Figure 5
Figure 5. Targeting DC using anti-mClec9A mAb induces potent humoral responses. (A,B) Mice were injected intravenously with either 2 μg (n = 5), 0.4 μg (n = 5), 0.08 μg (n = 5), or 0.016 μg (n = 4) anti-mClec9A mAb (10B4) or with 50 μg (n = 5) and 10 μg (n = 5) of a nontargeting isotype control mAb-1 (eBioscience), or with 50 μg (n = 2) of an in-house isotype control mAb-2 (GL117). Serum anti-rat reactivity was measured by ELISA on week 2 (A) and week 4 (B). Mean titers plus or minus SEM are depicted. The titration experiment was performed twice. The 10-μg dose response represents the cumulative data of 5 experiments (week 2, n = 20; week 4, n = 19). (C) Mice (n = 5) were injected intravenously with 10 μg of either anti-mClec9A mAb or nontargeting isotype control mAb-1 (eBioscience). Serum samples were collected on weeks 2, 4, and 6, after which mice were injected with 10 μg of nontargeting isotype control mAb-2 (GL117). Serum anti–rat Ig reactivity was measured by ELISA on weeks 2, 4, 6, and 8 and is presented as mean titers plus or minus SEM (D) Mice were injected intravenously with 10 μg of either anti-mClec9A mAb (n = 7) or nontargeting isotype control mAb-2 (GL117; n = 4). The isotype of the serum anti–rat Ig reactivity was measured by ELISA on week 4. Bar graphs depict mean titers plus or minus SEM. The experiments were performed twice.

Targeting DC using anti-mClec9A mAb induces potent humoral responses. (A,B) Mice were injected intravenously with either 2 μg (n = 5), 0.4 μg (n = 5), 0.08 μg (n = 5), or 0.016 μg (n = 4) anti-mClec9A mAb (10B4) or with 50 μg (n = 5) and 10 μg (n = 5) of a nontargeting isotype control mAb-1 (eBioscience), or with 50 μg (n = 2) of an in-house isotype control mAb-2 (GL117). Serum anti-rat reactivity was measured by ELISA on week 2 (A) and week 4 (B). Mean titers plus or minus SEM are depicted. The titration experiment was performed twice. The 10-μg dose response represents the cumulative data of 5 experiments (week 2, n = 20; week 4, n = 19). (C) Mice (n = 5) were injected intravenously with 10 μg of either anti-mClec9A mAb or nontargeting isotype control mAb-1 (eBioscience). Serum samples were collected on weeks 2, 4, and 6, after which mice were injected with 10 μg of nontargeting isotype control mAb-2 (GL117). Serum anti–rat Ig reactivity was measured by ELISA on weeks 2, 4, 6, and 8 and is presented as mean titers plus or minus SEM (D) Mice were injected intravenously with 10 μg of either anti-mClec9A mAb (n = 7) or nontargeting isotype control mAb-2 (GL117; n = 4). The isotype of the serum anti–rat Ig reactivity was measured by ELISA on week 4. Bar graphs depict mean titers plus or minus SEM. The experiments were performed twice.

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