Brucellae are highly infectious intracellular pathogens found in a wide range of mammals causing abortion, infertility and undulant fever. Unlike other intracellular pathogens, Brucella spp. do not encode classical virulent factors. However, chronic intracellular persistence in host cells indicates Brucella effectors likely interact with unidentified eukaryotic targets to modify the cellular environment for bacterial survival. Minimal information is available on Brucella proteins that contribute to bacterial virulence indicating an immediate need to explore the mechanisms of Brucella pathogenesis. This proposal aims to characterize the contribution of a newly identified Brucella protein, termed TcpB encoded by BMEI1674 that contains a TIR domain and mimics properties of the Toll-like receptor adaptor protein TIRAP. TcpB efficiently blocks TLR2 and TLR4 mediated NF-?B activation and plays a significant role in the virulence of the bacterium. Our studies indicated that TcpB interacts with phosphatidylinositols (PtDIns) and co-localizes with the plasma membrane and cytoskeleton network. We hypothesize that TcpB-PtDIns interaction provides TLR specificity for TcpB, but the significance of TcpB-microtubule interaction, mediated by the BB-loop motif of TcpB is unknown. The exact mechanism of TcpB mediated NF-?B suppression is not yet understood, and no information is available on the secretion of TcpB by Brucella and the escape of TcpB from Brucella containing vacuoles. Based on our preliminary studies, TcpB plays a broader role in addition to the suppression of innate immune response. Therefore the present proposal will characterize TcpB in detail to unravel the mechanisms of action and bacterial secretion.
The specific aims of the present proposal are:
Aim 1. To explore the detailed mechanism of TcpB mediated NF-?B suppression. Large-scale yeast-two hybrid screening will analyze TcpB interaction with unidentified mammalian proteins. Positive interactions will be confirmed by co-immunuprecipitation and co-sub-cellular localization experiments.
Aim 2. To analyze the secretion of TcpB by Brucella melitensis and membrane penetration of TcpB. Secretion of TcpB by Brucella.melitensis will be analyzed in culture medium as well as in host cells. Western analysis of concentrated culture supernatant will be performed to test the secretion of TcpB. To analyze the secretion of TcpB inside the cells, a peptide tag-based (GSK-tag) reporter system over expressing TcpB-GSK will be used. To analyze the cell permeability purified TcpB protein will be incubated with mammalian cells and intracellular localized TcpB will be determined by western blotting. A cytokine ELISA will confirm that TcpB can enter host cells as well as demonstrate the suppression of cytokine by intracellular TcpB protein.
Aim 3 : To analyze the effect of TcpB on tubulin polymerization and TcpB mediated activation of small GTPases. To analyze the effect of TcpB on kinetics of tubulin assembly, fluorescent-based tubulin polymerization assays will be performed in the presence of purified TcpB or peptide harboring the BB-loop motif of TcpB that mediates microtubule interaction. The role of intact microtubules for TcpB mediated NF-?B suppression will be analyzed by reporter assays in the presence of the microtubule destabilizing agent nocodazole. To investigate the TcpB mediated activation of small GTPases, GTPase pull-down assays will be performed with the cell lysate transfected with TcpB. Phagocytosis assays will be performed to address whether TcpB mediated membrane ruffles and lamellipodia protrusions enhances phagocytosis. Our Preliminary Studies have identified a B. melitensis TIR domain containing protein, termed TcpB that possesses the ability to alter signaling events in host cells and disrupt innate immune mechanisms. Critical information gained from these specific aims will begin to bridge the gap between what we know about B. melitensis virulence and how virulence is regulated.

