Your search keyword '"Nicole Y. Lai"' showing total 9 results

1. FcεR1-expressing nociceptors trigger allergic airway inflammation

Author

Alp Ozcan, Simmie L. Foster, Mohammad Balood, Nicole Y. Lai, Abdelilah Majdoubi, Theo Crosson, Alexandre Parrin, Clifford J. Woolf, Xuan Huang, Benjamin Doyle, Maud Pascal, Hannah Merrison, Raja-Elie E. Abdulnour, Trevor Rajchgot, Elise Semenara, Bruce D. Levy, Jo-Chiao Wang, Jörg H. Fritz, Corey R. Seehus, Sébastien Talbot, Moutih Rafei, Barbara C. Mindt, and Jacques Thibodeau

Subjects

0301 basic medicine, Allergy, Ovalbumin, Immunology, TRPV1, Gene Expression, Respiratory Mucosa, Substance P, Immunoglobulin E, Article, Allergic inflammation, Allergic sensitization, 03 medical and health sciences, Mice, 0302 clinical medicine, Dorsal root ganglion, Hypersensitivity, Immunology and Allergy, Medicine, Animals, Genetic Predisposition to Disease, Mice, Knockout, Neurons, biology, business.industry, Receptors, IgE, FCER1, Nociceptors, Vagus Nerve, respiratory system, Allergens, medicine.disease, Disease Models, Animal, 030104 developmental biology, medicine.anatomical_structure, nervous system, Nociceptor, biology.protein, Calcium, Disease Susceptibility, business, 030217 neurology & neurosurgery

Abstract

Background Lung nociceptor neurons amplify immune cell activity and mucus metaplasia in response to an inhaled allergen challenge in sensitized mice. Objective We sought to identify the cellular mechanisms by which these sensory neurons are activated subsequent to allergen exposure. Methods We used calcium microscopy and electrophysiologic recording to assess whether vagal neurons directly respond to the model allergen ovalbumin (OVA). Next, we generated the first nociceptor-specific FceR1γ knockdown (TRPV1Cre::FceR1γfl/fl) mice to assess whether this targeted invalidation would affect the severity of allergic inflammation in response to allergen challenges. Results Lung-innervating jugular nodose complex ganglion neurons express the high-affinity IgE receptor FceR1, the levels of which increase in OVA-sensitized mice. FceR1γ-expressing vagal nociceptor neurons respond directly to OVA complexed with IgE with depolarization, action potential firing, calcium influx, and neuropeptide release. Activation of vagal neurons by IgE-allergen immune complexes, through the release of substance P from their peripheral terminals, directly amplifies TH2 cell influx and polarization in the airways. Allergic airway inflammation is decreased in TRPV1Cre::FceR1γfl/fl mice and in FceR1α–/– mice into which bone marrow has been transplanted. Finally, increased in vivo circulating levels of IgE following allergen sensitization enhances the responsiveness of FceR1 to immune complexes in both mouse jugular nodose complex ganglion neurons and human induced pluripotent stem cell–derived nociceptors. Conclusions Allergen sensitization triggers a feedforward inflammatory loop between IgE-producing plasma cells, FceR1-expressing vagal sensory neurons, and TH2 cells, which helps to both initiate and amplify allergic airway inflammation. These data highlight a novel target for reducing allergy, namely, FceR1γ expressed by nociceptors.

Published

2020

2. Silencing Nociceptor Neurons Reduces Allergic Airway Inflammation

Author

Maud Pascal, Josef M. Penninger, Simmie L. Foster, Raja-Elie E. Abdulnour, Isaac M. Chiu, Vijay K. Kuchroo, David Roberson, Bruce P. Bean, Clifford J. Woolf, Oliver Haworth, Christian A. von Hehn, Shane J. F. Cronin, Sébastien Talbot, Matthew DiBiase, Busranour Agac, Cédric J. Laedermann, Bruce D. Levy, Patrick R. Burkett, Seungkyu Lee, Johnathan V. Tran, Hiroyuki Seki, Nicole Y. Lai, and Nader Ghasemlou

Subjects

biology, Chemistry, General Neuroscience, medicine.medical_treatment, Sodium channel, Neuroscience(all), Vasoactive intestinal peptide, Article, respiratory tract diseases, 3. Good health, Allergic inflammation, Ovalbumin, Cytokine, Immune system, nervous system, Immunology, medicine, Nociceptor, biology.protein, Gene silencing

