血管内皮生长因子受体2胞外域基因修饰的树突状细胞疫苗对实验性肺转移小鼠模型的抗转移作用

[Anti-metastatic effect of vascular endothelial growth factor receptor 2 extracellular domain gene-modified dendritic cell vaccination in murine model with experimental pulmonary metastasis].

作者信息

Pan Jian-ping, Weng Yue-song, Wu Qian-qian

机构信息

Institute of Immunology, Zhejiang University, Hangzhou 310031, China.

出版信息

Zhonghua Zhong Liu Za Zhi. 2006 Sep;28(9):646-9.

PMID:17274366

Abstract

OBJECTIVE

To investigate the anti-metastatic effect of vascular endothelial growth factor receptor 2 extracellular domain gene-modified dendritic cell (DC-sVEGFR-2) vaccination.

METHODS

Dendritic cells (DC) were electroporated with pcDNA3. 1/sVEGFR-2 plasmid DNA. Expression of sVEGFR-2 was determined by ELISA. For immunization, C57BL/6 mice were intravenously injected three times with 1 x 10(5) cells per mouse of DC, pcDNA3. 1-transfected DC (DC-vector) , DC-sVEGFR-2, or 100 microl of PBS at 7-day intervals. At 10 days after the last immunization, the immunized mice were subjected to assessment of cytotoxic T lymphocyte ( CTL) response to VEGFR-2, alginate bead analysis of tumor cell-induced angiogenesis, and observation of the anti-metastatic effect in B16 melanoma metastasis model. CTL activity was determined by a standard 4-h 51Cr release assay against VEGFR-2 + vascular endothelial cell line H5V, 3LL cells stably transfected with pcDNA3. 1/sVEGFR-2 (3LL,-sVEGFR-2), and VEGFR-2- cell lines EL-4 and 3LL. Monoclonal antibodies GK1.5 anti-CD4 and 2.43 anti-CD8 were used to deplete in vivo CD4 + T cells and CD8' T cells, respectively.

RESULTS

DC-sVEGFR-2 could effectively express sVEGFR-2, whereas DC-vector and DC could not. Immunization of mice with DC-sVEGFR-2 significantly induce CTL activity against VEGFR-2 + cell lines H5V and 3LL-sVEGFR-2, however, no significant CTL activity was observed when VEGFR-2- syngeneic cell lines EL-4 and 3LL. were used as target cells, implying this CTL activity was VEGFR-2 specific. Alginate bead analysis of in vivo neoangiogenesis showed that the inhibition reached 50% in mice vaccinated with DC-sVEGFR-2 compared with mice vaccinated with DC, DC-vector or PBS. Anti-metastatic experiment showed that profound reduction in pulmonary metastases was found in mice immunized with DC-sVEGFR-2, while mice immunized with PBS, DC, DC-vector developed extensive pulmonary metastases. The number of tumor nodules on lung surface decreased by 81.9% in mice immunized with DC-sVEGFR-2 when compared with mice immunized with DC-vector (49.7+/-12.7 vs. 9.0+/-3.2). In vivo T cell subset depletion experiments showed that the anti-metastatic effect of DC-sVEGFR-2 vaccination was abrogated in CD8 + T cell-depleted but not in CD4+ T cell-depleted mice.

CONCLUSION

Immunization of mice with DC-sVEGFR-2 could break self-tolerance and induce a significant CTL response to VEGFR-2, leading to profound inhibition of tumor-cell induced angiogenesis and metastasis. This anti-metastatic effect is mainly mediated by CD8+ T cells.

摘要

目的

研究血管内皮生长因子受体2胞外区基因修饰的树突状细胞（DC-sVEGFR-2）疫苗接种的抗转移作用。

方法

用pcDNA3.1/sVEGFR-2质粒DNA对树突状细胞（DC）进行电穿孔。通过酶联免疫吸附测定法测定sVEGFR-2的表达。为进行免疫接种，以7天的间隔，给C57BL/6小鼠静脉注射3次，每次每只小鼠注射1×10⁵个细胞的DC、pcDNA3.1转染的DC（DC-载体）、DC-sVEGFR-2或100微升磷酸盐缓冲液。在最后一次免疫接种后10天，对免疫接种的小鼠进行针对VEGFR-2的细胞毒性T淋巴细胞（CTL）反应评估、肿瘤细胞诱导的血管生成的藻酸盐珠分析以及在B16黑色素瘤转移模型中观察抗转移作用。通过针对VEGFR-2⁺血管内皮细胞系H5V、稳定转染pcDNA3.1/sVEGFR-2的3LL细胞（3LL,-sVEGFR-2）以及VEGFR-2⁻细胞系EL-4和3LL的标准4小时⁵¹Cr释放试验来测定CTL活性。分别使用单克隆抗体GK1.5抗CD4和2.43抗CD8在体内清除CD4⁺T细胞和CD8⁺T细胞。

结果

DC-sVEGFR-2能有效表达sVEGFR-2，而DC-载体和DC则不能。用DC-sVEGFR-2免疫小鼠可显著诱导针对VEGFR-2⁺细胞系H5V和3LL-sVEGFR-2的CTL活性，然而，当使用VEGFR-2⁻同基因细胞系EL-4和3LL作为靶细胞时，未观察到显著的CTL活性，这意味着这种CTL活性是VEGFR-2特异性的。体内新生血管生成的藻酸盐珠分析表明，与接种DC、DC-载体或磷酸盐缓冲液的小鼠相比，接种DC-sVEGFR-2的小鼠的血管生成抑制率达到50%。抗转移实验表明，用DC-sVEGFR-2免疫的小鼠肺部转移明显减少，而用磷酸盐缓冲液、DC、DC-载体免疫的小鼠则出现广泛的肺部转移。与用DC-载体免疫的小鼠相比，用DC-sVEGFR-2免疫的小鼠肺表面肿瘤结节数量减少了81.9%（49.7±12.7对9.0±3.2）。体内T细胞亚群清除实验表明，DC-sVEGFR-2疫苗接种的抗转移作用在CD8⁺T细胞清除的小鼠中被消除，但在CD4⁺T细胞清除的小鼠中未被消除。