Figure 5
Figure 5. Resistance to metastatic disease and MDSC regression require FasL. (A) Resistance to metastatic disease requires host cell expression of FasL. BALB/c, FasL−/−, STAT6−/−, CD1−/−, CD1−/−FasL−/−, and STAT6−/−FasL−/− mice were inoculated on day 0 in the mammary gland with 7000 4T1 tumor cells. Primary tumors were removed 3-4 weeks later when metastatic disease was established, and mice were followed after surgery for survival. Numbers indicate the number of mice surviving > 247 days/total number of mice/group. Data are the pooled results of 2 independent experiments. (B) FasL−/− mice contain elevated levels of MDSCs. Data are the average + SD of 5 mice/group. (C) MDSC regression requires host cell expression of FasL. The BALB/c, FasL−/−, STAT6−/−, CD1−/−, CD1−/−FasL−/−, and STAT6−/−FasL−/− mice of Figure 5A were bled 10-12 days after removal of their primary tumors, and the percentage of Gr1+CD11b+ MDSCs in the blood was determined by flow cytometry. Dotted line represents the average percentage of Gr1+CD11b+ cells in the blood of tumor-free mice; solid lines represent the average percentage of Gr1+CD11b+ cells in each group. Each ○ represents an individual mouse. Data are pooled from 2 independent experiments. (D) Gr1+CD11b+ cells from postsurgery BALB/c, FasL−/−, STAT6−/−FasL−/−, and CD1−/−FasL−/− mice are equally suppressive. Gr1+CD11b+ cells from the peripheral blood of 4T1 tumor–bearing mice were cocultured with DO11.10 splenocytes and cognate (OVA323-339) peptide. T-cell activation was assessed by 3H-thymidine incorporation. Average +SD of 4 independent experiments for BALB/c and 2 independent experiments for FasL−/−, CD1−/−FasL−/−, and STAT6−/−FasL−/−mice. (E) Postsurgery resistance to 4T1-induced metastatic disease is perforin dependent. BALB/c, FasL−/−, and Pfp−/− mice were inoculated on day 0 in the abdominal mammary gland with 7000 4T1 tumor cells. Primary tumors were removed 3-4 weeks later when metastatic disease was established, and mice were followed after surgery for survival. Data are pooled from 5 independent experiments for BALB/c (n = 27 mice) and from 3 independent experiments for Pfp−/− and FasL−/− mice (n = 10 mice for each group). Pfp−/− mice survived significantly shorter than wild-type and FasL−/− mice (P < .01 by log-rank test). (F) FasL is required for MDSC reduction. BALB/c, Pfp−/−, FasL−/−, STAT6−/−Pfp−/−, and STAT6−/−FasL−/− mice were inoculated in the abdominal mammary gland with 7000 4T1 tumor cells. When primary tumors were 4-5 mm in diameter, the mice were bled, and the percentage of Gr1+CD11b+ MDSCs in the peripheral blood was determined by flow cytometry. *Statistically significantly different groups (P < .05); Average +SD of 3 mice/group. (G) MDSCs apoptose in vivo in response to activated T cells. DO11.10 transgenic mice were injected subcutaneously on day 0 with cognate peptide (OVA323-339) or irrelevant peptide (HA110-119). Splenocytes were collected on day 3, depleted for RBCs, and stained for Gr1, CD11b, and cleaved caspase3 or for CD4, DO11.10 TcR, and CD69. (Top) Gated Gr1+CD11b+ and CD4+DO11.10+ cells from representative individual mice; (bottom) percentage of CD11b+Gr1+cleaved caspase3+ and percentage of activated (CD69+) CD4+DO11.10+ cells. Average +SD of 5 mice/group. Data are from 1 of 2 independent experiments. (H) Fas+/+ but not Fas−/− MDSCs apoptose in vivo in response to activated T cells. C57BL/6 Fas+/+ and Fas−/− mice were adoptively transferred with CD8+ OT-1 T cells and challenged subcutaneously with cognate peptide. Splenocytes were harvested on day 3 and analyzed according to Figure 5G for percentage of caspase3+ MDSCs and for percentage of activated (CD69+) OT-1 T cells. Average +SD of 4 mice/group.

