Abstract

Mammals have evolved a number of innate immune defense mechanisms to detect microbial infection and protect the host. Previous studies of have demonstrated that intracellular multiprotein complexes, called inflammasomes, are important for host defense against infections. Inflammasomes sense infectious or noxious stimuli and activate effector proteases caspase-1 (casp-1) and caspase-11 (casp-11). Casp-1 processes pro- inflammatory cytokines IL-1band IL-18 to contribute to pathogen control. Casp-11 detects cytosolic lipopolysaccharide (LPS) and activates a pro-inflammatory cell death pathway termed pyroptosis when host cells are infected with Gram-negative pathogens or during septic shock induced by LPS. An increased understanding of how casp-11 is regulated during Gram-negative bacterial infections is necessary in order to develop new therapeutics to treat these infections. We have used Salmonella enterica serovars, which cause diseases ranging from self-limited gastroenteritis (e.g., S. Typhimurium) to systemic infections (e.g., S. Typhi) in humans, as a model Gram-negative pathogen to elucidate the molecular mechanisms of inflammasome activation. We have shown that intracellular S. Typhimurium (Stm) induce casp-11-dependent macrophage death, which is due to leakage of LPS from the Salmonella containing vacuole (SCV) into the macrophage cytosol. In ongoing experiments, we have found that casp-11 is regulated by both host and pathogen factors. Our preliminary data show that: (1) mouse complement factors regulate casp-11 gene expression, (2) two different casp-11 transcript variants, in addition to the full-length transcript, occur in macrophages treated with LPS, and (3) at least one Stm virulence factor that is translocated into host cells by a type 3 secretion system (T3SS) dampens the activation of casp-11 inflammasomes. These data suggest that the innate immune detection of intracellular Gram-negative bacteria and LPS that leads to casp-11 activation is regulated by the host at multiple levels (e.g., gene transcription, multiple casp-11 variants) and by Stm virulence factors. Given these findings, we hypothesize that specific host proteins direct casp-11 cell death and that Salmonella virulence factors modulate casp-11 activation. These hypotheses will be addressed in the experiments of the following Specific Aims: (1) identify host molecules and pathways involved in casp-11-dependent cell death, (2) characterize the expression and function of casp-11 transcript variants in the context of bacterial infection, and (3) identify Salmonella factors that impact casp-11-dependent cell death. The result of this study will lead to the identification and characterization of new host and bacterial factors that regulate casp-11 during bacterial infections. These findings may lead to novel therapeutics for the treatment of infections with Gram-negative pathogens and sepsis.

Public Health Relevance

These exploratory studies are relevant to public health for two reasons. First, they may provide new host pathways to target during systemic infections with Gram-negative bacterial pathogens or during sepsis, Secondly, they may lead to the development of new classes of antibiotics to treat bacterial infection.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
2R01AI095396-06
Application #
9222645
Study Section
Special Emphasis Panel (ZRG1)
Program Officer
Alexander, William A
Project Start
2011-12-01
Project End
2021-06-30
Budget Start
2017-07-19
Budget End
2018-06-30
Support Year
6
Fiscal Year
2017
Total Cost
Indirect Cost

  Institution

Name
Stanford University
Department
Microbiology/Immun/Virology
Type
Schools of Medicine
DUNS #
009214214
City
Stanford
State
CA
Country
United States
Zip Code
94304

  Publications

Yokoyama, Christine C; Baldridge, Megan T; Leung, Daisy W et al. (2018) LysMD3 is a type II membrane protein without an in vivo role in the response to a range of pathogens. J Biol Chem 293:6022-6038
Napier, Brooke A; Monack, Denise M (2017) Editorial: The sum of all defenses: tolerance + resistance. Pathog Dis 75:
Napier, Brooke A; Monack, Denise M (2017) Creating a RAW264.7 CRISPR-Cas9 Genome Wide Library. Bio Protoc 7:
Sastalla, Inka; Monack, Denise M; Kubatzky, Katharina F (2016) Editorial: Bacterial Exotoxins: How Bacteria Fight the Immune System. Front Immunol 7:300
Napier, Brooke A; Brubaker, Sky W; Sweeney, Timothy E et al. (2016) Complement pathway amplifies caspase-11-dependent cell death and endotoxin-induced sepsis severity. J Exp Med 213:2365-2382
Napier, Brooke A; Monack, Denise M (2016) IMMUNOLOGY. A lipid arsenal to control inflammation. Science 352:1173-4
Kortmann, Jens; Brubaker, Sky W; Monack, Denise M (2015) Cutting Edge: Inflammasome Activation in Primary Human Macrophages Is Dependent on Flagellin. J Immunol 195:815-9
Storek, Kelly M; Monack, Denise M (2015) Bacterial recognition pathways that lead to inflammasome activation. Immunol Rev 265:112-29
Storek, Kelly M; Gertsvolf, Nina A; Ohlson, Maikke B et al. (2015) cGAS and Ifi204 cooperate to produce type I IFNs in response to Francisella infection. J Immunol 194:3236-45
Carden, Sarah; Okoro, Chinyere; Dougan, Gordon et al. (2015) Non-typhoidal Salmonella Typhimurium ST313 isolates that cause bacteremia in humans stimulate less inflammasome activation than ST19 isolates associated with gastroenteritis. Pathog Dis 73:

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