(A) Study design of murine DSS-induced colitis model with prophylactic anti-DCIR mAbs treatment. huDCIR-KI mice were i.p. injected with 10 mpk anti-DCIR mAbs (9D9, 3F7) or isotype control (n = 5/antibody-treated group) on day 0 and 3 during the 7 days long 3%DSS water feeding period. (B) Body weight change of the mice treated with indicated antibodies during the DSS-colitis phase. Weight is presented relative to the initial body weight before DSS-water feeding. (C) Representative confocal laser endoscopy (CLE) image of the colonic crypts (green, labeled by Acriflavine) with infiltrated inflammatory neutrophils (red, labeled by NE680) from mice received 3%DSS for 7 days with different colitis severity. (D and E) Representative CLE image of colonic crypts with associated neutrophil activation score indicated by the NE680 staining (D), and representative H&E-stained colons (E) with associated histology score of the mice received anti-DCIR mAbs and isotype control treatment as illustrated in A. Scale bars: 20 μm for D and 100 μm for E. M, mucosal gland; SM, submucosa; TME, tunica muscularis externa; thin arrows, erosion; thick arrows, inflammatory cells; **, gland loss. (F) MIP-2 cytokine level in mice serum collected on day7 after the DSS-colitis. Data are normalized to isotype group. Each data point represents the individual mouse treated with indicated condition. Means ± SEM are shown, and statistical significance is determined by 1-way ANOVA test with Dunnett’s correction for multiple comparison to the isotype treated condition. *P < 0.05, ***P < 0.001.