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    The Effect of CC16 on Macrophage Polarization

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    Author
    Bacon, Cory Nicholas
    Issue Date
    2025
    Advisor
    Ledford, Julie
    
    Metadata
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    Publisher
    The University of Arizona.
    Rights
    Copyright © is held by the author. Digital access to this material is made possible by the University Libraries, University of Arizona. Further transmission, reproduction, presentation (such as public display or performance) of protected items is prohibited except with permission of the author.
    Abstract
    Club Cell Secretory Protein (CC16) is a protein that is secreted in the lungs and exhibits protective effects against the development of obstructive lung diseases, altered pulmonary function, airway remodeling, and helps lower pathogenic load in the lungs [3]. Deficiencies in CC16 have been linked to worsened symptoms in asthma [13], rapid decrease of lung function in COPD-like disease in mice [14] and has been linked to increasing airway remodeling in mice [12]. rCC16 has been demonstrated to regulate the expression of pro-inflammatory cytokines via NF-kB. Resident macrophages are known to participate in a variety of these processes, but whether CC16 exerts protective effects in the lung via macrophage-dependent mechanisms remains unknown and was the topic of study in this thesis. Experiments were conducted with RAW 264.7 and immortalized bone marrow derived macrophages (IBMDM) cells to shed light on the effects of CC16 on macrophage polarization. Stimulated RAW 264.7 cells were used to measure M2 polarization in the presence of M2 stimuli with and without rCC16. In these studies, rCC16 had minimal impact on limiting M2 polarization of RAW 264.7 cells at the dose and time point tested. Both RAW 264.7 and IBMDM cells were used to measure gene expression associated with M2 macrophage polarization, including expression of genes for IL-10, IL-13, Arg1, and PPAR-G. Major findings were that in RAW 264.7 cells, IL-10 was significantly upregulated by rCC16 alone and PPAR-G was significantly downregulated by rCC16 in the presence of IL-4+IL-13. In IBMDM cells, rCC16 has less impact on M2 gene expression resulting from IL-4 stimulation, however, rCC16 alone and in the presence of IL-4, also increased IL-10 gene expression.
    Type
    text
    Electronic Thesis
    Degree Name
    M.S.
    Degree Level
    masters
    Degree Program
    Graduate College
    Cellular and Molecular Medicine
    Degree Grantor
    University of Arizona
    Collections
    Master's Theses

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