(A) Colons from C57BL/6J mice were used to purify intestinal epithelial cells (IECs) and lamina propria lymphocytes (LPLs), and expression of miR147 was analyzed by qPCR. (B) Comparison of miR147 expression levels in ileal and colonic IECs derived from miR147tdTomato and C57BL/6J mice by qPCR. miR147tdTomato reporter mice were used to map miR147 expression within the large intestine. (C) Representative image of the luminal surface of the colon showing fluorescent tdTomato expression. (D) Portion of the lamina propria with remaining colonic crypts showing miR147 expression localized to the upper (luminal) portion of the crypts. Black arrows indicate the stem cell areas that lack reporter expression. (E) Purified intact colonic crypts visualized under differential interference contrast (DIC) and fluorescent light; yellow arrows indicate the luminal portion of the crypts with visible tdTomato expression. (F–I) Validation of tdTomato expression in miR147tdTomato mice using fluorescent staining. Frozen intestinal sections were stained with primary anti-tdTomato and secondary (Alexa Fluor 488, AF488) and visualized by confocal microscopy. (F) Medial colon. (G) Proximal colon. Both panels show overlays of miR147tdTomato colon stained with anti-tdTomato/secondary and DAPI, with AF488 fluorescence shown in the right panels. (H) Overlay of secondary AF488 and DAPI (left) and secondary alone (right). (I) C57BL/6J medial colon, showing overlay of anti-tdTomato/secondary and DAPI (left) and anti-tdTomato/secondary alone (right). In A and B, n = 3 mice/group; pooled, expression normalized to U6 snRNA; data presented as mean ± SEM. **P < 0.01 by unpaired t test (A) or 2-way ANOVA with Šídák’s test (B). In C–I, experiments repeated at least 3 times. Both male and female mice were used. Scale bars: 200 μm (C), 50 μm (D and E), and 100 μm (F–I).