Emphysema is an important pathologic finding in Chronic Obstructive Lung Disease (COPD), a leading cause of death in the United States and worldwide. Emphysema is characterized by increased DNA damage and the consequences of failed DNA repair: apoptosis, cellular senescence, and inflammation. Cigarette smoke (CS) is the most important etiology for DNA damage in emphysema. Yet, emphysema does not occur universally among smokers and there is little understanding of protective mechanisms that underlie this heterogeneity. Therefore, identifying cellular responses to CS that promote DNA repair may lead to new therapies for this disease. This proposal seeks to understand the role of Macrophage Migration Inhibitory Factor (MIF) in promoting DNA repair and antagonizing the development of emphysema. MIF is a cytokine secreted in response to CS and a critical regulator of multiple signaling pathways. We previously demonstrated that circulating MIF is decreased in patients with COPD, and genetic deletion of murine MIF results in increased susceptibility to CS mediated airspace enlargement. The endothelial cells of MIF-KO mice are particularly susceptible to CS-mediated DNA damage and consequent apoptosis and cellular senescence. The source of protective MIF is unknown. Our preliminary data suggests that MIF promotes DNA repair in endothelial cells exposed to CS extract and that endothelial cells may be an importance source of protective MIF. Based on these findings, we propose the following hypotheses and specific aims: Hypotheses 1. MIF, via its receptor CD74, promotes HR and NHEJ following CS-mediated DNA damage. 2. MIF, via CD74, protects lung endothelial cells from CS-mediated cellular senescence and apoptosis by promoting BRCA1 gene expression. 3. Deletion of MIF in the endothelium is necessary and sufficient to increase murine susceptibility to DNA damage and emphysema.
Aims 1. Define the DNA repair mechanism(s) promoted by MIF in lung endothelial cells. 2. Determine the role of BRCA1 in mediating MIF's protective effect. 3. Define the protective role of endothelial-derived MIF in CS-mediated emphysema. Experimental Approach To address Aim 1, we will use primary mouse and human endothelial cells and expose them to CS extract, followed by a recovery period to observe DNA repair. We will characterize DNA damage and repair using single- cell gel electrophoresis, imaging-flow cytometry (Amnis) and host cell reactivation assays. We will use silencing RNA and chemical inhibitors of MIF-CD74 binding to determine if MIF promotes DNA repair via its receptor CD74.
In Aim 2, we will characterize the effects of CS on BRCA1 gene expression and protein in primary lung endothelial cells and paraffin-embedded, de-identified human lung tissue samples. We will use chromatin precipitation assays to determine the mechanism via which MIF promotes BRCA1 gene expression, and we will measure consequences of CS extract in endothelial cells, such as apoptosis and cellular senescence, to determine if MIF protects against these consequences in a BRCA1-dependent manner. We will use silencing RNA and chemical inhibitors of MIF-CD74 binding to determine if MIF promotes BRCA1 gene expression in a CD74-dependent manner.
In Aim 3, we will assess the development of emphysema in mice exposed to CS with an endothelial specific deletion of MIF. We will also determine if an endothelial-specific lentiviral vector expressing MIF can rescue the susceptibility of MIF-KO mice to CS. This work will provide us with insight into the pathogenesis of emphysema in addition to the novel regulatory functions of MIF in promoting DNA repair. This grant proposes a research mentorship program at Yale University under the primary sponsorship of Dr. Richard Bucala, an expert in immunology and MIF biology, and Dr. Patty Lee, an expert in oxidant-mediated vascular injury and repair in the lungs as co-mentor. We have also enlisted the expertise of multiple Yale investigators, including two experts in DNA repair research, Dr. Joann Sweasy and Dr. Peter Glazer, Dr. Naftali Kaminski, who is an expert on translational pulmonary research, and Dr. Veronique Neumeister, who has significant expertise in immunohistology. The advisory committee members will provide scientific and career counseling, and the proposed career and research program as outlined will provide an extraordinary scientific environment wherein Dr. Sauler can launch his future independent career as a physician- scientist.

Public Health Relevance

Chronic Obstructive Pulmonary Disease (COPD) is the third leading cause of death in the United States, yet there are few effective therapies for this disease. Chronic exposure to cigarettes smoke is the most important risk factor for COPD, but most current or former smokers never develop this disease and there is little understanding of the host response to cigarette smoke that protects against disease development. We have identified the protein Macrophage Migration Inhibitory Factor (MIF) as a stress-response protein that protects against the development of emphysema, and this proposal seeks to understand the mechanisms via which MIF mediates its protective effect.

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Clinical Investigator Award (CIA) (K08)
Project #
5K08HL135402-02
Application #
9406886
Study Section
NHLBI Mentored Clinical and Basic Science Review Committee (MCBS)
Program Officer
Tigno, Xenia
Project Start
2017-01-01
Project End
2021-12-31
Budget Start
2018-01-01
Budget End
2018-12-31
Support Year
2
Fiscal Year
2018
Total Cost
Indirect Cost
Name
Yale University
Department
Internal Medicine/Medicine
Type
Schools of Medicine
DUNS #
043207562
City
New Haven
State
CT
Country
United States
Zip Code
Pellowe, Amanda S; Sauler, Maor; Hou, Yue et al. (2018) Endothelial cell-secreted MIF reduces pericyte contractility and enhances neutrophil extravasation. FASEB J :fj201800480R
Sauler, Maor; Lamontagne, Maxime; Finnemore, Eric et al. (2018) The DNA repair transcriptome in severe COPD. Eur Respir J 52: