[肿瘤抗原负载树突状细胞联合细胞因子诱导杀手(CIK)通过促进ASK1激活增强人食管癌细胞的杀伤活性]。

Zheng Duan, Honglin Li, Bin Hu, Yun Li, Li Huang
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Annexin V-FITC/PI double staining was used to detect the apoptosis rate of cells, immunofluorescence staining to detect the expression of phosphorylated apoptotic signal-regulated kinase 1 (p-ASK1) and Western blot analysis to detect the expression of ASK1 pathway related proteins. A nude mouse model of esophageal cancer transplantation tumor was constructed and divided into control group, DC combined with CIK group and Ag-DC combined with CIK group. The corresponding immune cells were injected into the tail vein for treatment and the tumor volume was measured every 2 days. After 21 days, all nude mice were sacrificed with the tumors taken out. HE staining was used to observe the tumor pathological changes and immunohistochemical staining was performed to detect the expression of ki67 and ASK1 in the tumor tissue. Results Comparedwith the CIK group alone and the DC combined with CIK group, the ratio of CD3<sup>+</sup> CD8<sup>+</sup> and CD3<sup>+</sup> CD56<sup>+</sup> in the cells significantly increased after Ag-DCs and CIKs co-culture, along with the increased killing rate of EC9706 cells, increased apoptosis rate of EC9706 cells, and the improved activation level of ASK1. Compared with the CIK group and the DC combined with CIK group, the growth of the transplanted tumor in nude mice treated with Ag-DCs combined with CIKs was significantly inhibited, and after 21 days, it was observed that the tumor tissue mass in this group was relatively smaller, with sparsely arranged cells in the tumor tissue and a decline in the positive rate of ki67 in tumor tissue, while the positive rate of ASK1 was significantly increased. Conclusion Co-cultivation of tumor antigen-loaded DCs with CIKs can significantly increase the killing activity of esophageal cancer tumor cells. 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引用次数: 0

摘要

目的探讨肿瘤抗原负载树突状细胞(tumor antigen-loaded dendritic cells, Ag-DCs)联合细胞因子诱导杀伤剂(cytofactor -induced killer, CIKs)杀伤食管癌肿瘤细胞的作用及机制。方法对外周血dc和CIKs进行诱导培养,将dc负载肿瘤抗原获得ag - dc, ag - dc与CIKs共培养。实验分为CIK组、DC联合CIK组、Ag-DC联合CIK组。流式细胞术检测细胞表型。采用MTT法测定其对EC9706细胞的杀伤活性。Annexin V-FITC/PI双染色检测细胞凋亡率,免疫荧光染色检测磷酸化凋亡信号调节激酶1 (p-ASK1)的表达,Western blot检测ASK1通路相关蛋白的表达。建立食管癌移植瘤裸鼠模型,分为对照组、DC联合CIK组和Ag-DC联合CIK组。将相应的免疫细胞注入尾静脉治疗,每2天测量肿瘤体积。21 d后处死裸鼠,摘除肿瘤。HE染色观察肿瘤病理变化,免疫组化染色检测ki67、ASK1在肿瘤组织中的表达。结果Ag-DCs与CIKs共培养后,与CIK单独组和DC联合CIK组比较,细胞中CD3+ CD8+和CD3+ CD56+比值显著升高,EC9706细胞杀伤率升高,EC9706细胞凋亡率升高,ASK1活化水平提高。与CIK组和DC联合CIK组相比,Ag-DCs联合CIK治疗裸鼠移植瘤的生长明显受到抑制,21天后观察到该组肿瘤组织质量相对较小,肿瘤组织中细胞排列稀疏,肿瘤组织中ki67的阳性率下降,而ASK1的阳性率明显升高。结论载瘤抗原dc与CIKs共培养可显著提高对食管癌肿瘤细胞的杀伤活性。其作用机制可能与ASK1通路的激活有关。
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[Tumor antigen-loaded dendritic cells combined with cytokine-induced killer (CIK) enhance the killing activity of human esophageal cancer cells by promoting ASK1 activation].

Objective To clarify the effect and mechanism of tumor antigen-loaded dendritic cells (Ag-DCs) combined with cytokine-induced killers (CIKs) on the killing of esophageal cancer tumor cells. Methods Peripheral blood DCs and CIKs were induced and cultured, and the DCs were loaded with tumor antigen to obtain Ag-DCs, and Ag-DCs were co-cultured with CIKs. The experiment was divided into CIK group, DC combined with CIK group, Ag-DC combined with CIK group. Flow cytometry was used to detect the phenotype of cells. MTT assay was employed to determine the killing activity against EC9706 cells. Annexin V-FITC/PI double staining was used to detect the apoptosis rate of cells, immunofluorescence staining to detect the expression of phosphorylated apoptotic signal-regulated kinase 1 (p-ASK1) and Western blot analysis to detect the expression of ASK1 pathway related proteins. A nude mouse model of esophageal cancer transplantation tumor was constructed and divided into control group, DC combined with CIK group and Ag-DC combined with CIK group. The corresponding immune cells were injected into the tail vein for treatment and the tumor volume was measured every 2 days. After 21 days, all nude mice were sacrificed with the tumors taken out. HE staining was used to observe the tumor pathological changes and immunohistochemical staining was performed to detect the expression of ki67 and ASK1 in the tumor tissue. Results Comparedwith the CIK group alone and the DC combined with CIK group, the ratio of CD3+ CD8+ and CD3+ CD56+ in the cells significantly increased after Ag-DCs and CIKs co-culture, along with the increased killing rate of EC9706 cells, increased apoptosis rate of EC9706 cells, and the improved activation level of ASK1. Compared with the CIK group and the DC combined with CIK group, the growth of the transplanted tumor in nude mice treated with Ag-DCs combined with CIKs was significantly inhibited, and after 21 days, it was observed that the tumor tissue mass in this group was relatively smaller, with sparsely arranged cells in the tumor tissue and a decline in the positive rate of ki67 in tumor tissue, while the positive rate of ASK1 was significantly increased. Conclusion Co-cultivation of tumor antigen-loaded DCs with CIKs can significantly increase the killing activity of esophageal cancer tumor cells. The mechanism of action may be related to the activation of the ASK1 pathway.

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