Your search keyword '"Ignacio S Caballero"' showing total 20 results

1. Heterogeneity in Human Induced Pluripotent Stem Cell-derived Alveolar Epithelial Type II Cells Revealed with ABCA3/SFTPC Reporters

Author

Krithi Gopalan, Jessie Huang, Darrell N. Kotton, Michael F. Beers, Carlos Villacorta-Martin, Killian Hurley, Yuliang L. Sun, Anne Hinds, Jeffrey A. Whitsett, Ignacio S. Caballero, Joseph A. Kitzmiller, and Scott J. Russo

Subjects

Pulmonary and Respiratory Medicine, Pulmonary Surfactant-Associated Proteins, Clinical Biochemistry, Induced Pluripotent Stem Cells, Biology, ABCA3, Pulmonary surfactant, Genome editing, medicine, Humans, Progenitor cell, Induced pluripotent stem cell, Molecular Biology, Lung, Editorials, Cell Differentiation, Epithelial Cells, Cell Biology, respiratory system, Pulmonary Surfactant-Associated Protein C, respiratory tract diseases, Cell biology, Pulmonary Alveoli, medicine.anatomical_structure, Alveolar Epithelial Cells, biology.protein, ATP-Binding Cassette Transporters

Abstract

Alveolar epithelial type 2 cells (AEC2s), the facultative progenitors of lung alveoli, are typically identified through the use of the canonical markers, SFTPC and ABCA3. Self-renewing AEC2-like cells have been generated from human induced pluripotent stem cells (iPSCs) through the use of knock-in SFTPC fluorochrome reporters. However, developmentally, SFTPC expression onset begins in the fetal distal lung bud tip and thus is not specific to mature AEC2s. Furthermore, SFTPC reporters appear to identify only those iPSC-derived AEC2s (iAEC2s) expressing the highest SFTPC levels. Here, we generate an ABCA3 knock-in GFP fusion reporter (ABCA3:GFP) that enables the purification of iAEC2s while allowing visualization of lamellar bodies, organelles associated with AEC2 maturation. Using an SFTPC

Published

2021

2. Where Is the Cystic Fibrosis Transmembrane Conductance Regulator?

Author

Ignacio S. Caballero, Brice Marcet, Pascal Barbry, Institut de pharmacologie moléculaire et cellulaire (IPMC), Centre National de la Recherche Scientifique (CNRS)-Université Nice Sophia Antipolis (... - 2019) (UNS), COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-Université Côte d'Azur (UCA), Infectiologie et Santé Publique (UMR ISP), Université de Tours-Institut National de Recherche pour l’Agriculture, l’Alimentation et l’Environnement (INRAE), Vaincre la Mucoviscidose (RF20180502280), Fondation pour la Recherche Médicale (DEQ20180339158), Chan Zuckerberg Initiative (Silicon Valley Foundation), Inserm (Human Developmental Cell Atlas program), ANR-19-CE14-0027,SAHARRA,Analyse par des approches de profilage à large échelle sur cellule unique de la régénération et du remodelage des voies respiratoires chez les patients asthmatiques(2019), ANR-19-P3IA-0002,3IA@cote d'azur,3IA Côte d'Azur(2019), European Project: 874656,discovAIR, Université Nice Sophia Antipolis (1965 - 2019) (UNS), COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-Centre National de la Recherche Scientifique (CNRS)-Université Côte d'Azur (UCA), and Université de Tours (UT)-Institut National de Recherche pour l’Agriculture, l’Alimentation et l’Environnement (INRAE)

Subjects

Pulmonary and Respiratory Medicine, congenital, hereditary, and neonatal diseases and abnormalities, Cystic Fibrosis, Cell Culture Techniques, Cystic Fibrosis Transmembrane Conductance Regulator, Respiratory Mucosa, [SDV.BC]Life Sciences [q-bio]/Cellular Biology, 030204 cardiovascular system & hematology, Critical Care and Intensive Care Medicine, [SDV.MHEP.PSR]Life Sciences [q-bio]/Human health and pathology/Pulmonology and respiratory tract, 03 medical and health sciences, 0302 clinical medicine, Medicine, Humans, ComputingMilieux_MISCELLANEOUS, 030304 developmental biology, 0303 health sciences, Ion Transport, biology, business.industry, Editorials, Epithelial Cells, Original Articles, respiratory system, Cystic fibrosis transmembrane conductance regulator, digestive system diseases, Cell biology, respiratory tract diseases, Case-Control Studies, biology.protein, business, Signal Transduction

Abstract

Rationale: Identification of the specific cell types expressing CFTR (cystic fibrosis [CF] transmembrane conductance regulator) is required for precision medicine therapies for CF. However, a full characterization of CFTR expression in normal human airway epithelia is missing. Objectives: To identify the cell types that contribute to CFTR expression and function within the proximal–distal axis of the normal human lung. Methods: Single-cell RNA (scRNA) sequencing (scRNA-seq) was performed on freshly isolated human large and small airway epithelial cells. scRNA in situ hybridization (ISH) and single-cell qRT-PCR were performed for validation. In vitro culture systems correlated CFTR function with cell types. Lentiviruses were used for cell type–specific transduction of wild-type CFTR in CF cells. Measurements and Main Results: scRNA-seq identified secretory cells as dominating CFTR expression in normal human large and, particularly, small airway superficial epithelia, followed by basal cells. Ionocytes expressed the highest CFTR levels but were rare, whereas the expression in ciliated cells was infrequent and low. scRNA ISH and single-cell qRT-PCR confirmed the scRNA-seq findings. CF lungs exhibited distributions of CFTR and ionocytes similar to those of normal control subjects. CFTR mediated Cl(−) secretion in cultures tracked secretory cell, but not ionocyte, densities. Furthermore, the nucleotide–purinergic regulatory system that controls CFTR-mediated hydration was associated with secretory cells and not with ionocytes. Lentiviral transduction of wild-type CFTR produced CFTR-mediated Cl(−) secretion in CF airway secretory cells but not in ciliated cells. Conclusions: Secretory cells dominate CFTR expression and function in human airway superficial epithelia. CFTR therapies may need to restore CFTR function to multiple cell types, with a focus on secretory cells.

Published

2021

3. Single-Cell Transcriptomic Profiling of Pluripotent Stem Cell-Derived SCGB3A2+ Airway Epithelium

Author

Seunghyi Kook, Edward E. Morrisey, Anjali Jacob, Konstantinos-Dionysios Alysandratos, Susan H. Guttentag, Michael Morley, Wenli Yang, Marall Vedaie, Barry R. Stripp, Darrell N. Kotton, Ignacio S. Caballero, Katherine B. McCauley, Gianni Carraro, Finn Hawkins, and Katherine J. Slovik

Subjects

0301 basic medicine, Time Factors, Cell Plasticity, Cell, Endogeny, Regenerative Medicine, Biochemistry, Epithelium, Transcriptome, Mice, Genes, Reporter, Induced pluripotent stem cell, Lung, Wnt Signaling Pathway, lcsh:QH301-705.5, lcsh:R5-920, Wnt signaling pathway, Cell Differentiation, respiratory system, 3. Good health, Cell biology, medicine.anatomical_structure, Respiratory, Single-Cell Analysis, pluripotent stem cells, lcsh:Medicine (General), Sequence Analysis, Induced Pluripotent Stem Cells, Clinical Sciences, Biology, Secretoglobins, Article, single-cell RNA sequencing, Cell Line, lung epithelium, 03 medical and health sciences, Directed differentiation, Spheroids, Cellular, Genetics, medicine, Animals, Humans, Cell Lineage, Stem Cell Research - Embryonic - Human, Reporter, alveoli, Stem Cell Research - Induced Pluripotent Stem Cell, Sequence Analysis, RNA, Gene Expression Profiling, directed differentiation, Cell Biology, Stem Cell Research, respiratory tract diseases, Kinetics, 030104 developmental biology, Genes, Solubility, lcsh:Biology (General), airway, RNA, Respiratory epithelium, Cellular, Biochemistry and Cell Biology, Spheroids, Developmental Biology

Abstract

Summary Lung epithelial lineages have been difficult to maintain in pure form in vitro, and lineage-specific reporters have proven invaluable for monitoring their emergence from cultured pluripotent stem cells (PSCs). However, reporter constructs for tracking proximal airway lineages generated from PSCs have not been previously available, limiting the characterization of these cells. Here, we engineer mouse and human PSC lines carrying airway secretory lineage reporters that facilitate the tracking, purification, and profiling of this lung subtype. Through bulk and single-cell-based global transcriptomic profiling, we find PSC-derived airway secretory cells are susceptible to phenotypic plasticity exemplified by the tendency to co-express both a proximal airway secretory program as well as an alveolar type 2 cell program, which can be minimized by inhibiting endogenous Wnt signaling. Our results provide global profiles of engineered lung cell fates, a guide for improving their directed differentiation, and a human model of the developing airway., Graphical Abstract, Highlights • Reporter lines allow detailed profiling of pluripotent stem cell-derived airway • PSC-derived airway spheres contain basal and secretory cells as well as non-lung • Single-cell RNA-seq reveals heterogeneity and potential plasticity, In this article, Kotton and colleagues show that human pluripotent stem cell-derived airway epithelial spheres contain basal and secretory airway cells. Using reporter lines for the secretory airway lineage alongside transcriptomic and functional analyses, they demonstrate that these cells have characteristic features of this population but are susceptible to Wnt-dependent phenotypic drift toward an alveolar type II cell-like program.

Published

2018

4. Single-cell time-series mapping of cell fate trajectories reveals an expanded developmental potential for human PSC-derived distal lung progenitors

Author

Jun Ding, Darrell N. Kotton, Aditya Mithal, Carlos Villacorta-Martin, Yuliang L. Sun, Ziv Bar-Joseph, Andrew A. Wilson, Michael J. Herriges, Ignacio S. Caballero, Marall Vedaie, Rhiannon B. Werder, Gustavo Mostoslavsky, Killian Hurley, Alejo E. Rodriguez-Fraticelli, Susan H. Guttentag, Fernando D. Camargo, Farida Ahangari, Konstantinos D. Alysandratos, Naftali Kaminski, Chieh Lin, and Anjali Jacob

Subjects

0303 health sciences, Regeneration (biology), Wnt signaling pathway, Biology, Cell fate determination, Phenotype, Cell biology, Transcriptome, 03 medical and health sciences, 0302 clinical medicine, Directed differentiation, Progenitor cell, Induced pluripotent stem cell, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

Alveolar epithelial type 2 cells (AEC2s) are the facultative progenitors responsible for maintaining lung alveoli throughout life, yet are difficult to access from patients for biomedical research or lung regeneration applications. Here we engineer AEC2s from human induced pluripotent stem cells (iPSCs) in vitro and use single cell RNA sequencing (scRNA-seq) to profile the detailed kinetics of their differentiation over time. We focus on both the desired target cells as well as those that appear to diverge to alternative endodermal fates. By combining scRNA-seq with lentiviral barcoding to trace differentiating clones, we reveal the bifurcating cell fate trajectories followed as primordial lung progenitors differentiate into mature AEC2s. We define the global transcriptomic signatures of primary developing human AEC2s from fetal through adult stages in order to identify the subset of in vitro differentiating cells that appear to recapitulate the path of in vivo development. In addition, we develop computational methods based on Continuous State Hidden Markov Models (CSHMM) to identify the precise timing and type of signals, such as over-exuberant Wnt responses, that induce some early multipotent NKX2-1+ progenitors to lose lung fate as they clonally diverge into a variety of non-lung endodermal lineages. Finally, we find that this initial developmental plasticity is regulatable via Wnt modulation, and subsides over time, ultimately resulting in iPSC-derived AEC2s that exhibit a stable phenotype and nearly limitless self-renewal capacity in vitro. Our methods and computational approaches can be widely applied to study and control directed differentiation, producing an inexhaustible supply of mature lineages, exemplified here by the generation of AEC2s.

Published

2019

5. Reconstructed Single-Cell Fate Trajectories Define Lineage Plasticity Windows during Differentiation of Human PSC-Derived Distal Lung Progenitors

Author

Carlos Villacorta-Martin, Andrew A. Wilson, Marall Vedaie, Yuliang L. Sun, Killian Hurley, Ziv Bar-Joseph, Jun Ding, Ignacio S. Caballero, Darrell N. Kotton, Alejo E. Rodriguez-Fraticelli, Naftali Kaminski, Farida Ahangari, Anjali Jacob, Jessie Huang, Susan H. Guttentag, Konstantinos D. Alysandratos, Michael J. Herriges, Gustavo Mostoslavsky, Irene Oglesby, Chieh Lin, Rhiannon B. Werder, Fernando D. Camargo, and Aditya Mithal

Subjects

Pluripotent Stem Cells, Lineage (genetic), Biology, Cell fate determination, Article, 03 medical and health sciences, 0302 clinical medicine, Directed differentiation, Genetics, Humans, Progenitor cell, Induced pluripotent stem cell, Lung, 030304 developmental biology, 0303 health sciences, Wnt signaling pathway, Cell Differentiation, Cell Biology, respiratory system, Phenotype, Cell biology, Pulmonary Alveoli, Alveolar Epithelial Cells, Molecular Medicine, Developmental plasticity, 030217 neurology & neurosurgery

Abstract

Summary Alveolar epithelial type 2 cells (AEC2s) are the facultative progenitors responsible for maintaining lung alveoli throughout life but are difficult to isolate from patients. Here, we engineer AEC2s from human pluripotent stem cells (PSCs) in vitro and use time-series single-cell RNA sequencing with lentiviral barcoding to profile the kinetics of their differentiation in comparison to primary fetal and adult AEC2 benchmarks. We observe bifurcating cell-fate trajectories as primordial lung progenitors differentiate in vitro, with some progeny reaching their AEC2 fate target, while others diverge to alternative non-lung endodermal fates. We develop a Continuous State Hidden Markov model to identify the timing and type of signals, such as overexuberant Wnt responses, that induce some early multipotent NKX2-1+ progenitors to lose lung fate. Finally, we find that this initial developmental plasticity is regulatable and subsides over time, ultimately resulting in PSC-derived AEC2s that exhibit a stable phenotype and nearly limitless self-renewal capacity.

Published

2019

6. Novel dynamics of human mucociliary differentiation revealed by single-cell RNA sequencing of nasal epithelial cultures

Author

Marin Truchi, Sylvie Leroy, Marie-Jeanne Arguel, Agnès Paquet, Marie Deprez, Ignacio S. Caballero, Brice Marcet, Kevin Lebrigand, Amélie Cavard, Pascal Barbry, Charles-Hugo Marquette, Virginie Magnone, Laure-Emmanuelle Zaragosi, Sandra Ruiz García, COMUE Université Côte d'Azur (2015-2019) (COMUE UCA), Infectiologie et Santé Publique (UMR ISP), Institut National de la Recherche Agronomique (INRA)-Université de Tours, Service de Pneumologie, Centre Hospitalier Universitaire de Nice (CHU Nice)-Hôpital de l'Archet, Fondation pour la Recherche Medicale (DEQ20180339158), Labex Signalife (ANR-11-LABX-0028-01), Association Vaincre la Mucoviscidose (RF20180502280), Commissariat aux Grands Investissements (ANR-10-INBS-09-03, ANR-10-INBS-09-02), Chan Zuckerberg Initiative [(Silicon Valley Community Foundation) 2017-175159-5022], Canceropole PACA, Institut de pharmacologie moléculaire et cellulaire (IPMC), Université Nice Sophia Antipolis (... - 2019) (UNS), COMUE Université Côte d'Azur (2015 - 2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015 - 2019) (COMUE UCA)-Centre National de la Recherche Scientifique (CNRS)-Université Côte d'Azur (UCA), Centre National de la Recherche Scientifique (CNRS), Université Côte d'Azur (UCA), COMUE Université Côte d'Azur (2015 - 2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015 - 2019) (COMUE UCA)-Centre National de la Recherche Scientifique (CNRS), Physiological Genomics of the Eukaryotes, Hôpital Pasteur [Nice] (CHU), Université Côte d'Azur (UCA)-Université Côte d'Azur (UCA)-Centre National de la Recherche Scientifique (CNRS), UR Infectiologie animale et Santé publique (UR IASP), Institut National de la Recherche Agronomique (INRA), Institut National de la Recherche Agronomique (INRA)-Université de Tours (UT), Barbry, Pascal, and Zaragosi, Laure-Emmanuelle

