Abstract

This application is submitted in response to the broad challenge area of Translational Science (15-ES-101*) and the specific challenge topic of """"""""Effects of environmental exposures on phenotypic outcomes using non- human models."""""""" Chronic inflammatory diseases of the airways such as asthma or chronic obstructive pulmonary disease (COPD) arise from a complex interaction between genetic factors and environmental exposures. Our laboratory has established murine models that mimic the pathology of ozone (O3)-induced exacerbation of airway inflammation. The current application will utilize this model together with gene knockout and conditional over expressor mice to investigate the importance in changes in gene expression and post translational modifications of surfactant protein D, an immunoprotective component of the proximal and distal airway lining. Our studies showed that inhalation of O3, a common air pollutant, induced a significant exacerbation of the asthmatic changes in allergen sensitized mice together with the appearance of abnormal, trimeric SP-D and activated, myeloid dendritic cells. We hypothesize that SP-D acts as a """"""""master switch"""""""" between the onset and resolution of airway inflammation: Native SP-D is a suppressor of activation of the proinflammatory dendritic cells and acts through the C-terminal by binding to the negative signal receptor SIRP. In contrast, a de-oligomerized (trimeric) SP-D that has undergone oxidative damage by O3, activates dendritic cells through the exposed N-terminal by ligating the collagen receptor, calreticulin/CD91. The asthmatic airways are particularly susceptible to O3-induced changes in the SP-D molecule because of the presence of mature myeloid dendritic cells carrying the calreticulin/CD91.
Aim 1 is to investigate the hypothesis that O3-induced exacerbation of allergic airway inflammation is associated with the appearance of SP-D trimers with an active N-terminal domain.
Aim 2 is to study the hypothesis that native SP-D binds to SIRP? and delivers inhibitory signals while trimeric SP-D binds to calreticulin/CD91 and induces proinflammatory activation of NF-kB, TNF and TARC (Ccl17) release by dendritic cells.
Aim 3 is to investigate whether the C- terminal suppresses and the trimeric SP-D activates epithelial migration of bone marrow derived, proinflammatory dendritic cells. In vitro bone-marrow derived dendritic cell cultures and in vivo conditional SP-D expressing mice and adeno-associated virus gene replacement of wild-type and mutant SP-D (mimicking either the C-terminal of the molecule or the SP-D trimer) will be studied for maturation and migration of dendritic cells. Results of this project will yield clinically and scientifically significant information on the role of SP-D in regulation of the innate immune system during O3-induced airway changes and on potential therapeutic utilization of this naturally occurring immuno-protective agent in the lung.

Public Health Relevance

Air pollution, particularly O3, induces exacerbations of asthma that substantially worsen morbidity and mortality. In healthy individuals inhalation of O3 elicits mechanisms such as homeostatic increase in SP-D synthesis that protect the lung from development of chronic damage. Currently neither the mechanism of O3-induced SP-D production nor the consequent alterations of the pulmonary immune system is understood. Results from this application will define the implications of SP-D in O3-induced exacerbation of asthma and will provide novel approaches to manipulate the pulmonary immune system.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Environmental Health Sciences (NIEHS)
Type
NIH Challenge Grants and Partnerships Program (RC1)
Project #
1RC1ES018505-01
Application #
7818195
Study Section
Special Emphasis Panel (ZRG1-IMM-E (58))
Program Officer
Nadadur, Srikanth
Project Start
2009-09-28
Project End
2011-06-30
Budget Start
2009-09-28
Budget End
2010-06-30
Support Year
1
Fiscal Year
2009
Total Cost
$500,000
Indirect Cost

  Institution

Name
University of Pennsylvania
Department
Internal Medicine/Medicine
Type
Schools of Medicine
DUNS #
042250712
City
Philadelphia
State
PA
Country
United States
Zip Code
19104

  Publications

Yousefi, Shida; Sharma, Satish K; Stojkov, Darko et al. (2018) Oxidative damage of SP-D abolishes control of eosinophil extracellular DNA trap formation. J Leukoc Biol 104:205-214
Ge, Moyar Qing; Kokalari, Blerina; Flayer, Cameron H et al. (2016) Correction: Cutting Edge: Role of NK Cells and Surfactant Protein D in Dendritic Cell Lymph Node Homing: Effects of Ozone Exposure. J Immunol 196:3212
Yang, Qi; Ge, Moyar Q; Kokalari, Blerina et al. (2016) Group 2 innate lymphoid cells mediate ozone-induced airway inflammation and hyperresponsiveness in mice. J Allergy Clin Immunol 137:571-8
Wang, Yuan; Miwa, Takashi; Ducka-Kokalari, Blerina et al. (2015) Properdin Contributes to Allergic Airway Inflammation through Local C3a Generation. J Immunol 195:1171-81
Fang, C L; Yin, L J; Sharma, S et al. (2015) Resistin-like molecule-? (RELM-?) targets airways fibroblasts to effect remodelling in asthma: from mouse to man. Clin Exp Allergy 45:940-952
Jordan, Martha; Haczku, Angela (2013) Autoreactive bronchus-associated lymphoid tissue in interstitial lung disease: friend or foe? Am J Respir Cell Mol Biol 48:397-8
Haczku, Angela (2012) The dendritic cell niche in chronic obstructive pulmonary disease. Respir Res 13:80
Sziksz, Erna; Vannay, Adám; Haczku, Angela (2012) Galectin-9: a suppressor of food allergy? Allergy 67:293-5
Anderson, Amy L; Zheng, Yi; Song, Decheng et al. (2012) The B-cell superantigen Finegoldia magna protein L causes pulmonary inflammation by a mechanism dependent on MyD88 but not B cells or immunoglobulins. Inflamm Res 61:161-9
Sharma, S K; Almeida, F A; Kierstein, S et al. (2012) Systemic FasL neutralization increases eosinophilic inflammation in a mouse model of asthma. Allergy 67:328-35

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