Abstract

DNA containing CpG motifs (CpG DNA) has incredible potential to treat cancer, infectious and allergic diseases. Despite this potential, response to our own nucleic acids, including DNA, triggers autoimmune diseases such as systemic lupus erythematosus. Localization and trafficking of the specific receptor, TLR9, may play a key role in self/foreign DNA discrimination. Uncovering the molecular mechanisms of TLR9 trafficking is the first step towards our long term goal of manipulating TLR9 trafficking to achieve modulation of CpG DNA response. We have shown that TLR9 is localized intracellularly, predominantly in the endoplasmic reticulum (ER), prior to CpG DNA stimulation. TLR9 traffics from the ER to endosomes and lysosomes where it co-localizes with endocytosed CpG DNA. These data raise the fundamental questions of what regulates TLR9 access to CpG DNA and how does access affect response to self and microbial DNA? Using new TLR9 trafficking assays, we have accumulated evidence that TLR9 constitutively exits the ER, that CpG DNA induces a secondary TLR9 trafficking event, and that both events occur through traditional cell trafficking pathways. Therefore, we hypothesize that TLR9 constitutively traffics in a highly regulated fashion through the cell secretory pathway from the Golgi complex to endolysosomes and that Golgi transit is a prerequisite for TLR9 response to CpG DNA. We believe that TLR9 trafficking may account for synergy with other TLRs and the autoimmune B cell receptor, and is regulated by post-translational modification of the TLR9 cytoplasmic tail. This hypothesis will be tested in three Specific Aims. First, transfected and endogenous TLR9 trafficking through the Golgi complex will be examined using multiple in vitro approaches including a novel protease cleavage assay. Second, we will examine the mechanism of TLR9-autoimmune B cell receptor synergism. Third, we will determine the role of TLR9 post-translational modification in regulating intracellular trafficking and in TLR-autoimmune B cell receptor synergy. By understanding the mechanism of TLR9 trafficking we can uncover how regulation of response to foreign DNA and lack of response to self-DNA is achieved. This knowledge will provide the basis for the further development of CpG DNA as an adjuvant and therapeutic as well as develop mechanisms to interrupt the cycle of autoimmune pathology.

Public Health Relevance

Despite incredible potential of CpG DNA to augment immune responses in cancer and infectious disease, inappropriate response to self DNA results in autoimmunity. This project seeks to identify key factors controlling localization of CpG DNA's specific receptor, Toll-like receptor 9. Through manipulating localization of TLR9, and thereby modulating CpG DNA activity, we hope to enhance vaccines and interrupt the cycle of autoimmune disease.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
3R01AI076588-01A2S1
Application #
7922302
Study Section
Innate Immunity and Inflammation Study Section (III)
Program Officer
Palker, Thomas J
Project Start
2009-09-17
Project End
2010-08-31
Budget Start
2009-09-17
Budget End
2010-08-31
Support Year
1
Fiscal Year
2009
Total Cost
$104,036
Indirect Cost

  Institution

Name
Cornell University
Department
Microbiology/Immun/Virology
Type
Schools of Veterinary Medicine
DUNS #
872612445
City
Ithaca
State
NY
Country
United States
Zip Code
14850

  Publications

Hasan, Maroof; Gruber, Erika; Cameron, Jody et al. (2016) TLR9 stability and signaling are regulated by phosphorylation and cell stress. J Leukoc Biol 100:525-33
Sinha, Siddhartha S; Cameron, Jody; Brooks, James C et al. (2016) Complex Negative Regulation of TLR9 by Multiple Proteolytic Cleavage Events. J Immunol 197:1343-52
Leifer, Cynthia A; Medvedev, Andrei E (2016) Molecular mechanisms of regulation of Toll-like receptor signaling. J Leukoc Biol 100:927-941
Patel, Hardik J; Patel, Pallav D; Ochiana, Stefan O et al. (2015) Structure-activity relationship in a purine-scaffold compound series with selectivity for the endoplasmic reticulum Hsp90 paralog Grp94. J Med Chem 58:3922-43
Rosenthal, Joseph A; Huang, Chung-Jr; Doody, Anne M et al. (2014) Mechanistic insight into the TH1-biased immune response to recombinant subunit vaccines delivered by probiotic bacteria-derived outer membrane vesicles. PLoS One 9:e112802
Leifer, Cynthia A; McConkey, Cameron; Li, Sha et al. (2014) Linking genetic variation in human Toll-like receptor 5 genes to the gut microbiome's potential to cause inflammation. Immunol Lett 162:3-9
Leifer, Cynthia A; Rose 2nd, William A; Botelho, Fernando (2013) Traditional biochemical assays for studying toll-like receptor 9. J Immunoassay Immunochem 34:1-15
Chockalingam, Annapoorani; Rose 2nd, William Alfred; Hasan, Maroof et al. (2012) Cutting edge: a TLR9 cytoplasmic tyrosine motif is selectively required for proinflammatory cytokine production. J Immunol 188:527-30
Rose 2nd, William Alfred; Sakamoto, Kaori; Leifer, Cynthia Anne (2012) TLR9 is important for protection against intestinal damage and for intestinal repair. Sci Rep 2:574
Brooks, James C; Sun, Weilin; Chiosis, Gabriela et al. (2012) Heat shock protein gp96 regulates Toll-like receptor 9 proteolytic processing and conformational stability. Biochem Biophys Res Commun 421:780-4

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