Subjects

épithélium, Swine, Cell, Pneumologie et système respiratoire, Basal cells, [SDV.BC.BC]Life Sciences [q-bio]/Cellular Biology/Subcellular Processes [q-bio.SC], [SDV.MHEP.PSR]Life Sciences [q-bio]/Human health and pathology/Pulmonology and respiratory tract, Transcriptome, Mice, 0302 clinical medicine, Keratin, mucociliary differentiation, RNA-Seq, tractus respiratoire, [SDV.BDD]Life Sciences [q-bio]/Development Biology, immunohistologie, Cells, Cultured, cell trajectory, Goblet cells, chemistry.chemical_classification, 0303 health sciences, Biologie du développement, Wnt signaling pathway, Cell Differentiation, scRNAseq, Development Biology, [SDV.BIBS]Life Sciences [q-bio]/Quantitative Methods [q-bio.QM], 3. Good health, Cell biology, Trachea, medicine.anatomical_structure, Deuterosome, Differentiation, cellule isolée, Keratins, single cell RNA seq, Airway epithelium, Club cells, Multiciliated cells, Pathways, Single-cell RNA-seq, Respiratory Mucosa, Biology, 03 medical and health sciences, Techniques and Resources, [SDV.BBM.GTP]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Genomics [q-bio.GN], medicine, Animals, Humans, Pulmonology and respiratory tract, Molecular Biology, 030304 developmental biology, différenciation cellulaire, Regeneration (biology), Epithelial Cells, voie de signalisation, chemistry, Respiratory epithelium, 030217 neurology & neurosurgery, Function (biology), Developmental Biology

Abstract

The upper airway epithelium, which is mainly composed of multiciliated, goblet, club and basal cells, ensures proper mucociliary function and can regenerate in response to assaults. In chronic airway diseases, defective repair leads to tissue remodeling. Delineating key drivers of differentiation dynamics can help understand how normal or pathological regeneration occurs. Using single-cell transcriptomics and lineage inference, we have unraveled trajectories from basal to luminal cells, providing novel markers for specific populations. We report that: (1) a precursor subgroup of multiciliated cells, which we have entitled deuterosomal cells, is defined by specific markers, such as DEUP1, FOXN4, YPEL1, HES6 and CDC20B; (2) goblet cells can be precursors of multiciliated cells, thus explaining the presence of hybrid cells that co-express markers of goblet and multiciliated cells; and (3) a repertoire of molecules involved in the regeneration process, such as keratins or components of the Notch, Wnt or BMP/TGFβ pathways, can be identified. Confirmation of our results on fresh human and pig airway samples, and on mouse tracheal cells, extend and confirm our conclusions regarding the molecular and cellular choreography at work during mucociliary epithelial differentiation., Highlighted Article: Single-cell RNAseq data in fresh human airway epithelial tissues and air liquid cultures identifies novel cell populations and offers new insights into the molecular mechanisms occurring during mucociliary epithelium regeneration.

Published

2019

7. Single-cell RNA sequencing reveals novel cell differentiation dynamics during human airway epithelium regeneration

Author

Virginie Magnone, Ignacio S. Caballero, Agnès Paquet, Laure-Emmanuelle Zaragosi, Marie Deprez, Sylvie Leroy, Brice Marcet, Kevin Lebrigand, Sandra Ruiz García, Pascal Barbry, Amélie Cavard, Marie-Jeanne Arguel, and Charles-Hugo Marquette

Subjects

medicine.anatomical_structure, Cellular differentiation, Regeneration (biology), Cell, medicine, Wnt signaling pathway, Respiratory epithelium, respiratory system, Epithelium regeneration, Biology, Cell fate determination, Epithelium, Cell biology

Abstract

BackgroundIt is usually considered that the upper airway epithelium is composed of multiciliated, goblet, secretory and basal cells, which collectively constitute an efficient first line of defense against inhalation of noxious substances. Upon injury, regeneration of this epithelium through proliferation and differentiation can restore a proper mucociliary function. However, in chronic airway diseases, the injured epithelium frequently displays defective repair leading to tissue remodeling, characterized by a loss of multiciliated cells and mucus hyper-secretion. Delineating drivers of differentiation dynamics and cell fate in the human airway epithelium is important to preserve homeostasis.ResultsWe have used single cell transcriptomics to characterize the sequence of cellular and molecular processes taking place during human airway epithelium regeneration. We have characterized airway subpopulations with high resolution and lineage inference algorithms have unraveled cell trajectories from basal to luminal cells, providing markers for specific cell populations, such as deuterosomal cells, i.e. precursors of multiciliated cells. We report that goblet cells, like secretory cells, can act as precursors of multiciliated cells. Our study provides a repertoire of molecules involved in key steps of the regeneration process, either keratins or components of the Notch, Wnt or BMP/TGFβ signaling pathways. Our findings were confirmed in independent experiments performed on fresh human and pig airway samples, and on mouse tracheal epithelial cells.ConclusionsOur single-cell RNA-seq study provides novel insights about airway epithelium differentiation dynamics, clarifies cell trajectories between secretory, goblet and multiciliated cells, identifies novel cell subpopulations, and maps the activation and repression of key signaling pathways.

Published

2018

8. Pluripotent stem cell differentiation reveals distinct developmental pathways regulating lung- versus thyroid-lineage specification

Author

Konstantinos-Dionysios Alysandratos, Ignacio S. Caballero, Katherine B. McCauley, Jinyoung Choi, Anita A. Kurmann, Finn Hawkins, Anthony N. Hollenberg, John M. Shannon, Laertis Ikonomou, Maria Paola Serra, Marall Vedaie, Darrell N. Kotton, and Anjali Jacob

Subjects

Cell type, medicine.anatomical_structure, Somatic cell, Wnt signaling pathway, medicine, respiratory system, Biology, Endoderm, Progenitor cell, Fibroblast growth factor, Induced pluripotent stem cell, Progenitor, Cell biology

Abstract

The in vitro-directed differentiation of pluripotent stem cells (PSCs) through stimulation of developmental signaling pathways can generate mature somatic cell types for basic laboratory studies or regenerative therapies. However, there has been significant uncertainty regarding a method to separately derive lung versus thyroid epithelial lineages, as these two cell types each originate from Nkx2-1+ foregut progenitors and the minimal pathways claimed to regulate their distinct lineage specification in vivo or in vitro have varied in previous reports. Here, we employ PSCs to identify the key minimal signaling pathways (Wnt+BMP versus BMP+FGF) that regulate distinct lung- versus thyroid-lineage specification, respectively, from foregut endoderm. In contrast to most previous reports, these minimal pathways appear to be evolutionarily conserved between mice and humans, and FGF signaling, although required for thyroid specification, unexpectedly appears to be dispensable for lung specification. Once specified, distinct Nkx2-1+ lung or thyroid progenitor pools can now be independently derived for functional 3D culture maturation, basic developmental studies or future regenerative therapies.

