquatic environments. Zebrafish are an ideal model organism for studying many aspects of biology, including infectious diseases. Zebrafish can be easily and rapidly colonized by V. cholerae after exposure in water. Intestinal colonization by V. cholerae leads to the production of diarrhea and the excretion of replicated V. cholerae. These excreted bacteria can then go on to colonize new fish hosts. Here, we demonstrate how to assess V. cholerae-intestinal colonization in zebrafish and how to quantify V. cholerae-induced zebrafish diarrhea. The colonization model should be useful to researchers who are studying whether genes of interest may be important for host colonization and/or for environmental survival. The quantification of zebrafish diarrhea should be useful to researchers studying any intestinal pathogen who are interested in exploring zebrafish as a model system.

Published

2018

37. Identification and Isolation of Oligopotent and Lineage-committed Myeloid Progenitors from Mouse Bone Marrow

Author

Helen S. Goodridge and Alberto Yáñez

Subjects

Myeloid, medicine.diagnostic_test, General Immunology and Microbiology, Cellular differentiation, General Chemical Engineering, General Neuroscience, Cell Differentiation, Cell sorting, Biology, Flow Cytometry, General Biochemistry, Genetics and Molecular Biology, Flow cytometry, Cell biology, Mice, Haematopoiesis, medicine.anatomical_structure, Bone Marrow, medicine, Animals, Bone marrow, Progenitor cell, Myeloid Progenitor Cells, Immunology and Infection, Progenitor

Abstract

Myeloid progenitors that yield neutrophils, monocytes and dendritic cells (DCs) can be identified in and isolated from the bone marrow of mice for hematological and immunological analyses. For example, studies of the cellular and molecular properties of myeloid progenitor populations can reveal mechanisms underlying leukemic transformation, or demonstrate how the immune system responds to pathogen exposure. Previously described flow cytometry strategies for myeloid progenitor identification have enabled significant advances in many fields, but the fractions they identify are very heterogeneous. The most commonly used gating strategies define bone marrow fractions that are enriched for the desired populations, but also contain large numbers of "contaminating" progenitors. Our recent studies have resolved much of this heterogeneity, and the protocol we present here permits the isolation of 6 subpopulations of oligopotent and lineage-committed myeloid progenitors from 2 previously described bone marrow fractions. The protocol describes 3 stages: 1) isolation of bone marrow cells, 2) enrichment for hematopoietic progenitors by magnetic-activated cell sorting (lineage depletion by MACS), and 3) identification of myeloid progenitor subsets by flow cytometry (including fluorescence-activated cell sorting, FACS, if desired). This approach permits progenitor quantification and isolation for a variety of in vitro and in vivo applications, and has already yielded novel insight into pathways and mechanisms of neutrophil, monocyte, and DC differentiation.

Published

2018

38. Isolation, Expansion, and Adipogenic Induction of CD34+CD31+ Endothelial Cells from Human Omental and Subcutaneous Adipose Tissue

Author

Ryan W. Huyck, Avennette Pinto, Ashley J James, Omnia U Gaafar, Bronson A. Haynes, Anca D. Dobrian, Meghan E Carter, and Marjorie Day

Subjects

0301 basic medicine, Male, medicine.medical_specialty, Cellular differentiation, General Chemical Engineering, Population, Subcutaneous Fat, Adipose tissue, Inflammation, Antigens, CD34, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, chemistry.chemical_compound, Adipocyte, Internal medicine, medicine, Animals, Humans, education, Immunology and Infection, education.field_of_study, General Immunology and Microbiology, business.industry, General Neuroscience, Endothelial Cells, Cell Differentiation, Stromal vascular fraction, Obesity, Morbid, Platelet Endothelial Cell Adhesion Molecule-1, 030104 developmental biology, Endocrinology, chemistry, Adipogenesis, medicine.symptom, Adipocyte hypertrophy, business, Omentum

