中华眼视光学与视觉科学杂志
中華眼視光學與視覺科學雜誌
중화안시광학여시각과학잡지
CHINESE JOURNAL OF OPTOMETRY OPHTHALMOLOGY AND VISUAL SCIENCE
2012年
1期
47-52
,共6页
毛娅妮%李正原%黄娟%肖伟%陈晓云%凌士奇%项道满
毛婭妮%李正原%黃娟%肖偉%陳曉雲%凌士奇%項道滿
모아니%리정원%황연%초위%진효운%릉사기%항도만
血管内皮生长因子A%RNA干扰%视网膜新生血管化%视网膜病,早产儿%模型,动物
血管內皮生長因子A%RNA榦擾%視網膜新生血管化%視網膜病,早產兒%模型,動物
혈관내피생장인자A%RNA간우%시망막신생혈관화%시망막병,조산인%모형,동물
Vascular endothelial growth factor A%RNA interference%Retinal neovascularization%Retinopathy of prematurity%Models,animal
目的 探讨玻璃体腔注射靶向血管内皮生长因子(VEGF)的RNA干扰慢病毒抑制氧诱导视网膜病变(OIR)小鼠视网膜新生血管生成的作用及其机制.方法 实验研究.构建4对针对靶基因小鼠VEGF的siRNA干扰载体,筛选并进行慢病毒包装.60只C57BL/6J小鼠分成4组(每组15只):正常对照组,OIR模型组,OIR+空载体组,OIR+VEGF-RNA干扰组.OIR+空载体组和OIR+VEGF-RNA干扰慢病毒组的小鼠在生后第5天玻璃体腔注射相应的1μl的7.5×107空载体慢病毒和VEGF-RNA干扰慢病毒.后3组小鼠在生后第7天建立OIR模型.第17天时FITC-Dextran灌注视网膜铺片观察4组小鼠视网膜血管形态及面积变化,视网膜铺片免疫荧光染色检测紧密连接蛋白Claudin-5和Occludin的分布变化,Western blot检测VEGF、磷酸肌醇3激酶(PI3K)、酪氨酸蛋白激酶SRC、磷酸化细胞外信号调节激酶( p-ERK)蛋白表达量的变化.数据采用单因素方差分析进行比较.结果 FITC-Dextran灌注视网膜铺片显示正常组视网膜血管分布呈均匀网状;RNA干扰组新生血管面积(0.271 399 mm2)明显较OIR模型组(1.212 782 mm2)、空载体组(1.152 504 mm2)少(F=449.924,P<0.01).OIR模型组和空载体组间差异无统计学意义,其余两两间差异均有统计学意义(P<0.01).视网膜铺片免疫荧光染色显示紧密连接蛋白Claudin-5和Occludin在RNA干扰组中与正常组相似,呈均匀光滑线性分布,而在OIR模型组、空载体组的分布中断、不均匀,在新生血管团中可见团块状的强荧光;VEGF的RNA干扰组中VEGF、PI3K、酪氨酸蛋白激酶SRC和p-ERK的蛋白表达量较OIR模型和空载体组低.结论 玻璃体腔注射靶向VEGF的RNA干扰慢病毒能有效抑制OIR小鼠模型中VEGF及其下游通路蛋白的表达,从而抑制视网膜新生血管的形成,为临床上早产儿视网膜病变的防治提供了新思路和新途径.
目的 探討玻璃體腔註射靶嚮血管內皮生長因子(VEGF)的RNA榦擾慢病毒抑製氧誘導視網膜病變(OIR)小鼠視網膜新生血管生成的作用及其機製.方法 實驗研究.構建4對針對靶基因小鼠VEGF的siRNA榦擾載體,篩選併進行慢病毒包裝.60隻C57BL/6J小鼠分成4組(每組15隻):正常對照組,OIR模型組,OIR+空載體組,OIR+VEGF-RNA榦擾組.OIR+空載體組和OIR+VEGF-RNA榦擾慢病毒組的小鼠在生後第5天玻璃體腔註射相應的1μl的7.5×107空載體慢病毒和VEGF-RNA榦擾慢病毒.後3組小鼠在生後第7天建立OIR模型.第17天時FITC-Dextran灌註視網膜鋪片觀察4組小鼠視網膜血管形態及麵積變化,視網膜鋪片免疫熒光染色檢測緊密連接蛋白Claudin-5和Occludin的分佈變化,Western blot檢測VEGF、燐痠肌醇3激酶(PI3K)、酪氨痠蛋白激酶SRC、燐痠化細胞外信號調節激酶( p-ERK)蛋白錶達量的變化.數據採用單因素方差分析進行比較.結果 FITC-Dextran灌註視網膜鋪片顯示正常組視網膜血管分佈呈均勻網狀;RNA榦擾組新生血管麵積(0.271 399 mm2)明顯較OIR模型組(1.212 782 mm2)、空載體組(1.152 504 mm2)少(F=449.924,P<0.01).OIR模型組和空載體組間差異無統計學意義,其餘兩兩間差異均有統計學意義(P<0.01).視網膜鋪片免疫熒光染色顯示緊密連接蛋白Claudin-5和Occludin在RNA榦擾組中與正常組相似,呈均勻光滑線性分佈,而在OIR模型組、空載體組的分佈中斷、不均勻,在新生血管糰中可見糰塊狀的彊熒光;VEGF的RNA榦擾組中VEGF、PI3K、酪氨痠蛋白激酶SRC和p-ERK的蛋白錶達量較OIR模型和空載體組低.結論 玻璃體腔註射靶嚮VEGF的RNA榦擾慢病毒能有效抑製OIR小鼠模型中VEGF及其下遊通路蛋白的錶達,從而抑製視網膜新生血管的形成,為臨床上早產兒視網膜病變的防治提供瞭新思路和新途徑.