Published

2018

9. Modeling APC mutagenesis and familial adenomatous polyposis using human iPS cells

Author

Gustavo Mostoslavsky, Ignacio S. Caballero, F.J. Molina-Estevez, Andreia Gianotti-Sommer, Nicholas Skvir, Cesar Sommer, Amalia Capilla, and Sanjib Chowdhury

Subjects

0301 basic medicine, Cellular differentiation, Gene Expression, lcsh:Medicine, medicine.disease_cause, Loss of heterozygosity, Animal Cells, Medicine and Health Sciences, Organ Cultures, Induced pluripotent stem cell, lcsh:Science, Cells, Cultured, Connective Tissue Cells, Staining, Mutation, Multidisciplinary, biology, Stem Cells, Gene Expression Regulation, Developmental, Cell Staining, Cell Differentiation, 3. Good health, Intestines, Organoids, Cell Transformation, Neoplastic, Adenomatous Polyposis Coli, Connective Tissue, Biological Cultures, Cellular Types, Anatomy, Signal Transduction, Research Article, Adenomatous polyposis coli, Immune Cells, Adenomatous Polyposis Coli Protein, Induced Pluripotent Stem Cells, Immunology, Antigen-Presenting Cells, Mutagenesis (molecular biology technique), Research and Analysis Methods, Familial adenomatous polyposis, 03 medical and health sciences, Genetics, medicine, Humans, lcsh:R, Biology and Life Sciences, Cell Biology, Fibroblasts, medicine.disease, Gastrointestinal Tract, HEK293 Cells, Biological Tissue, 030104 developmental biology, Mutagenesis, Specimen Preparation and Treatment, Cancer research, biology.protein, lcsh:Q, Carcinogenesis, Digestive System, Developmental Biology

Abstract

Mutations in the gene Adenomatous Polyposis Coli or APC appear in most sporadic cases of colorectal cancer and it is the most frequent mutation causing hereditary Familial Adenomatous Polyposis. The detailed molecular mechanism by which APC mutations predispose to the development of colorectal cancer is not completely understood. This is in part due to the lack of accessibility to appropriate models that recapitulate the early events associated with APC mediated intestinal transformation. We have established a novel platform utilizing human induced Pluripotent Stem cells or iPSC from normal or FAP-specific APC mutant individuals and evaluated the effect of the mutation in the cells before and after differentiation into intestinal organoids. In order to minimize genetic background effects, we also established an isogenic platform using TALEN-mediated gene editing. Comparison of normal and APC mutant iPSC revealed a significant defect in cell identity and polarity due to the presence of APC in heterozygosity as well as chromosomal aberrations including abnormal anaphases and centrosome numbers. Importantly, upon specification into intestinal progeny, APC heterozygosity was responsible for a major change in the transcriptional identity of the cells with dysregulation of key signaling pathways, including metabolic reprogramming, abnormal lipid metabolism and intestinal-specific cadherin expression. In conclusion, we have developed a novel iPSC/intestinal model of APC mutagenesis and provide strong evidence that APC in heterozygosity imparts a clear phenotypic and molecular defect, affecting basic cellular functions and integrity, providing novel insights in the earlier events of APC-mediated tumorigenesis.

Published

2018

10. Unraveling the genetic diversity and phylogeny of Leishmania RNA virus 1 strains of infected Leishmania isolates circulating in French Guiana

Author

Emilie Mosnier, Marine Ginouves, Vincent Vantilcke, Vincent Lacoste, Eliane Bourreau, Ignacio S. Caballero, Christiane Bouchier, Damien Donato, Sourakhata Tirera, Pierre Couppié, Anne Lavergne, Ghislaine Prévot, Institut Pasteur de la Guyane, Réseau International des Instituts Pasteur (RIIP), Ecosystemes Amazoniens et Pathologie Tropicale (EPat), Institut National de la Santé et de la Recherche Médicale (INSERM)-Université de Guyane (UG), Centre Hospitalier Andrée Rosemon [Cayenne, Guyane Française], Boston University [Boston] (BU), Génomique (Plate-Forme) - Genomics Platform, Institut Pasteur [Paris] (IP), Centre Hospitalier de l'Ouest Guyanais, Département de Virologie - Department of Virology, ANR-10-LABX-0025,CEBA,CEnter of the study of Biodiversity in Amazonia(2010), ANR-10-INBS-0009,France-Génomique,Organisation et montée en puissance d'une Infrastructure Nationale de Génomique(2010), European Project: 285837,EC:FP7:REGPOT,FP7-REGPOT-2011-1,STRONGER(2011), Lacoste, Vincent, Laboratoires d'excellence - CEnter of the study of Biodiversity in Amazonia - - CEBA2010 - ANR-10-LABX-0025 - LABX - VALID, Organisation et montée en puissance d'une Infrastructure Nationale de Génomique - - France-Génomique2010 - ANR-10-INBS-0009 - INBS - VALID, Strengthening transdisciplinary research on infectious and emerging diseases in French Guiana: linking fieldwork, benchside and bedside - STRONGER - - EC:FP7:REGPOT2011-11-01 - 2015-04-30 - 285837 - VALID, and Institut Pasteur [Paris]

Subjects

0301 basic medicine, Male, MESH: Leishmaniavirus, MESH: Sequence Analysis, DNA, MESH: Leishmaniasis, [SDV]Life Sciences [q-bio], 0302 clinical medicine, Medicine and Health Sciences, Cluster Analysis, MESH: Genetic Variation, MESH: Phylogeny, Leishmaniasis, Phylogeny, Data Management, Genetics, Protozoans, Leishmania, MESH: Aged, MESH: Middle Aged, Phylogenetic tree, lcsh:Public aspects of medicine, Database and informatics methods, Sequence analysis, Phylogenetic Analysis, Middle Aged, 3. Good health, French Guiana, Phylogenetics, [SDV] Life Sciences [q-bio], Infectious Diseases, [SDV.MP]Life Sciences [q-bio]/Microbiology and Parasitology, MESH: Young Adult, MESH: RNA, Viral, RNA, Viral, Female, MESH: Genome, Viral, Research Article, Adult, Computer and Information Sciences, lcsh:Arctic medicine. Tropical medicine, lcsh:RC955-962, Bioinformatics, MESH: Leishmania, 030231 tropical medicine, Leishmaniavirus, MESH: Sequence Alignment, Nucleotide Sequencing, Genome, Viral, Biology, [SDV.GEN.GH] Life Sciences [q-bio]/Genetics/Human genetics, 03 medical and health sciences, Young Adult, Cutaneous leishmaniasis, Sequence Motif Analysis, MESH: French Guiana, medicine, Parasitic Diseases, Humans, Evolutionary Systematics, Molecular Biology Techniques, Sequencing Techniques, Genotyping, Molecular Biology, [SDV.MP] Life Sciences [q-bio]/Microbiology and Parasitology, DNA sequence analysis, Taxonomy, Aged, Evolutionary Biology, MESH: Humans, Public Health, Environmental and Occupational Health, Organisms, Biology and Life Sciences, Genetic Variation, RNA virus, lcsh:RA1-1270, MESH: Adult, Sequence Analysis, DNA, medicine.disease, biology.organism_classification, MESH: Cluster Analysis, Parasitic Protozoans, MESH: Male, Research and analysis methods, 030104 developmental biology, [SDV.GEN.GH]Life Sciences [q-bio]/Genetics/Human genetics, Sequence Alignment, MESH: Female

