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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 3
Transgenic overexpression of NKG2D ligands induces epithelial cell apoptosis and CTL activation.

(A) Effector caspase expression in lungs of Raet1a Tg mice administered 30 d DOX was assessed by Casp3/7 bioactivity in whole lung homogenates (n = 5 per group). (B) Apoptotic cell accumulation in the lungs was assessed by immunohistochemistry on paraffin-embedded sections using a rabbit antibody specific for active Casp3. The number of active Casp3+–stained cells was quantified from photomicrographs of lung sections and presented as mean ± SD cells per high-power field (hpf). (C) CTL effector function was induced by NKG2D ligand expression in vivo. Western blot analysis on whole lung homogenates using a granzyme B–specific antibody showed increased protein expression after NKG2D ligand induction in pulmonary epithelial cells. (D) MMP2 and MMP9 activity were not altered in the lungs of mice ectopically expressing RAET1. Gelatin zymography was conducted on lung homogenates of Raet1a Tg mice left untreated (n = 2) or treated with 30 d DOX (n = 3). Photomicrograph is representative of results obtained from 4–6 mice per group. (E) Transcript levels for MMP inhibitors Mmp12 and Mmp14 were not altered in the lungs of mice ectopically expressing RAET1. Real-time quantitative PCR was performed on RNA isolated from the lungs of Raet1a Tg mice left untreated or treated with 30 d DOX (n = 5 per group). *P < 0.05 versus no DOX control.