Abstract

SummaryLung nociceptors initiate cough and bronchoconstriction. To elucidate if these fibers also contribute to allergic airway inflammation, we stimulated lung nociceptors with capsaicin and observed increased neuropeptide release and immune cell infiltration. In contrast, ablating Nav1.8+ sensory neurons or silencing them with QX-314, a charged sodium channel inhibitor that enters via large-pore ion channels to specifically block nociceptors, substantially reduced ovalbumin- or house-dust-mite-induced airway inflammation and bronchial hyperresponsiveness. We also discovered that IL-5, a cytokine produced by activated immune cells, acts directly on nociceptors to induce the release of vasoactive intestinal peptide (VIP). VIP then stimulates CD4+ and resident innate lymphoid type 2 cells, creating an inflammatory signaling loop that promotes allergic inflammation. Our results indicate that nociceptors amplify pathological adaptive immune responses and that silencing these neurons with QX-314 interrupts this neuro-immune interplay, revealing a potential new therapeutic strategy for asthma.

Published

2015

3. Different Antigen-Processing Activities in Dendritic Cells, Macrophages, and Monocytes Lead to Uneven Production of HIV Epitopes and Affect CTL Recognition

Author

Yang Xu, Pauline Gourdain, Mariko Shimada, Ellen Duong, Nicole Y. Lai, Daniel G. Kavanagh, Edith Bracho-Sanchez, Marijana Rucevic, Jens Dinter, Musie Ghebremichael, Sylvie Le Gall, and Paul Liebesny

Subjects

Proteasome Endopeptidase Complex, Proteases, Immunology, Antigen presentation, HIV Infections, Biology, Major histocompatibility complex, Monocytes, Article, Epitope, Immunophenotyping, Epitopes, Cytosol, medicine, Animals, Humans, Immunology and Allergy, Cytotoxic T cell, Amino Acid Sequence, Cell Line, Transformed, Antigen Presentation, Protein Stability, Antigen processing, Macrophages, Monocyte, Toll-Like Receptors, HIV, Dendritic Cells, CTL, medicine.anatomical_structure, Antigens, Surface, Proteolysis, Leukocytes, Mononuclear, biology.protein, Peptides, Peptide Hydrolases, T-Lymphocytes, Cytotoxic

Abstract

Dendritic cells (DCs), macrophages (MPs), and monocytes are permissive to HIV. Whether they similarly process and present HIV epitopes to HIV-specific CD8 T cells is unknown despite the critical role of peptide processing and presentation for recognition and clearance of infected cells. Cytosolic peptidases degrade endogenous proteins originating from self or pathogens, exogenous Ags preprocessed in endolysosomes, thus shaping the peptidome available for endoplasmic reticulum translocation, trimming, and MHC-I presentation. In this study, we compared the capacity of DCs, MPs, and monocyte cytosolic extracts to produce epitope precursors and epitopes. We showed differences in the proteolytic activities and expression levels of cytosolic proteases between monocyte-derived DCs and MPs and upon maturation with LPS, R848, and CL097, with mature MPs having the highest activities. Using cytosol as a source of proteases to degrade epitope-containing HIV peptides, we showed by mass spectrometry that the degradation patterns of long peptides and the kinetics and amount of antigenic peptides produced differed among DCs, MPs, and monocytes. Additionally, variable intracellular stability of HIV peptides prior to loading onto MHC may accentuate the differences in epitope availability for presentation by MHC-I between these subsets. Differences in peptide degradation led to 2- to 25-fold differences in the CTL responses elicited by the degradation peptides generated in DCs, MPs, and monocytes. Differences in Ag-processing activities between these subsets might lead to variations in the timing and efficiency of recognition of HIV-infected cells by CTLs and contribute to the unequal capacity of HIV-specific CTLs to control viral load.

