A CCR4 antagonist reverses the tumor-promoting microenvironment of renal cancer
Chiara Berlato, Moddasar N. Khan, Tiziana Schioppa, Richard Thompson, Eleni Maniati, Anne Montfort, Maryam Jangani, Monica Canosa, Hagen Kulbe, Urs B. Hagemann, Alexander R. Duncan, Laura Fletcher, Robert W. Wilkinson, Thomas Powles, Sergio A. Quezada, Frances R. Balkwill
Chiara Berlato, Moddasar N. Khan, Tiziana Schioppa, Richard Thompson, Eleni Maniati, Anne Montfort, Maryam Jangani, Monica Canosa, Hagen Kulbe, Urs B. Hagemann, Alexander R. Duncan, Laura Fletcher, Robert W. Wilkinson, Thomas Powles, Sergio A. Quezada, Frances R. Balkwill
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Research Article Immunology Oncology

A CCR4 antagonist reverses the tumor-promoting microenvironment of renal cancer

Abstract

Elevated expression of the chemokine receptor CCR4 in tumors is associated with poor prognosis in several cancers. Here, we have determined that CCR4 was highly expressed in human renal cell carcinoma (RCC) biopsies and observed abnormal levels of CCR4 ligands in RCC patient plasma. An antagonistic anti-CCR4 antibody had antitumor activity in the RENCA mouse model of RCC. CCR4 inhibition did not reduce the proportion of infiltrating leukocytes in the tumor microenvironment but altered the phenotype of myeloid cells, increased NK cell and Th1 cytokine levels, and reduced immature myeloid cell infiltrate and blood chemokine levels. In spite of prominent changes in the myeloid compartment, the anti-CCR4 antibody did not affect RENCA tumors in T cell–deficient mice, and treatment with an anti–class II MHC antibody abrogated its antitumor activity. We concluded that the effects of the anti-CCR4 antibody required the adaptive immune system and CD4+ T cells. Moreover, CCL17-induced IFN-γ production was reduced when Th1-polarized normal CD4+ T cells were exposed to the CCR4 ligand, evidencing the involvement of CCR4 in Th1/Th2 regulation. The anti-CCR4 antibody, alone or in combination with other immune modulators, is a potential treatment approach to human solid cancers with high levels of CCR4-expressing tumor-infiltrating leukocytes and abnormal plasma CCR4 ligand levels.

Authors

Chiara Berlato, Moddasar N. Khan, Tiziana Schioppa, Richard Thompson, Eleni Maniati, Anne Montfort, Maryam Jangani, Monica Canosa, Hagen Kulbe, Urs B. Hagemann, Alexander R. Duncan, Laura Fletcher, Robert W. Wilkinson, Thomas Powles, Sergio A. Quezada, Frances R. Balkwill

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Figure 6

Effects of anti-CCR4 on the RENCA tumors require CD4+ cells.

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Effects of anti-CCR4 on the RENCA tumors require CD4+ cells. (A–D) BALB/...
(AD) BALB/c nu/nu mice were injected with 1 × 105 RENCA-luc cells and treated with Affi-5 (T) or isotype control (C) (10 mg/kg) twice weekly starting 48 hours after surgery. Mice were sacrificed at 17 days after surgery, and tumor weight was determined (n = 9 C, n = 8 T, not significant). Geometric mean of fluorescence intensity for MHCII (B) and MR (C) staining on macrophages (CD45+CD11b+F4/80+), for isotype-treated and Affi-5–treated dissociated tumors; n = 4. (D) Percentage of NK cells (CD45+CD3DX5+) among the CD45+ population; n = 4. (EH) BALB/c mice were injected with 1 × 105 RENCA-luc cells and treated with Affi-5 (T) or isotype control (C) (10 mg/kg) twice weekly starting 48 hours after surgery. Treatment with anti-MHCII or the relevant isotype control (10 mg/kg) was started 1 day prior to surgery and continued with 3 doses per week. Mice were sacrificed 17 days after surgery, tumor weight was determined (n =6 for each group), and tumors were dissociated and characterized by flow cytometry. (E) Blocking of MHCII has a significant effect on tumor weight (2-way ANOVA, *P = 0.049). Bonferroni post-test showed significant difference (P < 0.05) in weight of Affi-5–treated tumors in the presence versus absence of anti-MHCII. (F and G) Geometric mean of fluorescence intensity (MFI) for MHCII (F) and MR (G) staining on macrophages (CD45+CD11b+F4/80+). There is a significant difference between MHCII and MR expression of macrophages from Affi-5–treated tumors in the presence or absence of anti-MHCII (Kruskal-Wallis test with Dunn post-test, *P < 0.05 and 1-way ANOVA with Bonferroni post-test, **P < 0.001, with n = 3–4 for each group). (H) Percentage of NK cells (CD45+CD3DX5+) among the CD45+ population. There is a significant difference (1-way ANOVA with Bonferroni post-test, ***P < 0.001) in the percentage of NK cells from Affi-5–treated tumors in the presence versus absence of anti-MHCII.