Abstract

Introduction Leishmania RNA virus type 1 (LRV1) is an endosymbiont of some Leishmania (Vianna) species in South America. Presence of LRV1 in parasites exacerbates disease severity in animal models and humans, related to a disproportioned innate immune response, and is correlated with drug treatment failures in humans. Although the virus was identified decades ago, its genomic diversity has been overlooked until now. Methodology/Principles findings We subjected LRV1 strains from 19 L. (V.) guyanensis and one L. (V.) braziliensis isolates obtained from cutaneous leishmaniasis samples identified throughout French Guiana with next-generation sequencing and de novo sequence assembly. We generated and analyzed 24 unique LRV1 sequences over their full-length coding regions. Multiple alignment of these new sequences revealed variability (0.5%–23.5%) across the entire sequence except for highly conserved motifs within the 5’ untranslated region. Phylogenetic analyses showed that viral genomes of L. (V.) guyanensis grouped into five distinct clusters. They further showed a species-dependent clustering between viral genomes of L. (V.) guyanensis and L. (V.) braziliensis, confirming a long-term co-evolutionary history. Noteworthy, we identified cases of multiple LRV1 infections in three of the 20 Leishmania isolates. Conclusions/Significance Here, we present the first-ever estimate of LRV1 genomic diversity that exists in Leishmania (V.) guyanensis parasites. Genetic characterization and phylogenetic analyses of these viruses has shed light on their evolutionary relationships. To our knowledge, this study is also the first to report cases of multiple LRV1 infections in some parasites. Finally, this work has made it possible to develop molecular tools for adequate identification and genotyping of LRV1 strains for diagnostic purposes. Given the suspected worsening role of LRV1 infection in the pathogenesis of human leishmaniasis, these data have a major impact from a clinical viewpoint and for the management of Leishmania-infected patients., Author summary Leishmaniasis is a well-known parasitosis due to an infection by the protozoan Leishmania parasites firmly established in South America. In French Guiana, where leishmaniasis is a public health problem, having an annual incidence of 5.6 cases/10,000 inhabitants, 80% of Leishmania spp. parasites are infected by an endosymbiotic virus, Leishmania RNA virus 1 (LRV1). The purpose of this study was to gain insights on the genetic variability and evolution of LRV1 at the genomic level. We subjected 20 Leishmania isolates obtained from cutaneous lesions with next generation sequencing and de novo sequence assembly. This allowed generating 24 LRV1 full-length coding sequences presenting among themselves a significant genetic diversity. The inferred phylogenetic relationships enabled to identify distinct well-supported genotypes and support the hypothesis of co-evolution between LRV1 strains and their parasite hosts. In addition, we identified multiple LRV1 infections in three parasite isolates. Based on these data, future characterization of new strains from other geographic areas and other parasite species should extend knowledge of LRV1 diversification processes. Finally, these results allowed us to identify genomic regions where best to allocate resources for subsequent analyses of LRV1 viral diversity and genotyping that could serve for accurate routine molecular diagnostic applications.

Published

2017

11. Pluripotent stem cell differentiation reveals distinct developmental pathways regulating lung versus thyroid lineage specification

Author

Konstantinos-Dionysios Alysandratos, Marall Vedaie, Anthony N. Hollenberg, Anita A. Kurmann, Ignacio S. Caballero, Jinyoung Choi, Katherine B. McCauley, Finn Hawkins, John M. Shannon, Anjali Jacob, Maria Paola Serra, Darrell N. Kotton, and Laertis Ikonomou

Subjects

Pluripotent Stem Cells, 0301 basic medicine, Cell type, Somatic cell, Human Development, Green Fluorescent Proteins, Induced Pluripotent Stem Cells, Thyroid Gland, Embryonic Development, Biology, Fibroblast growth factor, Mice, 03 medical and health sciences, Spheroids, Cellular, medicine, Animals, Humans, Cell Lineage, Progenitor cell, Induced pluripotent stem cell, Lung, Molecular Biology, Body Patterning, Progenitor, Homeodomain Proteins, Gene Expression Profiling, Endoderm, Wnt signaling pathway, Gene Expression Regulation, Developmental, Reproducibility of Results, Cell Differentiation, Epithelial Cells, Mouse Embryonic Stem Cells, respiratory system, Embryo, Mammalian, Cell biology, Fibroblast Growth Factors, Wnt Proteins, 030104 developmental biology, medicine.anatomical_structure, Bone Morphogenetic Proteins, Immunology, Transcriptome, Biomarkers, Signal Transduction, Developmental Biology

Abstract

The in vitro-directed differentiation of pluripotent stem cells (PSCs) through stimulation of developmental signaling pathways can generate mature somatic cell types for basic laboratory studies or regenerative therapies. However, there has been significant uncertainty regarding a method to separately derive lung versus thyroid epithelial lineages, as these two cell types each originate from Nkx2-1+ foregut progenitors and the minimal pathways claimed to regulate their distinct lineage specification in vivo or in vitro have varied in previous reports. Here, we employ PSCs to identify the key minimal signaling pathways (Wnt+BMP versus BMP+FGF) that regulate distinct lung- versus thyroid-lineage specification, respectively, from foregut endoderm. In contrast to most previous reports, these minimal pathways appear to be evolutionarily conserved between mice and humans, and FGF signaling, although required for thyroid specification, unexpectedly appears to be dispensable for lung specification. Once specified, distinct Nkx2-1+ lung or thyroid progenitor pools can now be independently derived for functional 3D culture maturation, basic developmental studies or future regenerative therapies.

Published

2017

12. Generation of a Stable Transgenic Swine Model Expressing a Porcine Histone 2B-eGFP Fusion Protein for Cell Tracking and Chromosome Dynamics Studies

Author

Ignacio S. Caballero, Sean G Simpson, Robert M. Petters, Sehwon Koh, Bruce Collins, Renan Sper, Jeffrey R. Sommer, Xia Zhang, Jorge A. Piedrahita, Jeff L. Platt, Comparative Medicine Institute, North Carolina State University [Raleigh] (NC State), University of North Carolina System (UNC)-University of North Carolina System (UNC), Department of Molecular Biomedical Sciences, College of Veterinary Medicine, Department of Cell Biology, Charles University [Prague] (CU), Department of Surgery and Microbiology and Immunology, Department of Animal Science, College of Agriculture and Life Sciences, Infectiologie et Santé Publique (UMR ISP), Institut National de la Recherche Agronomique (INRA)-Université de Tours (UT), NIH [HL051587, R01HL051587], Charles University [Prague], Infectiologie Animale et Santé Publique - IASP (Nouzilly, France), Institut National de la Recherche Agronomique (INRA), and Institut National de la Recherche Agronomique (INRA)-Université de Tours

Subjects

Male, 0301 basic medicine, green fluorescent protein, Embryology, Swine, [SDV]Life Sciences [q-bio], lcsh:Medicine, Artificial Gene Amplification and Extension, Polymerase Chain Reaction, Green fluorescent protein, Transgenic Model, Cell Fusion, Histones, stem-cells, Fluorescence Microscopy, Pig Models, Animal Cells, lcsh:Science, spindle formation, Mammals, Microscopy, Multidisciplinary, Light Microscopy, wallerian degeneration, pigs, Agriculture, Animal Models, matrix-attachment regions, 3. Good health, Chromatin, Experimental Organism Systems, Cell Tracking, OVA, Vertebrates, Somatic cell nuclear transfer, Female, Cellular Types, living cells, Research Article, Cell Physiology, nuclear transfer, Livestock, mice, Imaging Techniques, Recombinant Fusion Proteins, Transgene, Green Fluorescent Proteins, Biology, Research and Analysis Methods, 03 medical and health sciences, embryos, Fluorescence Imaging, Animals, Molecular Biology Techniques, Scaffold/matrix attachment region, Molecular Biology, Organisms, Genetically Modified, lcsh:R, Organisms, Biology and Life Sciences, Cell Biology, Chromosomes, Mammalian, Fusion protein, Molecular biology, Transplantation, Germ Cells, 030104 developmental biology, Amniotes, Oocytes, lcsh:Q, Developmental Biology

Abstract

International audience; Transgenic pigs have become an attractive research model in the field of translational research, regenerative medicine, and stem cell therapy due to their anatomic, genetic and physiological similarities with humans. The development of fluorescent proteins as molecular tags has allowed investigators to track cell migration and engraftment levels after transplantation. Here we describe the development of two transgenic pig models via SCNT expressing a fusion protein composed of eGFP and porcine Histone 2B (pH2B). This fusion protein is targeted to the nucleosomes resulting a nuclear/chromatin eGFP signal. The first model (I) was generated via random insertion of pH2B-eGFP driven by the CAG promoter (chicken beta actin promoter and rabbit Globin poly A; pCAG-pH2B-eGFP) and protected by human interferon-beta matrix attachment regions (MARs). Despite the consistent, high, and ubiquitous expression of the fusion protein pH2B-eGFP in all tissues analyzed, two independently generated Model I transgenic lines developed neurodegenerative symptoms including Wallerian degeneration between 3-5 months of age, requiring euthanasia. A second transgenic model (II) was developed via CRISPR-Cas9 mediated homology-directed repair (HDR) of IRES-pH2B-eGFP into the endogenous beta-actin (ACTB) locus. Model II transgenic animals showed ubiquitous expression of pH2B-eGFP on all tissues analyzed. Unlike the pCAG-pH2B-eGFP/MAR line, all Model II animals were healthy and multiple pregnancies have been established with progeny showing the expected Mendelian ratio for the transmission of the pH2B-eGFP. Expression of pH2B-eGFP was used to examine the timing of the maternal to zygotic transition after IVF, and to examine chromosome segregation of SCNT embryos. To our knowledge this is the first viable transgenic pig model with chromatin-associated eGFP allowing both cell tracking and the study of chromatin dynamics in a large animal model.