Published

2014

4. A real-time killing assay to follow viral epitope presentation to CD8 T cells

Author

Julie Boucau, Pauline Gourdain, Ellen Duong, Sylvie Le Gall, Nicole Y. Lai, and Georgio Kourjian

Subjects

CD4-Positive T-Lymphocytes, Male, Immunology, Antigen presentation, Epitopes, T-Lymphocyte, HIV Infections, CD8-Positive T-Lymphocytes, Glucosephosphate Dehydrogenase, Biology, Major histocompatibility complex, Article, Epitope, chemistry.chemical_compound, Immune system, Humans, Immunology and Allergy, Cytotoxic T cell, Cell Line, Transformed, Antigen Presentation, Antigen processing, Carboxyfluorescein succinimidyl ester, Virology, Molecular biology, CTL, chemistry, HIV-1, biology.protein, Female

Abstract

The ability of cytotoxic T lymphocytes (CTL) to clear virus-infected cells requires the presentation of viral peptides intracellularly processed and displayed by major histocompatibility complex class I. Assays to measure CTL-mediated killing often use peptides exogenously added onto target cells –which does not account for epitope processing- or follow killing of infected cells at a single time point. In this study we established a real-time fluorogenic cytotoxic assay that measures the release of the Glucose-6-phosphate-dehydrogenase by dying target cells every 5 minutes after addition of CTL. It has comparable sensitivity to 51chromium-based killing assay with the additional advantage of incorporating the kinetics of epitope presentation. We showed that HIV infection of immortalized or primary CD4 T cells leads to asynchronous killing by two CTL clones specific for epitopes located in different proteins. Real-time monitoring of killing of virus-infected cells will enable identification of immune responses efficiently preventing virus dissemination.

Published

2013

5. Variable processing and presentation of HIV epitopes in dendritic cells and macrophages to CD8 T cells

Author

Paul Liebesny, Jens Dinter, Pauline Gourdain, Ellen Duong, Nicole Y. Lai, T Zhu, S Le Gall, Mariko Shimada, and Edith Bracho-Sanchez

Subjects

lcsh:Immunologic diseases. Allergy, Proteases, biology, business.industry, chemical and pharmacologic phenomena, Major histocompatibility complex, Epitope, Infectious Diseases, HIV Antigens, Virology, Poster Presentation, Immunology, biology.protein, Cytotoxic T cell, Medicine, Antibody, lcsh:RC581-607, Receptor, business, Intracellular

Abstract

Background Whether HIV-infectable subsets, such as CD4 T cells, monocytes, macrophages and dendritic cells (DCs), have equivalent capacity to produce and present MHC-I restricted epitopes to HIV-specific CD8 T cells is unknown. MHC-I epitopes are processed by an intracellular degradation pathway involving multiple proteases. In this study we analyzed the effect of toll-like receptor (TLR) agonist-mediated maturation on the processing and presentation of HIV antigens in monocyte-derived DCs and macrophages.

Published

2012

6. Aminopeptidase substrate preference affects HIV epitope presentation and predicts immune escape patterns in HIV-infected individuals

Author

Zabrina L. Brumme, Huabiao Chen, Sasha B. Godfrey, Mariko Shimada, Eric Martin, Chanson J. Brumme, Jonathan M. Carlson, Bruce D. Walker, Sylvie Le Gall, Shao Chong Zhang, Paul Liebesny, Shirley Locastro, Jennifer Fricke, Daniel G. Kavanagh, Oluwatobi Awele Ogbechie, and Nicole Y. Lai

Subjects

Immunology, Antigen presentation, Human Immunodeficiency Virus Proteins, Epitopes, T-Lymphocyte, HIV Infections, Cell Separation, Lymphocyte Activation, Aminopeptidase, Aminopeptidases, Epitope, Article, Immune system, MHC class I, Immunology and Allergy, Humans, Immune Evasion, Antigen Presentation, Linear epitope, biology, Histocompatibility Antigens Class I, Flow Cytometry, Virology, CTL, Viral evolution, Mutation, biology.protein

