[pEGFP-H1载体质粒介导的血管内皮生长因子短发夹RNA有效抑制胶质瘤增殖:一项实验研究]
[Vascular endothelial growth factor shRNA mediated by pEGFP-H1 vector plasmid effectively inhibits glioma proliferation: an experimental study].
作者信息
Jiang Xiao-bing, Zhao Hong-yang, Zhou Feng, Liu Ru-en, Zhang Fang-cheng, Zhao Jia-shan
机构信息
Department of Neurosurgery, Union Hospital, Tongji Medical College, Huazhong University of Science and Technology, Wuhan 430022, China.
出版信息
Zhonghua Yi Xue Za Zhi. 2005 Mar 2;85(8):547-50.
OBJECTIVE
To investigate the inhibitory effects of RNA silencing via plasmid-mediated vascular endothelial growth factor (VEGF) shRNA on proliferation of glioma cells in vitro and in vivo.
METHODS
pEGFP-H1/VEGF vector plasmid containing enhanced green fluorescent protein (EGFP) gene and expressing VEGF shRNA was constructed. The EGFP expression was detected by fluorescent microscopy and flow cytometry. Glioma cells of the line U251 were cultured and divided into 3 groups to be transfected with blank vector, pEGFP/H1plasmid, and pEGFP-H1/VEGF respectively. RT-PCR was used to detect the mRNA expression of VEGF in the supernatants of the culture media. The protein expression of VEGF in the supernatant was detected by ELISA. The cell growth was observed with MTT method. Fifteen nude rats were randomly divided into 3 equal groups to be transplanted with U251 cells and pEGFP-H1, U251 cells and pEGFP-H1/VEGF, and U251 cells only as blank control group. The growth of glioma was observed every day. 30 days after the rats were killed and the tumors were taken out to be examined.
RESULTS
Twenty-four hours after transplantation, fluorescence microscopy showed great numbers of U251 cells that expressed green fluorescence in both the pEGFP-H1 group and pEGFP-H1/VEGF group. Flow cytometry showed that the rates of green fluorescent protein positive cells were 68.37% and 65.29% in these 2 groups (P > 0.05). MTT method showed no significant difference in the effect on cell growth among the 3 groups (all P > 0.05). PCR showed that the VEGF mRNA expression was significantly inhibited in the pEGFP-H1/VEGF group in comparison with those in the blank control group and the group transfected with pEGFP-H1 (both P < 0.05). The concentration of VEGF protein of the U251 cells transfected with pEGFP-H1/VEGF was 530 ng/L +/- 118 ng/L, significantly lower than those of the control group (2571 ng/L +/- 572 ng/L) and the group transfected with pEGFP-H1 (2402 ng/L +/- 310 ng/L, by 77.9%) (both P < 0.01). Tumor could be touched 13 days after transplantation in the rats of pEGFP-H1/VEGF group, markedly later than in the other 2 groups. Thirty days after, the weight and volume of tumor were 0.5 g +/- 0.4 g and 401 mm(3) +/- 272 mm(3) respectively in the rats of pEGFP-H1/VEGF group, both significantly lower than those of the control group and pEGFP-H1 group (1.7 g +/- 0.4 g and 1573 mm(3) +/- 330 mm(3); and 1.5 g +/- 0.7 g and 1430 mm(3) +/- 382 mm(3)) (all P < 0.01).
CONCLUSION
The successfully constructed shRNA targeting at VEGF efficiently decreases the VEGF expression of the glioma cells in vitro and suppresses the growth of glioma cells in vivo.
目的
探讨质粒介导的血管内皮生长因子(VEGF)短发夹RNA(shRNA)通过RNA沉默对体外及体内胶质瘤细胞增殖的抑制作用。
方法
构建含增强型绿色荧光蛋白(EGFP)基因并表达VEGF shRNA的pEGFP-H1/VEGF载体质粒。通过荧光显微镜和流式细胞术检测EGFP表达。培养人U251胶质瘤细胞并分为3组,分别用空白载体、pEGFP/H1质粒和pEGFP-H1/VEGF转染。采用逆转录聚合酶链反应(RT-PCR)检测培养基上清中VEGF的mRNA表达。用酶联免疫吸附测定(ELISA)检测上清中VEGF的蛋白表达。采用MTT法观察细胞生长情况。将15只裸鼠随机分为3组,分别移植U251细胞与pEGFP-H1、U251细胞与pEGFP-H1/VEGF,仅移植U251细胞作为空白对照组。每天观察胶质瘤生长情况。30天后处死大鼠,取出肿瘤进行检测。
结果
移植后24小时,荧光显微镜显示pEGFP-H1组和pEGFP-H1/VEGF组中有大量表达绿色荧光的U251细胞。流式细胞术显示这2组中绿色荧光蛋白阳性细胞率分别为68.37%和65.29%(P>0.05)。MTT法显示3组对细胞生长的影响无显著差异(均P>0.05)。PCR显示,与空白对照组和pEGFP-H1转染组相比,pEGFP-H1/VEGF组中VEGF mRNA表达明显受到抑制(均P<0.05)。pEGFP-H1/VEGF转染的U251细胞中VEGF蛋白浓度为530 ng/L±118 ng/L,明显低于对照组(2571 ng/L±572 ng/L)和pEGFP-H1转染组(2402 ng/L±310 ng/L,降低77.9%)(均P<0.01)。pEGFP-H1/VEGF组大鼠移植后13天可触及肿瘤,明显晚于其他2组。30天后,pEGFP-H1/VEGF组大鼠肿瘤重量和体积分别为0.5 g±0.4 g和401 mm³±272 mm³,均明显低于对照组和pEGFP-H1组(分别为1.7 g±0.4 g和1573 mm³±330 mm³;以及1.5 g±0.7 g和1430 mm³±382 mm³)(均P<0.01)。
结论
成功构建的靶向VEGF的shRNA可有效降低体外胶质瘤细胞的VEGF表达,并抑制体内胶质瘤细胞生长。
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