Public Health Relevance

Our proposal will determine the effect of a TIR domain containing protein of Brucella melitensis that suppresses NF?B signaling as well as hijack the signaling pathway of Toll-Like Receptor proteins that possess an extracellular leucine-rich domain and a cytoplasmic domain referred to as Toll/IL-1R domain or TIR domain. Brucella spp. encode a TIR domain-containing protein (27 kDa) that can suppress the innate immune responses allowing the bacterium to successfully establish an intracellular niche. We are confident of achieving our project goals based on preliminary data that demonstrate our ability in each specific aim. We will first explore the detailed mechanism of TcpB mediated NF-?B suppression.
This aim will identify the various host proteins that TcpB engages. Second, we will analyze the secretion of TcpB by Brucella melitensis and membrane penetration of TcpB.
This aim will link the mechanism of TcpB transport from the bacterium to the internal environment of the cell. Third, we will analyze the effect of TcpB on tubulin polymerization and TcpB mediated activation of small GTPases.
This aim will identify how TcpB disrupts cell architecture and potentially alters additional host signaling processes. We are confident of achieving these goals based on preliminary data that demonstrate our ability in each specific aim. The Problem: B. melitensis, a Gram-negative facultative intracellular bacterium, induces chronic infectious disease in humans and domestic animals. While an initial framework of several B. melitensis virulence traits has been documented, little is known about the mechanisms used by Brucella virulence associated proteins that permit an intracellular lifestyle. Now, we have preliminary data supporting a role for the Brucella protein TcpB to disrupt the very early steps of host cell response to this pathogen by disrupting the initial signaling events of innate immunity. Thus, pathogenic intracellular Brucella utilize a number of mechanisms to evade macrophage killing. Unfortunately, little is known regarding how any of these Brucella proteins function mechanistically to hijack host intracellular defenses. The Product: Our Preliminary Studies have identified a B. melitensis TIR domain containing protein, termed TcpB that possesses the ability to alter signaling events in host cells and disrupt innate immune mechanisms. Critical information gained from these specific aims will begin to bridge the gap between what we know about B. melitensis virulence and how virulence is regulated.

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Exploratory/Developmental Grants (R21)
Project #
1R21AI088038-01
Application #
7871109
Study Section
Special Emphasis Panel (ZRG1-IDM-A (90))
Program Officer
Mukhopadhyay, Suman
Project Start
2010-02-01
Project End
2012-01-31
Budget Start
2010-02-01
Budget End
2011-01-31
Support Year
1
Fiscal Year
2010
Total Cost
$185,625
Indirect Cost
Name
University of Wisconsin Madison
Department
Veterinary Sciences
Type
Schools of Veterinary Medicine
DUNS #
161202122
City
Madison
State
WI
Country
United States
Zip Code
53715
Splitter, Gary; Harms, Jerome; Petersen, Erik et al. (2014) Studying host-pathogen interaction events in living mice visualized in real time using biophotonic imaging. Methods Mol Biol 1197:67-85
Smith, Judith A; Khan, Mike; Magnani, Diogo D et al. (2013) Brucella induces an unfolded protein response via TcpB that supports intracellular replication in macrophages. PLoS Pathog 9:e1003785
Petersen, Erik; Rajashekara, Gireesh; Sanakkayala, Neelima et al. (2013) Erythritol triggers expression of virulence traits in Brucella melitensis. Microbes Infect 15:440-9
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Eskra, Linda; Covert, Jill; Glasner, Jeremy et al. (2012) Differential expression of iron acquisition genes by Brucella melitensis and Brucella canis during macrophage infection. PLoS One 7:e31747
Petersen, Erik; Chaudhuri, Pallab; Gourley, Chris et al. (2011) Brucella melitensis cyclic di-GMP phosphodiesterase BpdA controls expression of flagellar genes. J Bacteriol 193:5683-91
Radhakrishnan, Girish K; Harms, Jerome S; Splitter, Gary A (2011) Modulation of microtubule dynamics by a TIR domain protein from the intracellular pathogen Brucella melitensis. Biochem J 439:79-83
Radhakrishnan, Girish K; Splitter, Gary A (2010) Biochemical and functional analysis of TIR domain containing protein from Brucella melitensis. Biochem Biophys Res Commun 397:59-63

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