(A) Representative H&E-stained images of WT and TG^cog/cog thyroids (n = 6 animals/group), showing thyrocyte distention with apically displaced nuclei in TG^cog/cog mice compared with a thin monolayer of thyrocytes in WT (^+/+) mice. Scale bars: 20 μm. (B) Representative anti-Tg immunofluorescence in thyroid glands of WT and TG^cog/cog mice (n = 8 animals/group), with DAPI counterstain. Scale bars: 20 μm. (C) Representative immunofluorescence of T4-containing protein in thyroid follicles of WT or TG^cog/cog mice (n = 6 animals/group). Thyrocytes are highlighted by PAX8-positive nuclear transcription factor with DAPI counterstain. Scale bars: 10 μm. (D) Endoglycosidase H digest of thyroid homogenates before SDS-PAGE and Tg Western blotting from WT and TG^cog/cog mice (n = 3 animals/group; 2 of each kind shown). R, endoglycosidase H resistant; S, endoglycosidase H sensitive. (E) Top: Western blotting of BiP, p58ipk, and CHOP in the thyroids of TG^cog/cog mice (n = 3–4; each lane represents 1 animal). Bottom: Quantitation of bands (normalized to tubulin), shown as mean ± SD. ***P < 0.001 (unpaired 2-tailed Student’s t test). (F) Representative TUNEL staining and immunofluorescence of T4-containing protein with DAPI counterstain in thyroid sections of WT and TG^cog/cog mice (n = 7 animals/group). For clarity, in the merged image from TG^cog/cog mice, a dashed white line delimits the thyroid follicle lumen. Scale bars: 20 μm. (G) Thyroid homogenate from TG^cog/cog mice (n = 3) was immunoprecipitated with mAb anti-T4 in the presence or absence of T4 competitor, followed by either mock digest or Endo H digest and SDS-PAGE plus immunoblotting with mAb antibody that recognizes intact Tg. As a positive control, WT Tg secreted from PCCL3 (rat) thyrocytes was digested for Endo H resistance. The T4-containing Tg protein of TG^cog/cog mice was entirely Endo H sensitive. The position of the 250 kDa molecular weight marker is shown.