Resistance to metastatic disease and MDSC regression require FasL. (A) Resistance to metastatic disease requires host cell expression of FasL. BALB/c, FasL−/−, STAT6−/−, CD1−/−, CD1−/−FasL−/−, and STAT6−/−FasL−/− mice were inoculated on day 0 in the mammary gland with 7000 4T1 tumor cells. Primary tumors were removed 3-4 weeks later when metastatic disease was established, and mice were followed after surgery for survival. Numbers indicate the number of mice surviving > 247 days/total number of mice/group. Data are the pooled results of 2 independent experiments. (B) FasL−/− mice contain elevated levels of MDSCs. Data are the average + SD of 5 mice/group. (C) MDSC regression requires host cell expression of FasL. The BALB/c, FasL−/−, STAT6−/−, CD1−/−, CD1−/−FasL−/−, and STAT6−/−FasL−/− mice of Figure 5A were bled 10-12 days after removal of their primary tumors, and the percentage of Gr1+CD11b+ MDSCs in the blood was determined by flow cytometry. Dotted line represents the average percentage of Gr1+CD11b+ cells in the blood of tumor-free mice; solid lines represent the average percentage of Gr1+CD11b+ cells in each group. Each ○ represents an individual mouse. Data are pooled from 2 independent experiments. (D) Gr1+CD11b+ cells from postsurgery BALB/c, FasL−/−, STAT6−/−FasL−/−, and CD1−/−FasL−/− mice are equally suppressive. Gr1+CD11b+ cells from the peripheral blood of 4T1 tumor–bearing mice were cocultured with DO11.10 splenocytes and cognate (OVA323-339) peptide. T-cell activation was assessed by 3H-thymidine incorporation. Average +SD of 4 independent experiments for BALB/c and 2 independent experiments for FasL−/−, CD1−/−FasL−/−, and STAT6−/−FasL−/−mice. (E) Postsurgery resistance to 4T1-induced metastatic disease is perforin dependent. BALB/c, FasL−/−, and Pfp−/− mice were inoculated on day 0 in the abdominal mammary gland with 7000 4T1 tumor cells. Primary tumors were removed 3-4 weeks later when metastatic disease was established, and mice were followed after surgery for survival. Data are pooled from 5 independent experiments for BALB/c (n = 27 mice) and from 3 independent experiments for Pfp−/− and FasL−/− mice (n = 10 mice for each group). Pfp−/− mice survived significantly shorter than wild-type and FasL−/− mice (P < .01 by log-rank test). (F) FasL is required for MDSC reduction. BALB/c, Pfp−/−, FasL−/−, STAT6−/−Pfp−/−, and STAT6−/−FasL−/− mice were inoculated in the abdominal mammary gland with 7000 4T1 tumor cells. When primary tumors were 4-5 mm in diameter, the mice were bled, and the percentage of Gr1+CD11b+ MDSCs in the peripheral blood was determined by flow cytometry. *Statistically significantly different groups (P < .05); Average +SD of 3 mice/group. (G) MDSCs apoptose in vivo in response to activated T cells. DO11.10 transgenic mice were injected subcutaneously on day 0 with cognate peptide (OVA323-339) or irrelevant peptide (HA110-119). Splenocytes were collected on day 3, depleted for RBCs, and stained for Gr1, CD11b, and cleaved caspase3 or for CD4, DO11.10 TcR, and CD69. (Top) Gated Gr1+CD11b+ and CD4+DO11.10+ cells from representative individual mice; (bottom) percentage of CD11b+Gr1+cleaved caspase3+ and percentage of activated (CD69+) CD4+DO11.10+ cells. Average +SD of 5 mice/group. Data are from 1 of 2 independent experiments. (H) Fas+/+ but not Fas−/− MDSCs apoptose in vivo in response to activated T cells. C57BL/6 Fas+/+ and Fas−/− mice were adoptively transferred with CD8+ OT-1 T cells and challenged subcutaneously with cognate peptide. Splenocytes were harvested on day 3 and analyzed according to Figure 5G for percentage of caspase3+ MDSCs and for percentage of activated (CD69+) OT-1 T cells. Average +SD of 4 mice/group.

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