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Michael T. Borchers, Scott C. Wesselkamper, Victor Curull, Alba Ramirez-Sarmiento, Albert Sánchez-Font, Judith Garcia-Aymerich, Carlos Coronell, Josep Lloreta, Alvar G. Agusti, Joaquim Gea, John A. Howington, Michael F. Reed, Sandra L. Starnes, Nathaniel L. Harris, Mark Vitucci, Bryan L. Eppert, Gregory T. Motz, Kevin Fogel, Dennis W. McGraw, Jay W. Tichelaar, Mauricio Orozco-Levi
Published in Volume 119, Issue 3
J Clin Invest. 2009; 119(3):636–649 doi:10.1172/JCI34462
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Figure 2
In Raet1a Tg mice, inducible expression of RAET1 on pulmonary epithelial cells leads to pulmonary emphysema.

(A) Lymphocyte populations in digested whole lungs of mice given DOX for the indicated times were quantitated by flow cytometry using antibodies specific for the indicated cell surface markers. Data are results of 3 independent experiments using pooled samples from at least 3 mice per group. Inflammatory cells in the lung were assessed by enumeration of cell differentials in the BAL (n = 5 per group). (B) H&E-stained lung sections from mice that were left untreated, administered DOX for 5, 15, 30, and 60 d, or administered 30 d DOX concurrently with an NKG2D blocking antibody. Photomicrographs are representative of 5 mice per group. Scale bar: 100 μm. (C) Time course of alveolar destruction, quantified as mean linear intercept. (DF) Mice were administered DOX for 60 d, and static compliance (D), dynamic compliance (E), and pressure-volume loops (F) were determined using a forced oscillation technique. These functional indicators of elastic recoil loss reflect the ease with which the lung distends. Values are mean ± SD (n = 3–5 per group). (G) Specificity for NKG2D-mediated effects (n = 5 per group). Lymphocyte populations were specifically depleted as described in Methods, and mean linear intercept was assessed after 30 d DOX treatment. *P < 0.05 versus respective no DOX control.