基于载体的RNA干扰靶向血管内皮生长因子-C可抑制小鼠体内结直肠癌的肿瘤淋巴管生成和生长。
Vector-based RNA interference against vascular endothelial growth factor-C inhibits tumor lymphangiogenesis and growth of colorectal cancer in vivo in mice.
作者信息
He Xiao-wen, Yu Xiao, Liu Ting, Yu Shi-yi, Chen Dao-jin
机构信息
Department of General Surgery, Third Xiangya Hospital, Central South University, Changsha, Hunan 410013, China.
出版信息
Chin Med J (Engl). 2008 Mar 5;121(5):439-44.
BACKGROUND
RNA interference (RNAi) technology is emerging as a very potent tool to generate a cellular knockdown of a desired gene. The aim of this study was to explore whether RNAi targeting vascular endothelial growth factor-C (VEGF-C) could inhibit colorectal tumor lymphangiogenesis and tumor growth.
METHODS
We used vector-based RNAi to inhibit VEGF-C expression in colon cancer in vitro and in vivo. VEGF-C expression was quantified by real-time polymerase chain reaction and Westen blotting. To establish LoVo cell tumor xenografts in mice, we subcutaneously inoculated 1.0 x 10(6) LoVo cells in nude mice; after injection, tumors were allowed to grow for 4 weeks until the volume reached (75.8+/-55.8) mm(3). The mice were then randomly divided into two groups: (1) the VEGF-C-siRNA group (n=10) received direct injection of "therapeutic" plasmid 50 microg of LoVo-VEGF-C-siRNA into the tumor mass; (2) the control group (n=10) were injected with LoVo-control in 20 microl of sterile 0.9% NaCl solution into the tumor mass. Tumor growth, microlymphatics and microvessels were compared for mice administered either systemic VEGF-C-siRNA or control over 4 weeks.
RESULTS
The mRNA and protein expression of VEGF-C in the colon tumor cell line, LoVo, stably transfected with a VEGF-C-siRNA vector, were significantly downregulated 45.3% and 35.3% respectively. In vivo, four weeks after injection, the tumor volume were significantly smaller in VEGF-C-siRNA group than in LoVo-control group ((314.8+/-54.8) mm(3) vs (553.9+/-90.1) mm(3)); the incidences of lymph node metastasis (30%) in VEGF-C-siRNA were significantly inhibited compared with LoVo-control group (70%); in VEGF-C-siRNA group, the number of microlymphatics per microscopic field was (5.3+/-0.7) and the number of microvessels per microscopic field was (24.2+/-6.5) decreased compared with LoVo-control group (12.5+/-6.9) and (42.1+/-7.4) (all P<0.001).
CONCLUSION
Inhibition of VEGF-C expression using siRNA-mediated gene silencing vectors reduced lymphangiogenesis and lymph node metastasis and enhanced survival.
背景
RNA干扰(RNAi)技术正成为一种非常有效的工具,可在细胞水平上敲低所需基因。本研究的目的是探讨靶向血管内皮生长因子C(VEGF-C)的RNAi是否能抑制结直肠癌的淋巴管生成和肿瘤生长。
方法
我们使用基于载体的RNAi在体外和体内抑制结肠癌中VEGF-C的表达。通过实时聚合酶链反应和蛋白质免疫印迹法对VEGF-C的表达进行定量。为了在小鼠中建立LoVo细胞肿瘤异种移植模型,我们将1.0×10⁶个LoVo细胞皮下接种到裸鼠体内;注射后,让肿瘤生长4周直至体积达到(75.8±55.8)mm³。然后将小鼠随机分为两组:(1)VEGF-C-siRNA组(n = 10),将50μg的LoVo-VEGF-C-siRNA“治疗性”质粒直接注射到肿瘤块中;(2)对照组(n = 10),将20μl无菌0.9%氯化钠溶液中的LoVo对照注射到肿瘤块中。比较给予系统性VEGF-C-siRNA或对照的小鼠在4周内的肿瘤生长、微淋巴管和微血管情况。
结果
用VEGF-C-siRNA载体稳定转染的结肠肿瘤细胞系LoVo中,VEGF-C的mRNA和蛋白表达分别显著下调了45.3%和35.3%。在体内,注射后4周,VEGF-C-siRNA组的肿瘤体积明显小于LoVo对照组((314.8±54.8)mm³对(553.9±90.1)mm³);VEGF-C-siRNA组的淋巴结转移发生率(30%)与LoVo对照组(70%)相比显著受到抑制;在VEGF-C-siRNA组中,每个显微镜视野的微淋巴管数量为(5.3±0.7),每个显微镜视野的微血管数量为(24.2±6.5),与LoVo对照组(12.5±6.9)和(42.1±7.4)相比减少(所有P<0.001)。
结论
使用siRNA介导的基因沉默载体抑制VEGF-C表达可减少淋巴管生成和淋巴结转移并提高生存率。
Zotero 插件