Published

2017

13. Laquinimod arrests experimental autoimmune encephalomyelitis by activating the aryl hydrocarbon receptor

Author

Rina Kashi, Aric Orbach, Victor Piryatinsky, Daphna Laifenfeld, Mark A. Ator, Tal Birnberg, Doron Shinar, Tal Hingaly, Efrat Rubinstein, Emanuel Raymond, Einat Amit-Romach, Fadi Towfic, Ralph Laufer, Yael Marantz, Iris Grossman, Joel Kaye, Ignacio S. Caballero, Volker Knappertz, and Michael R. Hayden

Subjects

0301 basic medicine, Encephalomyelitis, Autoimmune, Experimental, T-Lymphocytes, Gene Expression, Quinolones, Biology, Myelin oligodendrocyte glycoprotein, Mice, 03 medical and health sciences, chemistry.chemical_compound, Immune system, Cytochrome P-450 CYP1A1, medicine, Animals, Humans, Neuroinflammation, Mice, Knockout, Multidisciplinary, Microglia, Gene Expression Profiling, Multiple sclerosis, Experimental autoimmune encephalomyelitis, respiratory system, medicine.disease, Aryl hydrocarbon receptor, 030104 developmental biology, medicine.anatomical_structure, PNAS Plus, Gene Expression Regulation, Receptors, Aryl Hydrocarbon, chemistry, Immune System, Immunology, Hepatocytes, biology.protein, Female, Transcriptome, Laquinimod, Gene Deletion

Abstract

Laquinimod is an oral drug currently being evaluated for the treatment of relapsing, remitting, and primary progressive multiple sclerosis and Huntington’s disease. Laquinimod exerts beneficial activities on both the peripheral immune system and the CNS with distinctive changes in CNS resident cell populations, especially astrocytes and microglia. Analysis of genome-wide expression data revealed activation of the aryl hydrocarbon receptor (AhR) pathway in laquinimod-treated mice. The AhR pathway modulates the differentiation and function of several cell populations, many of which play an important role in neuroinflammation. We therefore tested the consequences of AhR activation in myelin oligodendrocyte glycoprotein (MOG)-induced experimental autoimmune encephalomyelitis (EAE) using AhR knockout mice. We demonstrate that the pronounced effect of laquinimod on clinical score, CNS inflammation, and demyelination in EAE was abolished in AhR−/− mice. Furthermore, using bone marrow chimeras we show that deletion of AhR in the immune system fully abrogates, whereas deletion within the CNS partially abrogates the effect of laquinimod in EAE. These data strongly support the idea that AhR is necessary for the efficacy of laquinimod in EAE and that laquinimod may represent a first-in-class drug targeting AhR for the treatment of multiple sclerosis and other neurodegenerative diseases.

Published

2016

14. In vivo Ebola virus infection leads to a strong innate response in circulating immune cells

Author

Stephen K. Gire, Chiara Gerhardinger, Lisa E. Hensley, Sarah M. Winnicki, Pardis C. Sabeti, Marta Melé, Anna N. Honko, John L. Rinn, Ignacio S. Caballero, John H. Connor, and Aaron E. Lin

Subjects

0301 basic medicine, viruses, Biology, medicine.disease_cause, Virus Replication, Virus, Pathogenesis, 03 medical and health sciences, Ebola virus, Mice, Immune system, Transcriptional response, medicine, Genetics, Animals, Gene Regulatory Networks, Transcriptomics, Interferon-stimulated genes, Ebolavirus, Innate immune system, Sequence Analysis, RNA, Gene Expression Profiling, Hemorrhagic Fever, Ebola, Virology, ISG15, Immunity, Innate, 3. Good health, 030104 developmental biology, Viral replication, Gene Expression Regulation, Immunology, Leukocytes, Mononuclear, Macaca, Biotechnology, Research Article

Abstract

Background Ebola virus is the causative agent of a severe syndrome in humans with a fatality rate that can approach 90 %. During infection, the host immune response is thought to become dysregulated, but the mechanisms through which this happens are not entirely understood. In this study, we analyze RNA sequencing data to determine the host response to Ebola virus infection in circulating immune cells. Results Approximately half of the 100 genes with the strongest early increases in expression were interferon-stimulated genes, such as ISG15, OAS1, IFIT2, HERC5, MX1 and DHX58. Other highly upregulated genes included cytokines CXCL11, CCL7, IL2RA, IL2R1, IL15RA, and CSF2RB, which have not been previously reported to change during Ebola virus infection. Comparing this response in two different models of exposure (intramuscular and aerosol) revealed a similar signature of infection. The strong innate response in the aerosol model was seen not only in circulating cells, but also in primary and secondary target tissues. Conversely, the innate immune response of vaccinated macaques was almost non-existent. This suggests that the innate response is a major aspect of the cellular response to Ebola virus infection in multiple tissues. Conclusions Ebola virus causes a severe infection in humans that is associated with high mortality. The host immune response to virus infection is thought to be an important aspect leading to severe pathology, but the components of this overactive response are not well characterized. Here, we analyzed how circulating immune cells respond to the virus and found that there is a strong innate response dependent on active virus replication. This finding is in stark contrast to in vitro evidence showing a suppression of innate immune signaling, and it suggests that the strong innate response we observe in infected animals may be an important contributor to pathogenesis. Electronic supplementary material The online version of this article (doi:10.1186/s12864-016-3060-0) contains supplementary material, which is available to authorized users.

Published

2016

15. Transcriptional Profiling of the Immune Response to Marburg Virus Infection

Author

Lisa E. Hensley, Judy Y. Yen, John H. Connor, Kenny L. Lin, Ignacio S. Caballero, Sara Garamszegi, Shikha Malhotra, and Arthur J. Goff

Subjects

Immunology, Real-Time Polymerase Chain Reaction, Microbiology, Virus, Pathogenesis, Marburg virus, Immune system, Immunity, Marburg virus disease, Virology, Animals, Marburg Virus Disease, Innate immune system, biology, Gene Expression Profiling, Marburgvirus, biology.organism_classification, Microarray Analysis, Macaca mulatta, Immunity, Innate, Gene Expression Regulation, Insect Science, Leukocytes, Mononuclear, Cytokines, Pathogenesis and Immunity, Biomarkers