목적 탐토파리체강주사파향혈관내피생장인자(VEGF)적RNA간우만병독억제양유도시망막병변(OIR)소서시망막신생혈관생성적작용급기궤제.방법 실험연구.구건4대침대파기인소서VEGF적siRNA간우재체,사선병진행만병독포장.60지C57BL/6J소서분성4조(매조15지):정상대조조,OIR모형조,OIR+공재체조,OIR+VEGF-RNA간우조.OIR+공재체조화OIR+VEGF-RNA간우만병독조적소서재생후제5천파리체강주사상응적1μl적7.5×107공재체만병독화VEGF-RNA간우만병독.후3조소서재생후제7천건립OIR모형.제17천시FITC-Dextran관주시망막포편관찰4조소서시망막혈관형태급면적변화,시망막포편면역형광염색검측긴밀련접단백Claudin-5화Occludin적분포변화,Western blot검측VEGF、린산기순3격매(PI3K)、락안산단백격매SRC、린산화세포외신호조절격매( p-ERK)단백표체량적변화.수거채용단인소방차분석진행비교.결과 FITC-Dextran관주시망막포편현시정상조시망막혈관분포정균균망상;RNA간우조신생혈관면적(0.271 399 mm2)명현교OIR모형조(1.212 782 mm2)、공재체조(1.152 504 mm2)소(F=449.924,P<0.01).OIR모형조화공재체조간차이무통계학의의,기여량량간차이균유통계학의의(P<0.01).시망막포편면역형광염색현시긴밀련접단백Claudin-5화Occludin재RNA간우조중여정상조상사,정균균광활선성분포,이재OIR모형조、공재체조적분포중단、불균균,재신생혈관단중가견단괴상적강형광;VEGF적RNA간우조중VEGF、PI3K、락안산단백격매SRC화p-ERK적단백표체량교OIR모형화공재체조저.결론 파리체강주사파향VEGF적RNA간우만병독능유효억제OIR소서모형중VEGF급기하유통로단백적표체,종이억제시망막신생혈관적형성,위림상상조산인시망막병변적방치제공료신사로화신도경.
Objective To investigate the inhibitory effect of vascular endothelial growth factor (VEGF)-targeted RNA interference on the retinal neovascularization of mice with oxygen-induced retinopathy (OIR).Methods This was an experimental study.OIR mice models were induced by exposing mice to a 75% concentration of oxygen from postnatal day 7 (P7) to P12 and then returned to room air from P12 to P17.VEGF-siRNA was designed,screened and packaged in 293T cells to produce VEGF-RNAi-lentivirus.Sixty C57BL/6J mice were divided into 4 groups (every group n=15):normal control group,OIR group,OIR+lentivirus (OIR-K-virus) group,and OIR+VEGF-RNAi-lentivirus (OIR-Ri-virus) group.Intravitreal injection of lentivirus was performed at P5 in the OIR-K-virus group and OIR-Ri-virus group.After FITC-Dextran perfusion,a retinal flat-mount was used to observe the area of retinal neovascularization.The distribution of Claudin-5 and Occludin was detected by double immunofluorescence staining of the retinal flat-mount.The expression of VEGF,phosphotylinosital 3 kinase (PI3K),tyrosine kinase SRC,extracellular signal-regulated kinase (ERK) and phosphorylation ERK (p-ERK) proteins was analyzed by Western blot.Data were analyzed with a one-way ANOVA.Results A study of the retinal flat-mounts after FITC-Dextran perfusion showed that the distribution of retinal vessels was uniform and there was no neovascularization in the normal group.The area of retinal neovascularization in the OIR group was 1.212 782 mm2,OIR-K-virus group was 1.152 504 mm2,and OIR-Ri-virus group was 0.271 399 mm2,the difference between groups was significant (F=449.924,P<0.01).There was no significant difference in the areas of retinal neovascularization between the OIR group and OIR-K-virus group.The areas of retinal neovascularization in the OIR-Ri-virus group were reduced significantly (P<0.01) compared to the OIR group or the OIR-K-virus group.The distribution of Claudin-5 and Occludin in the retinal vessels of the OIR-Ri-virus group was more uniform and smoother than distribution in the OIR group or OIR-K-virus group.The expression of VEGF,PI3K,tyrosine kinase SRC and p-ERK protein in the OIR-Ri-virus group was significantly decreased compared to expression in the OIR and OIR-K-virus groups and was similar to the expression of the normal group.Conclusion The expression of VEGF and its signal pathway and development of retinal neovascularization in the OIR mice model were significantly inhibited by the intravitreal injection of lentivirus-mediated VEGF RNA interference,which may provide a new approach for the treatment of retinopathy of prematurity (ROP) in the clinic.
