Abstract

Tuberculosis (TB) is a leading cause of infectious disease mortality worldwide, accounting for 10.4 million new cases and 1.3 million deaths annually. An understanding of the immune response to Mtb is of central importance in the development of improved vaccines. In this regard our laboratory, under the auspices of the VA Merit Program, has defined Mucosal Associated Invariant T (MAIT) cells as a class of cells that are restricted by the highly conserved MR1 molecule, recognize Mtb-infected cells, have effector capacity in the thymus and cord blood, yet display evidence for memory following exposure to Mtb, and are enriched in the lungs. MAIT cells are found in tissues such as the lung and intestine. Because MAIT cells recognize small molecules, such as metabolites of riboflavin, we postulate that the cell surface expression of MR1 is tightly regulated to avoid activation of these cells in the absence of intracellular infection. Indeed, with the support of the VA Merit Program, we have found that MR1 is both located in an endosome, requires a ligand for translocation to the cell surface, and is dependent on vesicular trafficking for the presentation of Mtb-derived antigens to MR1T cells. Furthermore, we find that the mechanisms underlying presentation of Mtb-derived antigens can be distinguished from antigens that are exogenously delivered, suggesting that there are specialized mechanisms for sampling the intracellular environment. Therefore, in this application we will focus on defining the molecular mechanisms that allow for the appropriate presentation of intracellular infection, with a focus on Mtb. We will 1) Define the molecular chaperones required for the presentation of microbials ligands, and 2) Define the role of MR1 SNPs and splice variants in controlling the recognition of the Mtb infected cell, and will evaluate these variants in clinically relevant outcomes following exposure to Mtb. This project contains two Aims:
AIM 1 : Define the molecular chaperones necessary for the presentation of Mtb-derived ligands 1a. Determine the molecular chaperones associated with MR1. 1b. Determine the role of riboflavin transporters in the uptake or trafficking of MR1 ligands.
AIM 2 : Define the role of MR1 SNPs and splice variants in human susceptibility to TB 2a. Determine the relationship of MR1 SNPs and splice variants and clinical outcomes associated with exposure to Mtb. 2b. Determine the functional significance of MR1 SNPs. 2c. Determine the relationship of MR1 splice variant expression and the capacity of cells to present MR1 ligands to MR1T cells.

Public Health Relevance

Tuberculosis remains an important cause of infectious disease morbidity and mortality worldwide, and remains a problem of particular concern to those in the armed forces. The organism that causes tuberculosis, Mycobacterium tuberculosis, is an intracellular pathogen such that improved definition of those mechanisms by which the immune system recognizes intracellular infection provides direct application to improved vaccines and diagnostics. This application is focused on understanding how a unique population of innate human CD8+ T cells identify those cells containing Mtb.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
Veterans Affairs (VA)
Type
Non-HHS Research Projects (I01)
Project #
2I01BX000533-09A1
Application #
10124862
Study Section
Special Emphasis Panel (ZRD1)
Project Start
2010-04-01
Project End
2024-12-31
Budget Start
2021-01-01
Budget End
2021-12-31
Support Year
9
Fiscal Year
2021
Total Cost
Indirect Cost

  Institution

Name
Portland VA Medical Center
Department
Type
DUNS #
089461255
City
Portland
State
OR
Country
United States
Zip Code
97239

  Publications

Harriff, Melanie J; McMurtrey, Curtis; Froyd, Cara A et al. (2018) MR1 displays the microbial metabolome driving selective MR1-restricted T cell receptor usage. Sci Immunol 3:
Hartmann, Nadine; McMurtrey, Curtis; Sorensen, Michelle L et al. (2018) Riboflavin Metabolism Variation among Clinical Isolates of Streptococcus pneumoniae Results in Differential Activation of Mucosal-associated Invariant T Cells. Am J Respir Cell Mol Biol 58:767-776
Meermeier, Erin W; Harriff, Melanie J; Karamooz, Elham et al. (2018) MAIT cells and microbial immunity. Immunol Cell Biol 96:607-617
Hartmann, Nadine; Harriff, Melanie J; McMurtrey, Curtis P et al. (2018) Role of MAIT cells in pulmonary bacterial infection. Mol Immunol 101:155-159
Greene, J M; Dash, P; Roy, S et al. (2017) MR1-restricted mucosal-associated invariant T (MAIT) cells respond to mycobacterial vaccination and infection in nonhuman primates. Mucosal Immunol 10:802-813
Harriff, Melanie J; Wolfe, Lisa M; Swarbrick, Gwendolyn et al. (2017) HLA-E Presents Glycopeptides from the Mycobacterium tuberculosis Protein MPT32 to Human CD8+ T cells. Sci Rep 7:4622
McMurtrey, Curtis; Harriff, Melanie J; Swarbrick, Gwendolyn M et al. (2017) T cell recognition of Mycobacterium tuberculosis peptides presented by HLA-E derived from infected human cells. PLoS One 12:e0188288
Nyendak, Melissa; Swarbrick, Gwendolyn M; Duncan, Amanda et al. (2016) Adenovirally-Induced Polyfunctional T Cells Do Not Necessarily Recognize the Infected Target: Lessons from a Phase I Trial of the AERAS-402 Vaccine. Sci Rep 6:36355
Laugel, Bruno; Lloyd, Angharad; Meermeier, Erin W et al. (2016) Engineering of Isogenic Cells Deficient for MR1 with a CRISPR/Cas9 Lentiviral System: Tools To Study Microbial Antigen Processing and Presentation to Human MR1-Restricted T Cells. J Immunol 197:971-82
Meermeier, Erin W; Laugel, Bruno F; Sewell, Andrew K et al. (2016) Human TRAV1-2-negative MR1-restricted T cells detect S. pyogenes and alternatives to MAIT riboflavin-based antigens. Nat Commun 7:12506

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