| 携带靶向干扰小鼠早期生长反应基因1短发夹RNA的慢病毒载体转染小鼠视网膜的干扰效率研究 |
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| 引用本文: | 蒋晶晶,刘双珍,文丹,王沙.携带靶向干扰小鼠早期生长反应基因1短发夹RNA的慢病毒载体转染小鼠视网膜的干扰效率研究[J].中华生物医学工程杂志,2011,17(2):115-119. |
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| 作者姓名: | 蒋晶晶 刘双珍 文丹 王沙 |
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| 作者单位: | 中南大学湘雅医院眼科,长沙,410008 |
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| 基金项目: | 湖南省自然科学基金,湖南省科技厅重点项目 |
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| 摘 要: | 目的 构建携带绿色荧光蛋白(GFP)和靶向干扰早期生长反应基因1(Egr-1)短发夹RNA(shRNA)共表达的慢病毒载体,转染小鼠视网膜组织,观察其对Egr-1基因的干扰效率.方法 针对已经筛选确定的Egr-1基因shRNA有效靶序列,构建携带GFP和靶向干扰Egr-1 shRNA的慢病毒载体LV-shRNA(Egr...
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| 关 键 词: | 早期生长反应基因1 RNA干扰 转染 慢病毒载体 基因表达调控 |
Efficiency of targeted interference on early growth response factor-1 by lentivirus vector containing shRNA transfected into mouse retina |
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| JIANG Jing-jing,LIU Shuang-zhen,WEN Dan,WANG Sha.Efficiency of targeted interference on early growth response factor-1 by lentivirus vector containing shRNA transfected into mouse retina[J].Chinese Journal of Biomedical Engineering,2011,17(2):115-119. |
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| Authors: | JIANG Jing-jing LIU Shuang-zhen WEN Dan WANG Sha |
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| Abstract: | Objective To construct the lentivirus vector containing green fluorescent protein (GFP)and early growth response factor-1 short hairpin RNA(Egr-1 shRNA),and to determine the efficiency of interference on Egr-1 gene in lentivirus vector-transfected mouse retinal tissue.Methods Based on the target sequences of Egr-1 shRNA screened and identified previously,the LV-shRNA(Egr-1)containing GFP and Egr-1 shRNA Was constructed.Twenty 15-day-old C57BL/6 mice were randomly divided into experimental group and negative control group(n=10 each).LV-shRNA(Egr-1)lentivirus vector Was transfected into the right eyes in the experimental group with intravitreal injection.LV-NC lentivirus vector that did not target at any specific gene Was also transfected into the right eyes in the negative control group,while the left eyes were untreated in both two groups as the blank control group.After 2 weeks,the transfection of lentiviral vector was examined under fluorescence microscope.Moreover,real-time quantitative polymerase chain reaction (RQ-PCR), Western blot and immunofluorescence were used to detect the expression of Egr-1 gene for evaluation of the interference efficiency. Results After lentiviral vector was intravitreally injected and transfected into the mouse retinal tissue, GFP was found to be widely distributed in the whole layer of the retina including the retinal pigment epithelium. RQPCR showed significantly down-regulated expression of Egr-1 mRNA in the injected eyes of experimental group compared with blank or negative controls (0.290±0.074 vs 1.006±0.033, 1.010± 0.086, all P<0.001) , with the inhibition rate being 71.29%. Western blot demonstrated that the expression of Egr-1 protein was remarkably down-regulated in the injected eyes of experimental group (0.224±0.035 vs 0.674±0.050, 0.688±0.049, all P<0.00l) , with the inhibition rate being 67.44%. Furthermore, immunofluorescence revealed no expression of fluorescence protein, except sparse distribution of Egr-1 positive cells in the inner nuclear layer of injected eyes of the experimental group. Conclusions The lentivirus vector containing GFP and Egr-1 shRNA is successfully constructed, and it may have high transfection efficiency and a wide distribution in the intravitreally injected mice eyes. Furthermore, the lentivirus vector has a high inhibition efficiency of Egr-1 gene in the mouse retina. |
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| Keywords: | Early growth response factor-1 RNA interference Transfection Lentivirus vector Gene expression regulation |
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