Abstract

Marburg virus is a genetically simple RNA virus that causes a severe hemorrhagic fever in humans and nonhuman primates. The mechanism of pathogenesis of the infection is not well understood, but it is well accepted that pathogenesis is appreciably driven by a hyperactive immune response. To better understand the overall response to Marburg virus challenge, we undertook a transcriptomic analysis of immune cells circulating in the blood following aerosol exposure of rhesus macaques to a lethal dose of Marburg virus. Using two-color microarrays, we analyzed the transcriptomes of peripheral blood mononuclear cells that were collected throughout the course of infection from 1 to 9 days postexposure, representing the full course of the infection. The response followed a 3-stage induction (early infection, 1 to 3 days postexposure; midinfection, 5 days postexposure; late infection, 7 to 9 days postexposure) that was led by a robust innate immune response. The host response to aerosolized Marburg virus was evident at 1 day postexposure. Analysis of cytokine transcripts that were overexpressed during infection indicated that previously unanalyzed cytokines are likely induced in response to exposure to Marburg virus and further suggested that the early immune response is skewed toward a Th2 response that would hamper the development of an effective antiviral immune response early in disease. Late infection events included the upregulation of coagulation-associated factors. These findings demonstrate very early host responses to Marburg virus infection and provide a rich data set for identification of factors expressed throughout the course of infection that can be investigated as markers of infection and targets for therapy. IMPORTANCE Marburg virus causes a severe infection that is associated with high mortality and hemorrhage. The disease is associated with an immune response that contributes to the lethality of the disease. In this study, we investigated how the immune cells circulating in the blood of infected primates respond following exposure to Marburg virus. Our results show that there are three discernible stages of response to infection that correlate with presymptomatic, early, and late symptomatic stages of infection, a response format similar to that seen following challenge with other hemorrhagic fever viruses. In contrast to the ability of the virus to block innate immune signaling in vitro , the earliest and most sustained response is an interferon-like response. Our analysis also identifies a number of cytokines that are transcriptionally upregulated during late stages of infection and suggest that there is a Th2-skewed response to infection. When correlated with companion data describing the animal model from which our samples were collected, our results suggest that the innate immune response may contribute to overall pathogenesis.

Published

2015

16. Computed Tomography (CT) Scanning Facilitates Early Identification of Neonatal Cystic Fibrosis Piglets

Author

Patricia Berthon, Reuben Ramphal, Joseph Moënne-Loccoz, Andrea Bähr, Pierre Sarradin, François Lecompte, Sylvie Attucci, Ignacio S. Caballero, Mustapha Si-Tahar, Thierry Villemagne, Rémi Delaunay, Nikolai Klymiuk, Mustapha Berri, Antoine Guillon, Céline Barc, Jérémy Pezant, Claire Chevaleyre, Dominique Buzoni-Gatel, Hans Adriaensen, Eckhard Wolf, Centre d’Etude des Pathologies Respiratoires (CEPR), UMR 1100 (CEPR), Université de Tours (UT)-Institut National de la Santé et de la Recherche Médicale (INSERM), Service de réanimation polyvalente, Groupe Hospitalier Paris Saint-Joseph, Infectiologie et Santé Publique (UMR ISP), Institut National de la Recherche Agronomique (INRA)-Université de Tours (UT), Plateforme d'Infectiologie Expérimentale (PFIE), Institut National de la Recherche Agronomique (INRA), Physiologie de la reproduction et des comportements [Nouzilly] (PRC), Institut National de la Recherche Agronomique (INRA)-Institut Français du Cheval et de l'Equitation [Saumur]-Université de Tours (UT)-Centre National de la Recherche Scientifique (CNRS), Plateforme CIRE, Centre Hospitalier Régional Universitaire de Tours (CHRU Tours), Service anesthésie-réanimation, Gene Center and Center for Innovative Medical Models (CIMM), Foundation Vaincre la Mucoviscidose RF20130500925, Region Centre 32000604, Université de Tours-Institut National de la Santé et de la Recherche Médicale (INSERM), Infectiologie Animale et Santé Publique - IASP (Nouzilly, France), Plateforme d'Infectiologie Expérimentale (PFIE - INRA UE 1277), Centre National de la Recherche Scientifique (CNRS)-Université de Tours-Institut Français du Cheval et de l'Equitation [Saumur]-Institut National de la Recherche Agronomique (INRA), Centre Hospitalier Régional Universitaire de Tours (CHRU TOURS), Institut National de la Santé et de la Recherche Médicale (INSERM)-Université de Tours, Institut National de la Recherche Agronomique (INRA)-Université de Tours, Institut National de la Recherche Agronomique (INRA)-Institut Français du Cheval et de l'Equitation [Saumur]-Université de Tours-Centre National de la Recherche Scientifique (CNRS), Groupe Hospitalier Paris Saint-Joseph (hpsj), Institut National de la Recherche Agronomique (INRA)-Institut Français du Cheval et de l'Equitation [Saumur] (IFCE)-Université de Tours (UT)-Centre National de la Recherche Scientifique (CNRS), and ProdInra, Archive Ouverte

Subjects

Male, pig, Pathology, Cystic Fibrosis, Swine, medicine.medical_treatment, Cystic Fibrosis Transmembrane Conductance Regulator, lcsh:Medicine, Computed tomography, ileostomy, Gastroenterology, Cystic fibrosis, 0302 clinical medicine, fluids and secretions, maladie génétique, lcsh:Science, fibrose cystique, 0303 health sciences, Gastrointestinal tract, Multidisciplinary, biology, medicine.diagnostic_test, sucking pig, respiratory system, Cystic fibrosis transmembrane conductance regulator, 3. Good health, 030220 oncology & carcinogenesis, histopathology, Female, porcelet, Autre (Sciences du Vivant), Research Article, medicine.medical_specialty, [SDV.OT]Life Sciences [q-bio]/Other [q-bio.OT], congenital, hereditary, and neonatal diseases and abnormalities, Genotype, Meconium Ileus, ileostomie, [SDV.IB.MN]Life Sciences [q-bio]/Bioengineering/Nuclear medicine, [SDV.IB.MN] Life Sciences [q-bio]/Bioengineering/Nuclear medicine, 03 medical and health sciences, Ileostomy, tomodensitométrie, genetic disease, Intensive care, Internal medicine, medicine, Animals, porcin, 030304 developmental biology, [SDV.OT] Life Sciences [q-bio]/Other [q-bio.OT], business.industry, histopathologie, lcsh:R, medicine.disease, digestive system diseases, Animals, Newborn, Nuclear medicine, biology.protein, Histopathology, lcsh:Q, business, Tomography, X-Ray Computed, Médecine nucléaire

Abstract

Background Cystic Fibrosis (CF) is the most prevalent autosomal recessive disease in the Caucasian population. A cystic fibrosis transmembrane conductance regulator knockout (CFTR-/-) pig that displays most of the features of the human CF disease has been recently developed. However, CFTR -/- pigs presents a 100% prevalence of meconium ileus that leads to death in the first hours after birth, requiring a rapid diagnosis and surgical intervention to relieve intestinal obstruction. Identification of CFTR -/- piglets is usually performed by PCR genotyping, a procedure that lasts between 4 to 6 h. Here, we aimed to develop a procedure for rapid identification of CFTR -/- piglets that will allow placing them under intensive care soon after birth and immediately proceeding with the surgical correction. Methods and Principal Findings Male and female CFTR +/- pigs were crossed and the progeny was examined by computed tomography (CT) scan to detect the presence of meconium ileus and facilitate a rapid post-natal surgical intervention. Genotype was confirmed by PCR. CT scan presented a 94.4% sensitivity to diagnose CFTR -/- piglets. Diagnosis by CT scan reduced the birth-to-surgery time from a minimum of 10 h down to a minimum of 2.5 h and increased the survival of CFTR -/- piglets to a maximum of 13 days post-surgery as opposed to just 66 h after later surgery. Conclusion CT scan imaging of meconium ileus is an accurate method for rapid identification of CFTR -/- piglets. Early CT detection of meconium ileus may help to extend the lifespan of CFTR -/- piglets and, thus, improve experimental research on CF, still an incurable disease.

