机构地区:[1]天津医科大学眼科医院天津医科大学眼科研究所天津医科大学眼视光学院,300384
出 处:《中华实验眼科杂志》2017年第8期677-682,共6页Chinese Journal Of Experimental Ophthalmology
基 金:天津市高等学校科技发展计划项目(20120128)
摘 要:背景肿瘤抑素是迄今发现活性最强的内源性血管生成抑制因子,对病理性新生血管形成有明显抑制作用。Tum5片段为肿瘤抑素的抗血管生成活性片断。目的研究腺病毒介导的Tum5重组基因过表达对生理状态下人脐静脉内皮细胞(HUVECs)增生、迁移及管腔形成的影响。方法构建表达绿色荧光蛋白的空载体腺病毒(rAd—GFP)和携带重组几m5基因的腺病毒载体(rAd—Tum5)。将HUVECs分为正常对照组、空载体组(rAd-GFP组)和Tum5基因组(rAd-GFP—Tum5组)。将rAd—GFP和rAd—Tum5病毒颗粒(1×10^10/m1)各20μl分别加入rAd—GFP组和rAd—GFP—Tum5组培养液以感染培养的细胞48h,倒置荧光显微镜下观察各组细胞中GFP的表达,并计算病毒的感染效率;采用细胞计数试剂盒(CCK)-8检测各组细胞在波长为450nm处的吸光度(A)值并计算细胞增生率;采用Transwell小室实验测定各组的迁移细胞数目;采用基质胶(Matrigel)实验检测各组细胞的管腔形成数;采用人血管内皮生长因子(VEGF)ELISA试剂盒检测细胞感染后24、48和72h各组细胞培养上清液中VEGF质量浓度。结果倒置荧光显微镜下可见rAd—GFP组和rAd—GFP—Tum5组HUVECs中呈绿色荧光,rAd—GFP组和tad—GFP—Tum5组的感染效率分别为55.13%和50.31%。细胞感染后24h和48h,正常对照组、rAd—GFP组和rAd-GFP—Tum5组细胞增生率比较差异均无统计学意义(均P〉0.05);细胞感染后72h,rAd-GFP—Tum5组细胞增生率明显低于正常对照组和rAd—GFP组,差异均有统计学意义(均P〈0.01)。细胞感染后48h,正常对照组、rAd—GFP组和rAd—GFP—Tum5组迁移细胞数分别为(2260.25±930.44)、(2370.00±441.06)和(723.75±363.80)个,总体比较差异有统计学意义(F=8.524,P=0.008),rAd—GFP—Tum5组迁移细胞数量较正常对照组和rAd—GFP组均明显减少,差异�Background Tumstatin is the most active endogenous angiogenesis inhibitor, which has a marked inhibitory effect on pathological neovascularization, and Tum5 is an angiogenesis inhibitors fragment of full- length tumstatin. Objective This study was to investigate the effects of adenovirus-mediated overexpression of recombinant Turn5 gene on the proliferation, migration and tube formation of human umbilical vein endothelial cells (HUVECs) in physiological status. Methods The empty adenoviral vector expressing green fluorescent protein (rAd-GFP) and the viral vector expressing recombinant Turn5 gene were constructed. The HUVECs cultured in RPMI1640 medium were divided into normal control group, empty vector group (rAd-GFP group) and Tum5 gene infection group (rAd-GFP-Tum5 group). The rAd-GFP and rAd-GFP-Tum5 adenoviral particles at the density of 1 × 10^10/ml were added into the medium to infect the cells for 48 hours. The proliferation of the cells was assayed at 24, 48 and 72 hours by cell counting kit-8 ( CCK-8 ) to evaluate the proliferative rate; the migration number of the cells was detected at 48 hours after infection by Transwell chamber ; the tube formation number of the cells were detected by Matrigel method. The concentration of vascular endothelial growth factor (YEGF) in cell supernatants was assayed by ELISA at 24, 48, and 72 hours following adenoviral infection. Results The cultured ceils showed green fluorescence in the rAd-GFP group and rAd-GFP-Tum5 group under the inverted fluorescence microscope, and the infection efficiency of rAd-GFP and rAd-GFP-Tum5 was 55. 13 % and 50.31% , respectively. No significant difference was found in cell proliferative rate among normal control group,rAd-GFP group and rAd-GFP-Tum5 group both at 24 and 48 hours after infection ( both at P〉0.05) ,and the cell proliferative rate was significantly lower in the rAd-GFP- Tum5 group than that in the normal control group and rAd-GFP group at 72 hours after infection ( both at P〈0. 01 ). Th
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