Abstract

Obesity is accompanied by an extensive remodeling of adipose tissue primarily via adipocyte hypertrophy. Extreme adipocyte growth results in a poor response to insulin, local hypoxia, and inflammation. By stimulating the differentiation of functional white adipocytes from progenitors, radical hypertrophy of the adipocyte population can be prevented and, consequently, the metabolic health of adipose tissue can be improved along with a reduction of inflammation. Also, by stimulating a differentiation of beige/brown adipocytes, the total body energy expenditure can be increased, resulting in weight loss. This approach could prevent the development of obesity co-morbidities such as type 2 diabetes and cardiovascular disease. This paper describes the isolation, expansion, and differentiation of white and beige adipocytes from a subset of human adipose tissue endothelial cells that co-express the CD31 and CD34 markers. The method is relatively cheap and is not labor-intensive. It requires access to human adipose tissue and the subcutaneous depot is suitable for sampling. For this protocol, fresh adipose tissue samples from morbidly obese subjects [body mass index (BMI) >35] are collected during bariatric surgery procedures. Using a sequential immunoseparation from the stromal vascular fraction, enough cells are produced from as little as 2-3 g of fat. These cells can be expanded in culture over 10-14 days, can be cryopreserved, and retain their adipogenic properties with passaging up to passage 5-6. The cells are treated for 14 days with an adipogenic cocktail using a combination of human insulin and the PPARγ agonist-rosiglitazone. This methodology can be used for obtaining proof of concept experiments on molecular mechanisms that drive adipogenic responses in adipose endothelial cells, or for screening new drugs that can enhance the adipogenic response directed either towards white or beige/brown adipocyte differentiation. Using small subcutaneous biopsies, this methodology can be used to screen out non-responder subjects for clinical trials aimed to stimulate beige/brown and white adipocytes for the treatment of obesity and co-morbidities.

Published

2018

39. A High-throughput, High-content, Liquid-based C. elegans Pathosystem

Author

Quinton L, Anderson, Alexey V, Revtovich, and Natalia V, Kirienko

Subjects

Animals, Biological Assay, Caenorhabditis elegans, Immunology and Infection

Abstract

The number of new drugs identified by traditional, in vitro screens has waned, reducing the success of this approach in the search for new weapons to combat multiple drug resistance. This has led to the conclusion that researchers do not only need to find new drugs, but also need to develop new ways of finding them. Amongst the most promising candidate methods are whole-organism, in vivo assays that use high-throughput, phenotypic readouts and hosts that range from Caenorhabditis elegans to Danio rerio. These hosts have several powerful advantages, including dramatic reductions in false positive hits, as compounds that are toxic to the host and/or biounavailable are typically dropped in the initial screen, prior to costly follow up. Here we show how our assay has been used to interrogate host variation in the well-documented C. elegans—Pseudomonas aeruginosa liquid killing pathosystem. We also demonstrate several extensions of this well-worked out technique. For example, we are able to carry out high-throughput genetic screens using RNAi in 24- or 96-well plate formats to query host factors in this host-pathogen interaction. Using this assay, whole genome screens can be completed in only a few months, which can dramatically simplify the task of identifying drug targets, potentially without the need for laborious biochemical purification approaches. We also report here a variation of our method that substitutes the gram-positive bacterium Enterococcus faecalis for the gram-negative pathogen P. aeruginosa. Much as is the case for P. aeruginosa, killing by E. faecalis is time-dependent. Unlike previous C. elegans—E. faecalis assays, our assay for E. faecalis does not require preinfection, improving its safety profile and reducing the chances of contaminating liquid-handling equipment. The assay is highly robust, showing ~95% death rates 96 h post infection.

Published

2018

40. Long-term In Vivo Tracking of Inflammatory Cell Dynamics Within Drosophila Pupae

Author

Helen, Weavers, Anna, Franz, Will, Wood, and Paul, Martin

Subjects

Inflammation, Microscopy, Confocal, hemocyte, cell migration, Pupa, Wound healing, confocal microscopy, Drosophila pupa, Drosophila melanogaster, Issue 136, photoconversion, live-imaging, laser ablation, Animals, Drosophila, innate immunity, Immunology and Infection