Published

2015

17. Transcriptional profiling of the circulating immune response to lassa virus in an aerosol model of exposure

Author

John H. Connor, Judy Y. Yen, Shikha Malhotra, Ignacio S. Caballero, Eric M. Mucker, John C. Trefry, Sara Garamszegi, Anna N. Honko, Joshua C. Johnson, and Lisa E. Hensley

Subjects

Male, lcsh:Arctic medicine. Tropical medicine, Microarray, lcsh:RC955-962, Immunology, Viremia, Disease, Biology, Adaptive Immunity, medicine.disease_cause, Microbiology, Transcriptome, Immune Activation, Immune system, Lassa Fever, Model Organisms, Virology, medicine, Animals, Lassa virus, Immune Response, Regulation of gene expression, lcsh:Public aspects of medicine, Gene Expression Profiling, Toll-Like Receptors, Public Health, Environmental and Occupational Health, Immunity, Immunoregulation, lcsh:RA1-1270, Immune Defense, Animal Models, medicine.disease, Immunity, Innate, Innate Immunity, Host-Pathogen Interaction, Animal Models of Infection, Infectious Diseases, Leukocytes, Mononuclear, Macaca, Female, Viral load, Macaque, Research Article

Abstract

Lassa virus (LASV) is a significant human pathogen that is endemic to several countries in West Africa. Infection with LASV leads to the development of hemorrhagic fever in a significant number of cases, and it is estimated that thousands die each year from the disease. Little is known about the complex immune mechanisms governing the response to LASV or the genetic determinants of susceptibility and resistance to infection. In the study presented here, we have used a whole-genome, microarray-based approach to determine the temporal host response in the peripheral blood mononuclear cells (PBMCs) of non-human primates (NHP) following aerosol exposure to LASV. Sequential sampling over the entire disease course showed that there are strong transcriptional changes of the immune response to LASV exposure, including the early induction of interferon-responsive genes and Toll-like receptor signaling pathways. However, this increase in early innate responses was coupled with a lack of pro-inflammatory cytokine response in LASV exposed NHPs. There was a distinct lack of cytokines such as IL1β and IL23α, while immunosuppressive cytokines such as IL27 and IL6 were upregulated. Comparison of IRF/STAT1-stimulated gene expression with the viral load in LASV exposed NHPs suggests that mRNA expression significantly precedes viremia, and thus might be used for early diagnostics of the disease. Our results provide a transcriptomic survey of the circulating immune response to hemorrhagic LASV exposure and provide a foundation for biomarker identification to allow clinical diagnosis of LASV infection through analysis of the host response., Author Summary Lassa virus (LASV), a member of the Arenaviridae family, is a viral hemorrhagic fever causing virus endemic to several countries in West Africa with a history of sporadic importation into the United States. It has been characterized as a Category A agent, and despite the significant public health issues posed by LASV and the potential biodefense risks, little is known about the immune response to the virus. In the study presented here, we have taken an unbiased genomics approach to map the temporal host response in the peripheral blood mononuclear cells (PBMCs) of non-human primates (NHP) exposed to LASV. Gene expression patterns over the entire disease course showed that there are strong transcriptional changes of the immune response to LASV exposure, including the upregulation of Toll-like receptor signaling pathways and innate antiviral transcription factors. However, there was a lack of pro-inflammatory cytokine response in LASV exposed NHPs similar to what is seen in human disease. Our data suggests that LASV induces negative regulation of immunological events, leading to an inefficient adaptive immune response as observed in LASV-infected human patients. Our results provide a picture of the host's circulating immune response to hemorrhagic LASV exposure and demonstrate that gene expression patterns correlate with specific stages of disease progression.

Published

2012

18. Evaluation of the Serratia marcescens nuclease (NucA) as a transgenic cell ablation system in porcine

Author

Ignacio S. Caballero and Jorge A. Piedrahita

Subjects

Serratia, Swine, Transgene, Gene Expression, Bioengineering, Cell Separation, Biology, chemistry.chemical_compound, Gene expression, Endoribonucleases, Animals, Gene, Cells, Cultured, Diphtheria toxin, Endodeoxyribonucleases, Gene Transfer Techniques, Promoter, Fibroblasts, Serratia marcescens nuclease, Molecular biology, Blasticidin S, Electroporation, chemistry, Cell culture, Animal Science and Zoology, Rabbits, Biotechnology

Abstract

The efficiency of the Serratia marcescens nuclease encoded by the NucA gene, with or without a nuclear localization signal (NLS), and the commonly used diphtheria toxin A (DTA) were compared for their ability to ablate cells in culture. Constructs containing the test genes driven by the beta-actin promoter coupled with enhancer elements from the cytomegalovirus promoter and rabbit beta-globin gene (pCAG) and the blasticidin resistance gene driven by the phosphoglycerate kinase (PGK) promoter were generated and electroporated into porcine fetal fibroblasts. Three independent replicates were completed. Following blasticidin selection, the number of surviving colonies was counted to assess the efficiency of the toxic gene. Both NucA and DTA proved to be effective in killing porcine fibroblasts compared to controls. However, the efficiency of cell ablation was significantly higher with DTA than with NucA or NucANLS (p < 0.05). Gene expression analysis of surviving colonies indicated that survival is related to low or absent expression of the toxic genes. These results indicate that the NucA gene, while capable of mammalian cell ablation, is less efficient than DTA.

Published

2009

19. Lassa and Marburg viruses elicit distinct host transcriptional responses early after infection

Author

Arthur J. Goff, Ignacio S. Caballero, John H. Connor, Judy Y. Yen, Lisa E. Hensley, and Anna N. Honko

Subjects

Male, Hemorrhagic Fevers, Viral, Transcription, Genetic, Biology, medicine.disease_cause, Virus, Viral hemorrhagic fever, Marburg virus, Transcriptome, Transcriptional response, Genetics, medicine, Animals, Lassa virus, Transcriptomics, Interferon-stimulated genes, Pathogen, Regulation of gene expression, Sequence Analysis, RNA, Gene Expression Profiling, Monkey Diseases, Early stage diagnostics, Reproducibility of Results, Biomarker, Gene expression profile, medicine.disease, Marburgvirus, biology.organism_classification, Virology, Macaca fascicularis, Gene Expression Regulation, Host-Pathogen Interactions, Interferon Type I, Immunology, Leukocytes, Mononuclear, Female, Research Article, Biotechnology

Abstract

Background Lassa virus and Marburg virus are two causative agents of viral hemorrhagic fever. Their diagnosis is difficult because patients infected with either pathogen present similar nonspecific symptoms early after infection. Current diagnostic tests are based on detecting viral proteins or nucleic acids in the blood, but these cannot be found during the early stages of disease, before the virus starts replicating in the blood. Using the transcriptional response of the host during infection can lead to earlier diagnoses compared to those of traditional methods. Results In this study, we use RNA sequencing to obtain a high-resolution view of the in vivo transcriptional dynamics of peripheral blood mononuclear cells (PBMCs) throughout both types of infection. We report a subset of host mRNAs, including heat-shock proteins like HSPA1B, immunoglobulins like IGJ, and cell adhesion molecules like SIGLEC1, whose differences in expression are strong enough to distinguish Lassa infection from Marburg infection in non-human primates. We have validated these infection-specific expression differences by using microarrays on a larger set of samples, and by quantifying the expression of individual genes using RT-PCR. Conclusions These results suggest that host transcriptional signatures are correlated with specific viral infections, and that they can be used to identify highly pathogenic viruses during the early stages of disease, before standard detection methods become effective. Electronic supplementary material The online version of this article (doi:10.1186/1471-2164-15-960) contains supplementary material, which is available to authorized users.

Published

2014

20. Diagnosing Lassa virus infection by tracking the antiviral response

Author

Ignacio S. Caballero, Gracia Bonilla, Judy Y. Yen, and John H. Connor

Subjects

Hospitalized patients, viruses, Applied Mathematics, Mortality rate, Lassa virus infection, virus diseases, Biology, medicine.disease_cause, medicine.disease, Biochemistry, Virology, Computer Science Applications, Viral hemorrhagic fever, Lassa virus, Structural Biology, General malaise, Meeting Abstract, medicine, Sore throat, medicine.symptom, Lassa fever, Molecular Biology

Abstract

Background Lassa fever is an acute viral hemorrhagic fever caused by the Lassa virus. It infects 300,000 to 500,000 West Africans every year, with a mortality rate among hospitalized patients of 15%. It is difficult to diagnose because its early symptoms (fever, sore throat, general malaise) often go

Published

2012