Abstract

Toll-like receptors (TLRs) generate an innate immune signaling response upon recognizing broadly conserved microbial extracellular structures. Viral RNA is recognized by!TLR3, TLR7 and TLR8, and microbial DNA is recognized by TLR9. Until recently the prevailing paradigm was that TLR9 recognized unmethylated CpG DNA motifs, which are abundant in bacteria but relatively scarce in mammalian DNA. However, recent studies including our own preliminary data suggest that TLR9 binds natural DNA ligands independently of their sequence and methylation state. We propose a comprehensive analysis of the structural properties that allow TLR9 to recognize microbial DNA including sequence, length, duplex content, methylation state, backbone chemistry (phosphodiester versus phosphorothioate), curvature and higher order structure (such as junctions). We show in preliminary studies that DNA curvature-inducing proteins!HMGB1 and histones H2A and H2B significantly enhance binding to the C-terminal cleavage fragment of TLR9, suggesting that TLR9 preferentially recognizes curved DNA backbones. To determine the extent to which DNA curvature alone is responsible for the binding enhancement, we propose to measure the TLR9 binding affinity of DNA minicircles containing 75 to 120 base pairs. Since nucleosomes can induce TLR-dependent auto immunogenic signaling, we propose an in vitro biophysical analysis of whole nucleosomes as TLR9 ligands! These in vitro studies will be validated in vivo by measuring TLR9-dependent signaling responses in cells stimulated with various DNA or protein-DNA ligands including minicircles, nucleosomes, junctions and methylated DNA ligands. The TLR7/8/9 ectodomains must be proteolytically cleaved in order to produce receptors that are capable of signaling. In the first study with cleaved TLR9, we show in our preliminary data that both the N- and C-terminal TLR9 ectodomain fragments participate in ligand binding and receptor dimerization. We therefore hypothesize that the two fragments remain associated after proteolytic cleavage in the endosome, and that cleavage may be necessary for TLR9 to undergo the ligand-induced conformational change that activates the receptor. To test this hypothesis, we will explore the physical and functional relationships between the two TLR9 ectodomain fragments, and elucidate the physical basis of proteolytic activation using biophysical approaches. The lack of structural information for TLR7/8/9 limits our understanding of nucleic acid recognition by these receptors. We propose to use electron cryomicroscopy and X-ray crystallography as complementary approaches to gain insight into the structural basis of TLR9-DNA recognition. By providing a molecular-level understanding of the recognition of microbial DNA by TLR9, this project will provide the necessary tools to create more potent vaccine adjuvants, and a new class of anti-inflammatory therapeutics with a wide range of applications including in particular systemic lupus erythematosus, asthma, septic shock syndrome and organ transplant rejection.

Public Health Relevance

Innate immune receptors in specialized cellular compartments recognize the genetic material of invading pathogens. This recognition event triggers an inflammatory response that normally serves to fight infection; but in some cases can trigger the autoimmune disease lupus. By providing a molecular-level understanding of pathogen recognition; this project will provide some of the necessary tools to create more potent vaccine adjuvants; and a new class of anti-inflammatory therapeutics with a wide range of applications including in particular lupus; asthma; septic shock syndrome and organ transplant rejection.!

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
7R01GM102869-04
Application #
8978926
Study Section
Special Emphasis Panel (ZRG1-IMM-M (08))
Program Officer
Dunsmore, Sarah
Project Start
2012-08-01
Project End
2016-07-31
Budget Start
2015-01-01
Budget End
2015-07-31
Support Year
4
Fiscal Year
2014
Total Cost
$134,374
Indirect Cost
$9,954

  Institution

Name
University of Cambridge
Department
Type
DUNS #
226552610
City
Cambridge
State
Country
United Kingdom
Zip Code
CB2 1-TN

  Publications

Fenwick, Michael K; Li, Yue; Cresswell, Peter et al. (2017) Structural studies of viperin, an antiviral radical SAM enzyme. Proc Natl Acad Sci U S A 114:6806-6811
Prigozhin, Daniil M; Modis, Yorgo (2016) Flunarizine arrests hepatitis C virus membrane fusion. Hepatology 63:14-6
Ryslik, Gregory A; Cheng, Yuwei; Modis, Yorgo et al. (2016) Leveraging protein quaternary structure to identify oncogenic driver mutations. BMC Bioinformatics 17:137
Wong, Emily V; Cao, Wenxiang; Vörös, Judit et al. (2016) P(I) Release Limits the Intrinsic and RNA-Stimulated ATPase Cycles of DEAD-Box Protein 5 (Dbp5). J Mol Biol 428:492-508
Kim, Eunhee; Ilagan, Janine O; Liang, Yang et al. (2015) SRSF2 Mutations Contribute to Myelodysplasia by Mutant-Specific Effects on Exon Recognition. Cancer Cell 27:617-30
Espósito, Danillo L A; Nguyen, Jennifer B; DeWitt, David C et al. (2015) Physico-chemical requirements and kinetics of membrane fusion of flavivirus-like particles. J Gen Virol 96:1702-11
Modis, Yorgo (2015) An Inheritable variant of the innate immune receptor melanoma differentiation-associated gene 5 promotes clearance of hepatitis C virus. Hepatology 61:418-20
Wang, Jimin; Li, Yue; Modis, Yorgo (2014) Structural models of the membrane anchors of envelope glycoproteins E1 and E2 from pestiviruses. Virology 454-455:93-101
Ryslik, Gregory A; Cheng, Yuwei; Cheung, Kei-Hoi et al. (2014) A spatial simulation approach to account for protein structure when identifying non-random somatic mutations. BMC Bioinformatics 15:231
Wang, Jimin; Li, Yue; Modis, Yorgo (2014) Exploiting subtle structural differences in heavy-atom derivatives for experimental phasing. Acta Crystallogr D Biol Crystallogr 70:1873-83

Showing the most recent 10 out of 23 publications