Pancreatic cancer therapy with combined mesothelin-redirected chimeric antigen receptor T cells and cytokine-armed oncolytic adenoviruses
Keisuke Watanabe, … , Akseli Hemminki, Carl H. June
Keisuke Watanabe, … , Akseli Hemminki, Carl H. June
Published April 5, 2018
Citation Information: JCI Insight. 2018;3(7):e99573. https://doi.org/10.1172/jci.insight.99573.
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Research Article Therapeutics

Pancreatic cancer therapy with combined mesothelin-redirected chimeric antigen receptor T cells and cytokine-armed oncolytic adenoviruses

Abstract

Pancreatic ductal adenocarcinoma (PDA) is characterized by its highly immunosuppressive tumor microenvironment (TME) that limits T cell infiltration and induces T cell hypofunction. Mesothelin-redirected chimeric antigen receptor T cell (meso-CAR T cell) therapy has shown some efficacy in clinical trials but antitumor efficacy remains modest. We hypothesized that combined meso-CAR T cells with an oncolytic adenovirus expressing TNF-α and IL-2 (Ad5/3-E2F-D24-TNFa-IRES-IL2, or OAd-TNFa-IL2) would improve efficacy. OAd-TNFa-IL2 enhanced the antitumor efficacy of meso-CAR T cells in human-PDA-xenograft immunodeficient mice and efficacy was associated with robustly increased tumor-infiltrating lymphocytes (TILs), enhanced and prolonged T cell function. Mice treated with parental OAd combined with meso-CAR T developed tumor metastasis to the lungs even if primary tumors were controlled. However, no mice treated with combined OAd-TNFa-IL2 and meso-CAR T died of tumor metastasis. We also evaluated this approach in a syngeneic mouse tumor model by combining adenovirus expressing murine TNF-α and IL-2 (Ad-mTNFa-mIL2) and mouse CAR T cells. This approach induced significant tumor regression in mice engrafted with highly aggressive and immunosuppressive PDA tumors. Ad-mTNFa-mIL2 increased both CAR T cell and host T cell infiltration to the tumor and altered host tumor immune status with M1 polarization of macrophages and increased dendritic cell maturation. These findings indicate that combining cytokine-armed oncolytic adenovirus to enhance the efficacy of CAR T cell therapy is a promising approach to overcome the immunosuppressive TME for the treatment of PDA.

Authors

Keisuke Watanabe, Yanping Luo, Tong Da, Sonia Guedan, Marco Ruella, John Scholler, Brian Keith, Regina M. Young, Boris Engels, Suvi Sorsa, Mikko Siurala, Riikka Havunen, Siri Tähtinen, Akseli Hemminki, Carl H. June

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Figure 5

Intensity of functional T cell infiltration is associated with sustained tumor regression after mesothelin-redirected chimeric antigen receptor T cells (meso-CAR T cells) and oncolytic adenovirus expressing TNF-α and IL-2, Ad5/3-E2F-D24-TNFa-IRES-IL2 (Ad5/3-OAd-TNFa-IL2) treatment in an AsPC-1 tumor xenograft immunodeficient mouse model.

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Intensity of functional T cell infiltration is associated with sustained...
(A and B) Tumor volumes by caliper measurements and waterfall plots comparing baseline to day 57. Mice from the indicated 2 treatment groups were observed until day 57 and then sacrificed. Data for the surviving mice (6 of 8 mice for meso-CAR T cell group and all 7 mice for OAd-TNFa-IL2 + meso-CAR T cell group) is shown. Bars represent means and SEM in A. (C) Mesothelin expression on tumors at day 57. Mesothelin expression of the representative tumor from OAd-TNFa-IL2 + meso-CAR T cell group by immunohistochemistry (IHC) (upper panels) and digital masks (lower panels) on the same fields as upper panels are shown. The low-power fields (LPFs) show central necrosis and heterogeneity in mesothelin intensity (left panels). Representative high-power fields (HPFs) of mesothelin-positive area (center panels) and mesothelin low-negative area (right panels) from the tumor shown in the LPF. Blue, negative; Yellow, low intensity; Orange, mid intensity; Red, high intensity. Original magnification, ×20. Scale bars: 5 mm for LPF, 100 μm for HPF. (D) Correlation between mesothelin expression and tumor size at day 57. Areas of mesothelin positivity (%) against tumor volumes are plotted. n.s., not significant. (E) Correlation between CD3+ tumor-infiltrating lymphocyte (TIL) density and tumor volumes. Percentage CD3+ cells to tumor cells against tumor volumes are plotted. A linear regression line is shown. *P < 0.05. (F) Expression of Ki67 by TILs. Ki67 expression by CD3+ TILs from surviving mice was analyzed by flow cytometry (FCM). Columns are arranged in the order of tumor volumes at day 57 and the tumor sizes are shown at the top of each column. (G) Correlation between Ki67 expression by CD4+ and CD8+ TILs and tumor volumes. Percentage Ki67 expression by CD4+ TILs or CD8+ TILs against tumor volumes are plotted. Linear regression lines are shown. *P < 0.05, **P < 0.01. (H) Analysis of Treg infiltration into the tumor. CD25+FoxP3+ Tregs in CD4+ TILs were analyzed by FCM. Bars represent means and SEM. n.s., not significant by Student’s t test.