(A) Representative micrographs of anti–phospho-GCN2 immunostaining of rat lung sections demonstrating prominent Thr898 phosphorylation-GCN2 (GCN2-Pi) in pulmonary vascular ECs in vehicle-treated MCT rats, which was inhibited in A-92–treated MCT rat lungs. Lung tissue cryosections from basal control rats, vehicle-treated MCT rats (4 weeks), or compound A-92–treated MCT rats were immunostained with anti-Thr898 phospho-GCN2 antibody (red). ECs were immunostained with anti-CD31 (green), and nuclei were counterstained with DAPI (blue). Scale bar, 50 μm. (B) Graphical presentation of the experimental procedure. A-92 (0.5 mg/kg, i.p. daily) was administered to rats at 2 weeks after MCT. (C) RVSP measurement showing a marked increase of RVSP in MCT rats treated with vehicle compared with basal rats, which was reduced in A-92–treated MCT rats. (D) RV hypertrophy evident by increased RV/(LV+S) ratio seen in vehicle MCT rats was reduced in A-92 MCT rats. Basal n = 5, MCT veh n = 10, MCT A92 n = 10. (E) Representative micrographs of Russell-Movat pentachrome staining of rat lung sections showing attenuated vessel wall thickening. Br, bronchiole; V, vessel. (F) Quantification of average pulmonary vessel wall thickness. N = 5/group. MWT, media wall thickness. (G) Representative micrographs of anti–α-SMA (green) staining of basal rat, MCT vehicle rat, and A-92–treated MCT rat lung sections showing reduced number of muscularized distal pulmonary vessels in A-92–treated MCT rat lungs. Nuclei were counterstained with DAPI (blue). Arrows point to muscularized distal pulmonary vessels. (H) Quantification of muscularized distal pulmonary vessels. The total number of α-SMA–positive distal pulmonary vessels (d ≤ 50 μm) of 20× original magnification fields of each section was used for each rat. N = 5–7/group. Arrows point to muscularized vessels. Data are shown as means + SD. Scale bars, 50 μm. **, P < 0.01; ***, P < 0.001; ****, P < 0.0001. One-way ANOVA with Tukey’s multiple comparisons test (C, D, F, and H).