[基于肝素酶基因修饰树突状细胞的疫苗对胃癌细胞的免疫反应]

[Immune response of heparinase gene modified dendritic cell-based vaccine on gastric cancer cells].

作者信息

Cai Yong-guo, Fang Dian-chun, Chen Ling, Wang Dong-xu, Luo Yuan-hui, Tang Xu-dong, Chen Ting, Yang Shi-ming

机构信息

Institute of Gastroenterology of PLA, Southwest Hospital, Third Military Medical University, Chongqing 400038, China.

出版信息

Zhonghua Yi Xue Za Zhi. 2006 Nov 28;86(44):3122-7.

PMID:17313764

Abstract

OBJECTIVE

To explore the feasibility of heparinase vaccine in active immunity for gastric cancer.

METHODS

Dendritic cells originated from the peripheral blood mononuclear cells (PBMC) of healthy HLA-A2 positive donors were transfected with recombinant adenovirus containing heparinase full length cDNA of heparanase to generate heparanase gene modified DC vaccine. T lymphocytes from the same donors were activated by those genetically modified DC vaccine repeatedly to generate heparanase specific cytotoxicity T lymphocytes (CTL). CTL-mediated cell lysis to gastric cancer cells of the lines KATO-III and SGC-7901 was analyzed in vitro by standard (51)Cr releasing assay. Heparinase specific CTL were co-cultured with KATO-III and SGC-7901 cells, and then ELISA was used to detect the IFN-gamma release.

RESULTS

Expression of heparanase was significantly increased in the DCs transfected with heparinase recombinant adenovirus. Heparanase specific CTL generated from the genetically modified DC vaccine exhibited potent lysis to the KATO-III gastric cancer cells positive in both heparinase and HLA-A2 at each E/T ratio, whereas, these heparinase specific CTL could not lyse the SGC-7901 cells positive to heparinase but negative to HLA-A2, with a specific lysis rate of only 11.1% +/- 4.6% even at an E:T ratio of 40:1. Further study showed that heparanase vaccination had no detectable lysis on the autologous lymphocytes in vitro with a specific lysis rate of only 11.4% +/- 7.9% even at an E:T ratio of 40:1. The IFN-gamma release amount when the heparanase specific CTL were co-cultured with the KATO-III cells was 280.4 pg/ml +/- 23.5 pg/ml, significantly higher than that when the heparanase specific CTL were co-cultured with the rAd5-Lacz modified DC (120.6 pg/ml +/- 18.9 pg/ml), and that of the IL-2 stimulated T cells (60.0 pg/ml +/- 10.6 pg/ml, both P < 0.05). In contrast the IFN-gamma release amounts of the SGC-7901 cells and autologous lymphocytes remained unchanged when they were co-cultured with either above-mentioned effector cells (both P > 0.05).

CONCLUSION

DC genetically modified by heparanase gene activate heparanase specific CTL and induce potent immune response against HLA-matched and heparinase positive gastric cancer cells in vitro, whereas they have no killing effect on autologous lymphocytes. Heparanase is an effective and safe target for immunogen therapy of tumor, thus providing a new biotherapy method for advanced gastric cancer.

摘要

目的

探讨肝素酶疫苗用于胃癌主动免疫的可行性。

方法

从健康的HLA - A2阳性供者的外周血单个核细胞（PBMC）中提取树突状细胞（DC），用含硫酸乙酰肝素酶全长cDNA的重组腺病毒转染，构建硫酸乙酰肝素酶基因修饰的DC疫苗。用该基因修饰的DC疫苗反复激活同一供者的T淋巴细胞，产生硫酸乙酰肝素酶特异性细胞毒性T淋巴细胞（CTL）。采用标准的（51）Cr释放试验，体外分析CTL对KATO - III和SGC - 7901胃癌细胞系的细胞裂解作用。将硫酸乙酰肝素酶特异性CTL与KATO - III和SGC - 7901细胞共培养，然后用ELISA检测IFN - γ的释放量。

结果

用硫酸乙酰肝素酶重组腺病毒转染的DC中，硫酸乙酰肝素酶的表达显著增加。基因修饰的DC疫苗产生的硫酸乙酰肝素酶特异性CTL在各效靶比下对硫酸乙酰肝素酶和HLA - A2均阳性的KATO - III胃癌细胞表现出较强的裂解作用，而这些硫酸乙酰肝素酶特异性CTL不能裂解硫酸乙酰肝素酶阳性但HLA - A2阴性的SGC - 7901细胞，即使在效靶比为40∶1时，特异性裂解率也仅为11.1%±4.6%。进一步研究表明，硫酸乙酰肝素酶疫苗在体外对自体淋巴细胞无明显裂解作用，即使在效靶比为40∶1时，特异性裂解率也仅为11.4%±7.9%。硫酸乙酰肝素酶特异性CTL与KATO - III细胞共培养时IFN - γ释放量为280.4 pg/ml±23.5 pg/ml，显著高于硫酸乙酰肝素酶特异性CTL与rAd5 - Lacz修饰的DC共培养时的释放量（120.6 pg/ml±18.9 pg/ml），也高于IL - 2刺激的T细胞的释放量（60.0 pg/ml±10.6 pg/ml，P均<0.05）。相反，SGC - 7901细胞和自体淋巴细胞与上述任何一种效应细胞共培养时，IFN - γ释放量均无变化（P均>0.05）。