Abstract

Viruses evade immune detection partly through immune-associated mutations. Analyses of HIV sequences derived from infected individuals have identified numerous examples of HLA-associated mutations within or adjacent to T cell epitopes, but the potential impact of most mutations on epitope production and presentation remains unclear. The multistep breakdown of proteins into epitopes includes trimming of N-extended peptides into epitopes by aminopeptidases before loading onto MHC class I molecules. Definition of sequence signatures that modulate epitope production would lead to a better understanding of factors driving viral evolution and immune escape at the population level. In this study, we identified cytosolic aminopeptidases cleavage preferences in primary cells and its impact on HIV Ag degradation into epitopes in primary human cell extracts by mass spectrometry and on epitope presentation to CTL. We observed a hierarchy of preferred amino acid cleavage by cytosolic aminopeptidases. We demonstrated that flanking mutations producing more or less cleavable motifs can increase or decrease epitope production and presentation by up to 14-fold. We found that the efficiency of epitope production correlates with cleavability of flanking residues. These in vitro findings were supported by in vivo population-level analyses of clinically derived viral sequences from 1134 antiretroviral-naive HIV-infected individuals: HLA-associated mutations immune pressures drove the selection of residues that are less cleavable by aminopeptidases predominantly at N-flanking sites, leading to reduced epitope production and immune recognition. These results underscore an important and widespread role of Ag processing mutations in HIV immune escape and identify molecular mechanisms underlying impaired epitope presentation.

Published

2012

7. Variable Processing and Cross-presentation of HIV by Dendritic Cells and Macrophages Shapes CTL Immunodominance and Immune Escape

Author

Jens Dinter, Shao Chong Zhang, Sylvie Le Gall, Matthew J. Berberich, Hang Su, Nicole Y. Lai, Ellen Duong, Duong Chu, Edith Bracho-Sanchez, and Georgio Kourjian

Subjects

QH301-705.5, Immunology, Epitopes, T-Lymphocyte, HIV Infections, Immunodominance, Biology, Major histocompatibility complex, Microbiology, Mass Spectrometry, Epitope, Cross-Priming, Immune system, Antigen, Virology, Genetics, Humans, Biology (General), Molecular Biology, Immune Evasion, Immunodominant Epitopes, Macrophages, Cross-presentation, Dendritic Cells, RC581-607, 3. Good health, CTL, HIV Antigens, HIV-1, biology.protein, Parasitology, Immunologic diseases. Allergy, T-Lymphocytes, Cytotoxic, Research Article

Abstract

Dendritic cells (DCs) and macrophages (Møs) internalize and process exogenous HIV-derived antigens for cross-presentation by MHC-I to cytotoxic CD8+ T cells (CTL). However, how degradation patterns of HIV antigens in the cross-presentation pathways affect immunodominance and immune escape is poorly defined. Here, we studied the processing and cross-presentation of dominant and subdominant HIV-1 Gag-derived epitopes and HLA-restricted mutants by monocyte-derived DCs and Møs. The cross-presentation of HIV proteins by both DCs and Møs led to higher CTL responses specific for immunodominant epitopes. The low CTL responses to subdominant epitopes were increased by pretreatment of target cells with peptidase inhibitors, suggestive of higher intracellular degradation of the corresponding peptides. Using DC and Mø cell extracts as a source of cytosolic, endosomal or lysosomal proteases to degrade long HIV peptides, we identified by mass spectrometry cell-specific and compartment-specific degradation patterns, which favored the production of peptides containing immunodominant epitopes in all compartments. The intracellular stability of optimal HIV-1 epitopes prior to loading onto MHC was highly variable and sequence-dependent in all compartments, and followed CTL hierarchy with immunodominant epitopes presenting higher stability rates. Common HLA-associated mutations in a dominant epitope appearing during acute HIV infection modified the degradation patterns of long HIV peptides, reduced intracellular stability and epitope production in cross-presentation-competent cell compartments, showing that impaired epitope production in the cross-presentation pathway contributes to immune escape. These findings highlight the contribution of degradation patterns in the cross-presentation pathway to HIV immunodominance and provide the first demonstration of immune escape affecting epitope cross-presentation., Author Summary Pathogens such as HIV can enter cells by fusion at the plasma membrane for delivery in the cytosol, or by internalization in endolysosomal vesicles. Pathogens can be degraded in these various compartments into peptides (epitopes) displayed at the cell surface by MHC-I. The presentation of pathogen-derived peptides triggers the activation of T cell immune responses and the clearance of infected cells. How the diversity of compartments in which HIV traffics combined with the diversity of HIV sequences affects the degradation of HIV and the recognition of infected cells by immune cells is not understood. We compared the degradation of HIV proteins in subcellular compartments of dendritic cells and macrophages, two cell types targeted by HIV and the subsequent presentation of epitopes to T cells. We show variable degradation patterns of HIV according to compartments, and the preferential production and superior intracellular stability of immunodominant epitopes corresponding to stronger T cell responses. Frequent mutations in immunodominant epitopes during acute infection resulted in decreased production and intracellular stability of these epitopes. Together these results demonstrate the importance of protein degradation patterns in shaping immunodominant epitopes and the contribution of impaired epitope production in all cellular compartments to immune escape during HIV infection.

