Alveolar repair following LPS-induced injury requires cell-ECM interactions
Jennifer M.S. Sucre, Fabian Bock, Nicholas M. Negretti, John T. Benjamin, Peter M. Gulleman, Xinyu Dong, Kimberly T. Ferguson, Christopher S. Jetter, Wei Han, Yang Liu, Seunghyi Kook, Jason J. Gokey, Susan H. Guttentag, Jonathan A. Kropski, Timothy S. Blackwell, Roy Zent, Erin J. Plosa
Jennifer M.S. Sucre, Fabian Bock, Nicholas M. Negretti, John T. Benjamin, Peter M. Gulleman, Xinyu Dong, Kimberly T. Ferguson, Christopher S. Jetter, Wei Han, Yang Liu, Seunghyi Kook, Jason J. Gokey, Susan H. Guttentag, Jonathan A. Kropski, Timothy S. Blackwell, Roy Zent, Erin J. Plosa
View: Text | PDF
Research Article Cell biology Pulmonology

Alveolar repair following LPS-induced injury requires cell-ECM interactions

Abstract

During alveolar repair, alveolar type 2 (AT2) epithelial cell progenitors rapidly proliferate and differentiate into flat AT1 epithelial cells. Failure of normal alveolar repair mechanisms can lead to loss of alveolar structure (emphysema) or development of fibrosis, depending on the type and severity of injury. To test if β1-containing integrins are required during repair following acute injury, we administered E. coli lipopolysaccharide (LPS) by intratracheal injection to mice with a postdevelopmental deletion of β1 integrin in AT2 cells. While control mice recovered from LPS injury without structural abnormalities, β1-deficient mice had more severe inflammation and developed emphysema. In addition, recovering alveoli were repopulated with an abundance of rounded epithelial cells coexpressing AT2 epithelial, AT1 epithelial, and mixed intermediate cell state markers, with few mature type 1 cells. AT2 cells deficient in β1 showed persistently increased proliferation after injury, which was blocked by inhibiting NF-κB activation in these cells. Lineage tracing experiments revealed that β1-deficient AT2 cells failed to differentiate into mature AT1 epithelial cells. Together, these findings demonstrate that functional alveolar repair after injury with terminal alveolar epithelial differentiation requires β1-containing integrins.

Authors

Jennifer M.S. Sucre, Fabian Bock, Nicholas M. Negretti, John T. Benjamin, Peter M. Gulleman, Xinyu Dong, Kimberly T. Ferguson, Christopher S. Jetter, Wei Han, Yang Liu, Seunghyi Kook, Jason J. Gokey, Susan H. Guttentag, Jonathan A. Kropski, Timothy S. Blackwell, Roy Zent, Erin J. Plosa

×

Figure 1

Deletion of β1 integrin in AT2 cells results in increased inflammation, abnormal repair, and decreased survival after LPS-induced injury.

Options: View larger image (or click on image) Download as PowerPoint
Deletion of β1 integrin in AT2 cells results in increased inflammation, ...
(A) Representative images of lung histology demonstrate increased edema at 3 and 7 days postinjury in β1AT2-KO lungs compared with β1fl/fl lungs, as well as persistent inflammation and emphysematous remodeling in β1AT2-KO lungs by 21 days post-LPS. D3, D7, and D21 refer to 3, 7, and 21 days after LPS injury, respectively. (B) Mean linear intercept quantified emphysematous alveolar remodeling at 21 days after LPS, 28.5 ± 0.9 μm in β1fl/fl lungs versus 40.2 ± 2.8 μm in β1AT2-KO lungs (n = 6–7 mice/group, P = 0.0014 by 2-tailed t test). (C) Bicinchoninic acid (BCA) protein assay quantified increased bronchoalveolar lavage (BAL) fluid protein in uninjured β1AT2-KO lungs and at 3 and 7 days post-LPS injury in β1AT2-KO lungs compared with β1fl/fl lungs at the same time points (n = 6–14 mice/group, 2-tailed t test comparing genotypes at each time point, P = 0.0485 for uninjured mice; P = 0.0036 at D3; P = 0.005 at D7; P = 0.2628 at D21). (D) BAL cell counts are significantly increased in β1AT2-KO lungs compared with β1fl/fl littermates in uninjured mice and at 7 and 21 days post-LPS. Peak inflammation is present at 7 days in β1AT2-KO lungs, 55,663 ± 3,306 cells/mL in β1fl/fl BAL fluid versus 624,000 ± 118,753 cells/mL in β1AT2-KO BAL (n = 6–26 mice/group, 2-tailed t test comparing genotypes at each time point, P = 0.0002 for uninjured mice; P = 0.0730 at D3; P = 0.0007 at D7; P < 0.0001 at D21). Total numbers of BAL fluid macrophages are significantly increased in uninjured β1AT2-KO mice and at D7 and D21; lymphocytes and neutrophils are significantly increased in β1AT2-KO BAL at D7 only. Scale bar = 50 μm for A. * P < 0.05.