Abstract

During the rapid inflammatory response to tissue damage, cells of the innate immune system are quickly recruited to the injury site. Once at the wound, innate immune cells perform a number of essential functions, such as fighting infection, clearing necrotic debris, and stimulating matrix deposition. In order to fully understand the diverse signaling events that regulate this immune response, it is crucial to observe the complex behaviors of (and interactions that occur between) multiple cell lineages in vivo, and in real-time, with the high spatio-temporal resolution. The optical translucency and the genetic tractability of Drosophila embryos have established Drosophila as an invaluable model to live-image and dissect fundamental aspects of inflammatory cell behavior, including mechanisms of developmental dispersal, clearance of apoptotic corpses and/or microbial pathogens, and recruitment to wounds. However, more recent work has now demonstrated that employing a much later stage in the Drosophila lifecycle – the Drosophila pupa – offers a number of distinct advantages, including improved RNAi efficiency, longer imaging periods, and significantly greater immune cell numbers. Here we describe a protocol for imaging wound repair and the associated inflammatory response at the high spatio-temporal resolution in live Drosophila pupae. To follow the dynamics of both re-epithelialization and inflammation, we use a number of specific in vivo fluorescent markers for both the epithelium and innate immune cells. We also demonstrate the effectiveness of photo-convertible fluorophores, such as Kaede, for following the specific immune cell subsets, to track their behavior as they migrate to, and resolve from, the injury site.

Published

2018

41. Isolation of Peritoneum-derived Mast Cells and Their Functional Characterization with Ca(2+)-imaging and Degranulation Assays

Author

Tsvilovskyy, Volodymyr, Solis-Lopez, Alejandra, Öhlenschläger, Kathrin, and Freichel, Marc

Subjects

Mice, Animals, Mast Cells, Peritoneum, humanities, Immunology and Infection

Abstract

Mast cells (MCs), as a part of the immune system, play a key role in defending the host against several pathogens and in the initiation of the allergic immune response. The activation of MCs via the cross-linking of surface IgE bound to high affinity IgE receptor (FcεRI), as well as through the stimulation of several other receptors, initiates the rise of the free intracellular Ca(2+) level ([Ca(2+)](i)) that promotes the release of inflammatory and allergic mediators. The identification of molecular constituents involved in these signaling pathways is crucial for understanding the regulation of MC function. In this article, we describe a protocol for the isolation of murine connective tissue type MCs by peritoneal lavage and cultivation of peritoneal MCs (PMCs). Cultures of MCs from various knockout mouse models by this methodology represent a useful approach to the identification of proteins involved in MC signaling pathways. In addition, we also describe a protocol for single cell Fura-2 imaging as an important technique for the quantification of Ca(2+) signaling in MCs. Fluorescence-based monitoring of [Ca(2+)](i) is a reliable and commonly used approach to study Ca(2+) signaling events, including store-operated calcium entry, which is of utmost importance for MC activation. For the analysis of MC degranulation, we describe a β-hexosaminidase release assay. The amount of β-hexosaminidase released into the culture medium is considered as a degranulation marker for all three different secretory subsets described in MCs. β-hexosaminidase can easily be quantified by its reaction with a colorigenic substrate in a microtiter plate colorimetric assay. This highly reproducible technique is cost-effective and requires no specialized equipment. Overall, the provided protocol demonstrates a high yield of MCs expressing typical MC surface markers, displaying typical morphological and phenotypic features of MCs, and demonstrating highly reproducible responses to secretagogues in Ca(2+)-imaging and degranulation assays.

Published

2018

42. A Murine Pancreatic Islet Cell-based Screening for Diabetogenic Environmental Chemicals

Author

Shaodong Guo, Jing Wu, Andrei Golovko, Yuxiang Sun, Nengtai Ouyang, Jingshu Chen, Lei Zhong, Yanan Tian, Benjamin Morpurgo, and Sui Ke

Subjects

0301 basic medicine, endocrine system, General Chemical Engineering, Cell, medicine.disease_cause, General Biochemistry, Genetics and Molecular Biology, Xenobiotics, Mice, 03 medical and health sciences, chemistry.chemical_compound, Dichlorofluorescein, Insulin-Secreting Cells, medicine, Animals, Humans, Cell damage, Immunology and Infection, chemistry.chemical_classification, Reactive oxygen species, General Immunology and Microbiology, General Neuroscience, Pancreatic islets, Environmental Exposure, medicine.disease, Cell biology, Mice, Inbred C57BL, 030104 developmental biology, medicine.anatomical_structure, Diabetes Mellitus, Type 2, chemistry, Cell culture, Toxicity, Environmental Pollutants, Reactive Oxygen Species, Oxidative stress

