Cytokine-induced killer cells co-cultured with dendritic cells loaded with the protein lysate produced by radiofrequency ablation induce a specific antitumor response

Shan,Chan‑Chan; Shi,Liang‑Rong; Ding,Mei‑Qian; Zhu,Yi‑Bei; Li,Xiao‑Dong; Xu,Bin; Jiang,Jing‑Ting; Wu,Chang‑Ping

doi:10.3892/ol.2015.2977

Cytokine-induced killer cells co-cultured with dendritic cells loaded with the protein lysate produced by radiofrequency ablation induce a specific antitumor response

Authors:
- Chan‑Chan Shan
- Liang‑Rong Shi
- Mei‑Qian Ding
- Yi‑Bei Zhu
- Xiao‑Dong Li
- Bin Xu
- Jing‑Ting Jiang
- Chang‑Ping Wu
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Affiliations: Department of Tumor Biological Treatment, The Third Affiliated Hospital of Soochow University, Changzhou, Jiangsu, P.R. China, Department of Oncology, The Third Affiliated Hospital of Soochow University, Changzhou, Jiangsu, P.R. China, Institute of Biotechnology, Soochow University, Suzhou, Jiangsu, P.R. China
Published online on: February 17, 2015 https://doi.org/10.3892/ol.2015.2977
Pages: 1549-1556
Copyright: © Shan et al. This is an open access article distributed under the terms of Creative Commons Attribution License.

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Abstract

Radiofrequency ablation (RFA) causes coagulative necrosis of tumor tissue and the production of local tumor protein debris. These fragments of tumor protein debris contain a large number of various antigens, which can stimulate a specific cellular immune response. In the present study, dendritic cells (DCs) were loaded with tumor protein lysate antigens that were produced in situ by RFA, and were used to treat murine colon carcinoma in combination with cytokine‑induced killer (CIK) cells. Subsequent to the treatment of murine colon carcinoma by RFA, the in situ supernatant of tumor lysis was collected and the DCs were loaded with the lysate antigen to generate Ag‑DCs. CIK cells induced from the spleen cells of mice were co‑cultured with Ag‑DCs to generate Ag‑DC‑CIK cells. The results revealed that the Ag‑DC‑CIK cells exhibited strong antitumor activity in vitro and in vivo. The morphology and immunophenotypes of these cells were determined using microscopy and flow cytometry, respectively. The cytotoxic activity of Ag-DC-CIK cells was determined using a CCK-8 assay. To establish a mouse model, mice were randomized into Ag-DC-CIK, DC-CIK, CIK and PBS control groups and monitored for tumor growth and survival time. ANOVA was used to compare the trends in the three groups for implanted tumor volumes. The log-rank test was used to compare the survival time. The present findings indicated that DCs loaded with the protein lysate antigens of tumors, produced in situ by RFA, combined with CIK cells may be a novel strategy for cancer treatment.