Published

2015

8. Alteration of HIV epitope processing and presentation by HIV protease inhibitors

Author

Mariko Shimada, Julie Boucau, Georgio Kourjian, S Le Gall, and Nicole Y. Lai

Subjects

lcsh:Immunologic diseases. Allergy, Protease, medicine.medical_treatment, virus diseases, Biology, Major histocompatibility complex, Virology, Epitope, Infectious Diseases, Nelfinavir, Indinavir, Poster Presentation, medicine, biology.protein, HIV Protease Inhibitor, Ritonavir, lcsh:RC581-607, Saquinavir, medicine.drug

Abstract

Background Epitopes displayed by MHC-I come from the multistep degradation of proteins by intracellular peptidases such as proteasome and aminopeptidases or cathepsins in the exogenous pathway. We hypothesize that due to structural homologies HIV protease inhibitors (PIs) used in antiretroviral therapies may affect activities of cellular peptidases involved in epitope processing and may affect epitope presentation to immune cells. Methods Using a fluorogenic assay the effect of 5 HIV-1 PIs (Ritonavir, Saquinavir, Nelfinavir, Indinavir, Atazanavir) on proteasome, aminopeptidase and cathepsin activities was tested in PBMCs from at least 6 healthy donors. Using PBMC cytosol as a source of peptidases and HPLC and mass spectrometry to define and quantify the degradation products, the effect of HIV PIs on HIV peptide processing kinetics and HIV epitope half-life was assessed. Finally we assessed the impact of PIs on the endogenous processing and presentation of epitopes by infected cells to CD8 T cells using a fluorescence-based cytotoxicity assay. Results HIV PIs variably altered proteasome, post-proteasomal aminopeptidases and cathepsin activities. Depending on the PI, some activities were inhibited (from 1.1 to 5 folds, p

Published

2012

9. A simple methodology to assess endolysosomal protease activity involved in antigen processing in human primary cells

Author

Archana Vaithilingam, Yang Xu, Sylvie Le Gall, Malini Gandhi, Ellen Duong, Nicole Y. Lai, J. Boucau, and Mariko Shimada

Subjects

Proteases, Molecular Sequence Data, Antigen presentation, Primary cells, T cell epitope production, Protein degradation, Biology, Major histocompatibility complex, Epitope, Endolysosome, MHC class I, Humans, Amino Acid Sequence, Antigens, Cells, Cultured, Antigen Presentation, Mass spectrometry, Antigen processing, Methodology Article, HIV, Proteins, Cell Biology, Hydrogen-Ion Concentration, Cathepsins, Cell biology, Biochemistry, Leukocytes, Mononuclear, biology.protein, MHC, Lysosomes, Peptide Hydrolases

Abstract

Background Endolysosomes play a key role in maintaining the homeostasis of the cell. They are made of a complex set of proteins that degrade lipids, proteins and sugars. Studies involving endolysosome contribution to cellular functions such as MHC class I and II epitope production have used recombinant endolysosomal proteins, knockout mice that lack one of the enzymes or purified organelles from human tissue. Each of these approaches has some caveats in analyzing endolysosomal enzyme functions. Results In this study, we have developed a simple methodology to assess endolysosomal protease activity. By varying the pH in crude lysate from human peripheral blood mononuclear cells (PBMCs), we documented increased endolysosomal cathepsin activity in acidic conditions. Using this new method, we showed that the degradation of HIV peptides in low pH extracts analyzed by mass spectrometry followed similar kinetics and degradation patterns as those performed with purified endolysosomes. Conclusion By using crude lysate in the place of purified organelles this method will be a quick and useful tool to assess endolysosomal protease activities in primary cells of limited availability. This quick method will especially be useful to screen peptide susceptibility to degradation in endolysosomal compartments for antigen processing studies, following which detailed analysis using purified organelles may be used to study specific peptides.