Abstract

Exposure to certain environmental chemicals in human and animals has been found to cause cellular damage of the pancreatic β cells which will lead to the development of type 2 diabetes mellitus (T2DM). Although the mechanisms for the chemical-induced β cell damage were unclear and likely to be complex, one recurring finding is that these chemicals induce oxidative stress leading to the generation of excessive reactive oxygen species (ROS) which induce damage to the β cell. To identify potential diabetogenic environmental chemicals, we isolated pancreatic islet cells from C57BL/6 mice and cultured islet cells in 96-well cell culture plates; then, the islet cells were dosed with chemicals and the ROS generation was detected by 2',7'-dichlorofluorescein (DCFH-DA) fluorescent dye. Using this method, we found that bisphenol A (BPA), Benzo[a]pyrene (BaP), and polychlorinated biphenyls (PCBs), could induce high levels of ROS, suggesting that they may potentially induce damage in islet cells. This method should be useful for screening diabetogenic xenobiotics. In addition, the cultured islet cells may also be adapted for in vitro analysis of chemical-induced toxicity in pancreatic cells.

Published

2018

43. Long-term In Vivo Tracking of Inflammatory Cell Dynamics Within Drosophila Pupae

Author

Weavers, Helen, Franz, Anna, Wood, Will, and Martin, Paul

Subjects

Inflammation, Innate immunity, Live-imaging, Pupa/pathogenicity, Microscopy, Confocal, Photoconversion, Drosophila/physiology, Wound healing, Hemocyte, Inflammation/immunology, Laser ablation, Drosophila pupa, Confocal microscopy, Drosophila melanogaster, Issue 136, Animals, Cell migration, Immunology and Infection

Abstract

During the rapid inflammatory response to tissue damage, cells of the innate immune system are quickly recruited to the injury site. Once at the wound, innate immune cells perform a number of essential functions, such as fighting infection, clearing necrotic debris, and stimulating matrix deposition. In order to fully understand the diverse signaling events that regulate this immune response, it is crucial to observe the complex behaviors of (and interactions that occur between) multiple cell lineages in vivo, and in real-time, with the high spatio-temporal resolution. The optical translucency and the genetic tractability of Drosophila embryos have established Drosophila as an invaluable model to live-image and dissect fundamental aspects of inflammatory cell behavior, including mechanisms of developmental dispersal, clearance of apoptotic corpses and/or microbial pathogens, and recruitment to wounds. However, more recent work has now demonstrated that employing a much later stage in the Drosophila lifecycle – the Drosophila pupa – offers a number of distinct advantages, including improved RNAi efficiency, longer imaging periods, and significantly greater immune cell numbers. Here we describe a protocol for imaging wound repair and the associated inflammatory response at the high spatio-temporal resolution in live Drosophila pupae. To follow the dynamics of both re-epithelialization and inflammation, we use a number of specific in vivo fluorescent markers for both the epithelium and innate immune cells. We also demonstrate the effectiveness of photo-convertible fluorophores, such as Kaede, for following the specific immune cell subsets, to track their behavior as they migrate to, and resolve from, the injury site.

Published

2018

44. Light-sheet Microscopy for Three-dimensional Visualization of Human Immune Cells

Author

Markus Hoth, Rouven Schoppmeyer, Bin Qu, and Renping Zhao

Subjects

0301 basic medicine, Microscopy, General Immunology and Microbiology, Chemistry, General Chemical Engineering, General Neuroscience, Cell migration, Antigen-Antibody Complex, General Biochemistry, Genetics and Molecular Biology, Extracellular matrix, 03 medical and health sciences, 030104 developmental biology, Immune system, Imaging, Three-Dimensional, In vivo, Live cell imaging, Light sheet fluorescence microscopy, Biophysics, Cytotoxic T cell, Animals, Humans, Immunology and Infection

Abstract

In vivo, activation, proliferation, and function of immune cells all occur in a three-dimensional (3D) environment, for instance in lymph nodes or tissues. Up to date, most in vitro systems rely on two-dimensional (2D) surfaces, such as cell-culture plates or coverslips. To optimally mimic physiological conditions in vitro, we utilize a simple 3D collagen matrix. Collagen is one of the major components of extracellular matrix (ECM) and has been widely used to constitute 3D matrices. For 3D imaging, the recently developed light-sheet microscopy technology (also referred to as single plane illumination microscopy) is featured with high acquisition speed, large penetration depth, low bleaching, and photocytotoxicity. Furthermore, light-sheet microscopy is particularly advantageous for long-term measurement. Here we describe an optimized protocol how to set up and handle human immune cells, e.g. primary human cytotoxic T lymphocytes (CTL) and natural killer (NK) cells in the 3D collagen matrix for usage with the light-sheet microscopy for live cell imaging and fixed samples. The procedure for image acquisition and analysis of cell migration are presented. A particular focus is given to highlight critical steps and factors for sample preparation and data analysis. This protocol can be employed for other types of suspension cells in a 3D collagen matrix and is not limited to immune cells.

Published

2018

45. Using Terminal Transferase-mediated dUTP Nick End-labelling (TUNEL) and Caspase 3/7 Assays to Measure Epidermal Cell Death in Frogs with Chytridiomycosis

Author

Lee F. Skerratt, Alexandra A. Roberts, Laura A. Brannelly, and Lee Berger

Subjects

0301 basic medicine, Programmed cell death, General Chemical Engineering, Caspase 3, Apoptosis, Caspase 7, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Transferases, In Situ Nick-End Labeling, Animals, Caspase, Immunology and Infection, TUNEL assay, biology, General Immunology and Microbiology, Cell Death, General Neuroscience, Epithelial Cells, Molecular biology, 030104 developmental biology, Terminal deoxynucleotidyl transferase, biology.protein, Anura, Epidermis

Abstract

Amphibians are experiencing a great loss in biodiversity globally and one of the major causes is the infectious disease chytridiomycosis. This disease is caused by the fungal pathogen Batrachochytrium dendrobatidis (Bd), which infects and disrupts frog epidermis; however, pathological changes have not been explicitly characterized. Apoptosis (programmed cell death) can be used by pathogens to damage host tissue, but can also be a host mechanism of disease resistance for pathogen removal. In this study, we quantify epidermal cell death of infected and uninfected animals using two different assays: terminal transferase-mediated dUTP nick end-labelling (TUNEL), and caspase 3/7. Using ventral, dorsal, and thigh skin tissue in the TUNEL assay, we observe cell death in the epidermal cells in situ of clinically infected animals and compare cell death with uninfected animals using fluorescent microscopy. In order to determine how apoptosis levels in the epidermis change over the course of infection we remove toe-tip samples fortnightly over an 8-week period, and use a caspase 3/7 assay with extracted proteins to quantify activity within the samples. We then correlate caspase 3/7 activity with infection load. The TUNEL assay is useful for localization of cell death in situ, but is expensive and time intensive per sample. The caspase 3/7 assay is efficient for large sample sizes and time course experiments. However, because frog toe tip biopsies are small there is limited extract available for sample standardization via protein quantification methods, such as the Bradford assay. Therefore, we suggest estimating skin surface area through photographic analysis of toe biopsies to avoid consuming extracts during sample standardization.

Published

2018

46. Assessment of the Cytotoxic and Immunomodulatory Effects of Substances in Human Precision-cut Lung Slices

Author

Sebastian Konzok, Susann Dehmel, Gregor Warnecke, Hans-Gerd Fieguth, Danny Jonigk, Helena Obernolte, Katherina Sewald, Olga Danov, Peter Braubach, Vanessa Neuhaus, Patrick Zardo, Christian Martin, Armin Braun, and Publica

Subjects

0301 basic medicine, chemical, General Chemical Engineering, Human explant culture, Alpha (ethology), chemicals, Inflammation, Bioinformatics, immunomodulation, confocal microscopy, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Issue 135, medicine, Animals, Humans, biopsy, Lung, Immunology and Infection, organotypic tissue, Microscopy, Confocal, General Immunology and Microbiology, business.industry, General Neuroscience, Interleukin, Cytotoxicity Tests, Immunologic, 030104 developmental biology, medicine.anatomical_structure, lung material, ex vivo, cytotoxicity, Tumor necrosis factor alpha, Animal studies, medicine.symptom, precision-cut lung slices, Risk assessment, business, Ex vivo

Abstract

Respiratory diseases in their broad diversity need appropriate model systems to understand the underlying mechanisms and enable development of new therapeutics. Additionally, registration of new substances requires appropriate risk assessment with adequate testing systems to avoid the risk of individuals being harmed, for example, in the working environment. Such risk assessments are usually conducted in animal studies. In view of the 3Rs principle and public skepticism against animal experiments, human alternative methods, such as precision-cut lung slices (PCLS), have been evolving. The present paper describes the ex vivo technique of human PCLS to study the immunomodulatory potential of low-molecular-weight substances, such as ammonium hexachloroplatinate (HClPt). Measured endpoints include viability and local respiratory inflammation, marked by altered secretion of cytokines and chemokines. Pro-inflammatory cytokines, tumor necrosis factor alpha (TNF-alpha), and interleukin 1 alpha (IL-1alpha) were significantly increased in human PCLS after exposure to a sub-toxic concentration of HClPt. Even though the technique of PCLS has been substantially optimized over the past decades, its applicability for the testing of immunomodulation is still in development. Therefore, the results presented here are preliminary, even though they show the potential of human PCLS as a valuable tool in respiratory research.

Published

2018

47. Imaging Ca(2+) Responses During Shigella Infection of Epithelial Cells

Author

Smail, Yasmine, Sun, Chunhui, Combettes, Laurent, and Tran Van Nhieu, Guy

Subjects

Animals, Humans, Calcium, Epithelial Cells, Immunology and Infection, Dysentery, Bacillary

Abstract

Ca(2+) is a ubiquitous ion involved in all known cellular processes. While global Ca(2+) responses may affect cell fate, local variations in free Ca(2+) cytosolic concentrations, linked to release from internal stores or an influx through plasma membrane channels, regulate cortical cell processes. Pathogens that adhere to or invade host cells trigger a reorganization of the actin cytoskeleton underlying the host plasma membrane, which likely affects both global and local Ca(2+) signaling. Because these events may occur at low frequencies in a pseudo-stochastic manner over extended kinetics, the analysis of Ca(2+) signals induced by pathogens raises major technical challenges that need to be addressed. Here, we report protocols for the detection of global and local Ca(2+) signals upon a Shigella infection of epithelial cells. In these protocols, artefacts linked to a prolonged exposure and photodamage associated with the excitation of Ca(2+) fluorescent probes are troubleshot by stringently controlling the acquisition parameters over defined time periods during a Shigella invasion. Procedures are implemented to rigorously analyze the amplitude and frequency of global cytosolic Ca(2+) signals during extended infection kinetics using the chemical probe Fluo-4.

Published

2018

48. Isolation and Characterization of Extracellular Vesicles from Adult Schistosoma japonicum

Author

Liu, Juntao, Zhu, Lihui, Wang, Lihui, Chen, Yongjun, Giri, Bikash Ranjan, Li, Jianjun, and Cheng, Guofeng

Subjects

Extracellular Vesicles, Animals, Schistosoma japonicum, Immunology and Infection

Abstract

Extracellular vesicles (EVs) are membranous vesicles released by a variety of cells into the extracellular microenvironment. EVs represent a population of heterogeneous vesicles, whose size range between 40 and 1,000 nm. Accumulated evidence indicated that EVs play important regulatory roles in pathogen-host interactions. A deep understanding of schistosome EVs should provide insights into the mechanisms underlying schistosome-host interactions, enabling development of novel strategies against schistosomiasis. Here, we aim to further study EVs functions in schistosomes by presenting a protocol for the isolation and characterization of EVs from adult Schistosoma japonicum (S. japonicum). EVs were isolated from in vitro culture medium using centrifugation combined with a commercial exosome isolation kit. The isolated S. japonicum EVs (SjEVs) typically possess a diameter of 100 - 400 nm, and are characterized by transmission electronic microscopy and western blotting. The usage of PKH67 dye-labeled SjEVs has demonstrated that SjEVs are internalized by the recipient cells. Overall, our protocol provides an alternative method for isolating EVs from adult schistosomes; the isolated SjEVs may be suitable for functional analysis.

Published

2018

49. Replication of the Ordered, Nonredundant Library of Pseudomonas aeruginosa strain PA14 Transposon Insertion Mutants

Author

Eliana, Drenkard, Rhianna M, Hibbler, D Alina, Gutu, Alexander D, Eaton, Amy L, Silverio, Frederick M, Ausubel, Bryan P, Hurley, and Lael M, Yonker

Subjects

Mutagenesis, Insertional, Mutagenesis, Pseudomonas aeruginosa, DNA Transposable Elements, Animals, Humans, Immunology and Infection

Abstract

Pseudomonas aeruginosa is a phenotypically and genotypically diverse and adaptable Gram-negative bacterium ubiquitous in human environments. P. aeruginosa is able to form biofilms, develop antibiotic resistance, produce virulence factors, and rapidly evolve in the course of a chronic infection. Thus P. aeruginosa can cause both acute and chronic, difficult to treat infections, resulting in significant morbidity in certain patient populations. P. aeruginosa strain PA14 is a human clinical isolate with a conserved genome structure that infects a variety of mammalian and nonvertebrate hosts making PA14 an attractive strain for studying this pathogen. In 2006, a nonredundant transposon insertion mutant library containing 5,459 mutants corresponding to 4,596 predicted PA14 genes was generated. Since then, distribution of the PA14 library has allowed the research community to better understand the function of individual genes and complex pathways of P. aeruginosa. Maintenance of library integrity through the replication process requires proper handling and precise techniques. To that end, this manuscript presents protocols that describe in detail the steps involved in library replication, library quality control and proper storage of individual mutants.

Published

2018

50. Collection and Processing of Lymph Nodes from Large Animals for RNA Analysis: Preparing for Lymph Node Transcriptomic Studies of Large Animal Species

Author

Catherine E. Vrentas, Robert G. Schaut, Paola M. Boggiatto, and Steven C. Olsen

Subjects

0301 basic medicine, General Chemical Engineering, Context (language use), Animals, Wild, Brucella, Computational biology, General Biochemistry, Genetics and Molecular Biology, Bison bison, Transcriptome, 03 medical and health sciences, Gene expression, medicine, symbols.heraldic_charge, Animals, Lymph node, Immunology and Infection, biology, Bison, General Immunology and Microbiology, General Neuroscience, RNA, biology.organism_classification, 030104 developmental biology, medicine.anatomical_structure, symbols, Cattle, Lymph, Lymph Nodes

Abstract

Large animals (both livestock and wildlife) serve as important reservoirs of zoonotic pathogens, including Brucella, Mycobacterium bovis, Salmonella, and E. coli, and are useful for the study of pathogenesis and/or spread of the bacteria in natural hosts. With the key function of lymph nodes in the host immune response, lymph node tissues serve as a potential source of RNA for downstream transcriptomic analyses, in order to assess the temporal changes in gene expression in cells over the course of an infection. This article presents an overview of the process of lymph node collection, tissue sampling, and downstream RNA processing in livestock, using cattle (Bos taurus) as a model, with additional examples provided from the American bison (Bison bison). The protocol includes information about the location, identification, and removal of lymph nodes from multiple key sites in the body. Additionally, a biopsy sampling methodology is presented that allows for a consistency of sampling across multiple animals. Several considerations for sample preservation are discussed, including the generation of RNA suitable for downstream methodologies like RNA-sequencing and RT-PCR. Due to the long delays inherent in large animal vs. mouse time course studies, representative results from bison and bovine lymph node tissues are presented to describe the time course of the degradation in this tissue type, in the context of a review of previous methodological work on RNA degradation in other tissues. Overall, this protocol will be useful to both veterinary researchers beginning transcriptome projects on large animal samples and to molecular biologists interested in learning techniques for in vivo tissue sampling and in vitro processing.

Published

2018