中华妇产科杂志
中華婦產科雜誌
중화부산과잡지
CHINESE JOUNAL OF OBSTETRICS AND GYNECOLOGY
2008年
1期
45-49
,共5页
高华%施君%葛盛芳%狄文
高華%施君%葛盛芳%狄文
고화%시군%갈성방%적문
卵巢肿瘤%受体,IGF1型%RNA干扰%顺铂%药物筛选试验,抗肿瘤
卵巢腫瘤%受體,IGF1型%RNA榦擾%順鉑%藥物篩選試驗,抗腫瘤
란소종류%수체,IGF1형%RNA간우%순박%약물사선시험,항종류
Ovary neoplasms%Receptor,IGF type 1%RNA interference%Cisplatin%Drug screening assays,antitumor
目的 利用RNA干扰(RNAi)技术抑制卵巢上皮性癌(卵巢癌)HO8910PM细胞胰岛素样生长因子1型受体(IGF1R)基因的表达,探讨IGF1R的生物学功能及对顺铂敏感性的影响.方法 将IGF1R基因的特异性小分子干扰RNA(siRNA)、非特异性siRNA分别转染细胞;转染后48h通过实时PCR、蛋白印迹法(western blot)、流式细胞仪分别测定IGF1R mRNA、蛋白的表达及细胞周期变化;转染后24、48、72、96 h通过细胞增殖/毒性检测试剂cell counting kit-8(CCK-8)测定细胞增殖;于转染后24 h给予不同浓度的顺铂作用24 h,通过CCK-8法测定细胞增殖抑制率;于转染后24 h给予10μg/ml顺铂作用24 h,通过流式细胞仪及蛋白印迹法分别检测细胞凋亡和B淋巴细胞白血病/淋巴瘤蛋白2(Bcl-2)蛋白的表达.结果 (1)转染后48 h,IGF1R mRNA和蛋白的表达水平均明显下调,转染后IGF1R mRNA的表达水平下调了85.5%(P<0.01).(2)转染后48、72、96 h,细胞增殖被明显抑制,细胞增殖活性分别为1.71±0.13、2.32±0.23、2.79±0.28,与未转染及转染非特异性siRNA的对照细胞比较,差异均有统计学意义(P<0.01).(3)转染后48 h有24.37%的细胞处于G2期(P<0.05).(4)转染后24 h联合不同浓度的顺铂作用24 h,当顺铂浓度为2.5、5、10、20μg/ml时,细胞增殖被明显抑制,细胞增殖抑制率分别为(25.94±0.08)%、(40.25±0.05)%、(59.48±0.03)%、(74.18±0.08)%,差异均有统计学意义(P<0.01).(5)在转染siRNA 24 h后给予10μg/ml顺铂作用24 h,可使细胞的凋亡率增加至17.95%(P<0.05),并使Bcl-2蛋白的表达水平下调.结论 通过RNAi技术可有效抑制IGF1R基因在转录和翻译水平的表达,抑制肿瘤细胞的增殖,出现G2期阻滞,明显提高细胞对顺铂化疗的敏感性.
目的 利用RNA榦擾(RNAi)技術抑製卵巢上皮性癌(卵巢癌)HO8910PM細胞胰島素樣生長因子1型受體(IGF1R)基因的錶達,探討IGF1R的生物學功能及對順鉑敏感性的影響.方法 將IGF1R基因的特異性小分子榦擾RNA(siRNA)、非特異性siRNA分彆轉染細胞;轉染後48h通過實時PCR、蛋白印跡法(western blot)、流式細胞儀分彆測定IGF1R mRNA、蛋白的錶達及細胞週期變化;轉染後24、48、72、96 h通過細胞增殖/毒性檢測試劑cell counting kit-8(CCK-8)測定細胞增殖;于轉染後24 h給予不同濃度的順鉑作用24 h,通過CCK-8法測定細胞增殖抑製率;于轉染後24 h給予10μg/ml順鉑作用24 h,通過流式細胞儀及蛋白印跡法分彆檢測細胞凋亡和B淋巴細胞白血病/淋巴瘤蛋白2(Bcl-2)蛋白的錶達.結果 (1)轉染後48 h,IGF1R mRNA和蛋白的錶達水平均明顯下調,轉染後IGF1R mRNA的錶達水平下調瞭85.5%(P<0.01).(2)轉染後48、72、96 h,細胞增殖被明顯抑製,細胞增殖活性分彆為1.71±0.13、2.32±0.23、2.79±0.28,與未轉染及轉染非特異性siRNA的對照細胞比較,差異均有統計學意義(P<0.01).(3)轉染後48 h有24.37%的細胞處于G2期(P<0.05).(4)轉染後24 h聯閤不同濃度的順鉑作用24 h,噹順鉑濃度為2.5、5、10、20μg/ml時,細胞增殖被明顯抑製,細胞增殖抑製率分彆為(25.94±0.08)%、(40.25±0.05)%、(59.48±0.03)%、(74.18±0.08)%,差異均有統計學意義(P<0.01).(5)在轉染siRNA 24 h後給予10μg/ml順鉑作用24 h,可使細胞的凋亡率增加至17.95%(P<0.05),併使Bcl-2蛋白的錶達水平下調.結論 通過RNAi技術可有效抑製IGF1R基因在轉錄和翻譯水平的錶達,抑製腫瘤細胞的增殖,齣現G2期阻滯,明顯提高細胞對順鉑化療的敏感性.
목적 이용RNA간우(RNAi)기술억제란소상피성암(란소암)HO8910PM세포이도소양생장인자1형수체(IGF1R)기인적표체,탐토IGF1R적생물학공능급대순박민감성적영향.방법 장IGF1R기인적특이성소분자간우RNA(siRNA)、비특이성siRNA분별전염세포;전염후48h통과실시PCR、단백인적법(western blot)、류식세포의분별측정IGF1R mRNA、단백적표체급세포주기변화;전염후24、48、72、96 h통과세포증식/독성검측시제cell counting kit-8(CCK-8)측정세포증식;우전염후24 h급여불동농도적순박작용24 h,통과CCK-8법측정세포증식억제솔;우전염후24 h급여10μg/ml순박작용24 h,통과류식세포의급단백인적법분별검측세포조망화B림파세포백혈병/림파류단백2(Bcl-2)단백적표체.결과 (1)전염후48 h,IGF1R mRNA화단백적표체수평균명현하조,전염후IGF1R mRNA적표체수평하조료85.5%(P<0.01).(2)전염후48、72、96 h,세포증식피명현억제,세포증식활성분별위1.71±0.13、2.32±0.23、2.79±0.28,여미전염급전염비특이성siRNA적대조세포비교,차이균유통계학의의(P<0.01).(3)전염후48 h유24.37%적세포처우G2기(P<0.05).(4)전염후24 h연합불동농도적순박작용24 h,당순박농도위2.5、5、10、20μg/ml시,세포증식피명현억제,세포증식억제솔분별위(25.94±0.08)%、(40.25±0.05)%、(59.48±0.03)%、(74.18±0.08)%,차이균유통계학의의(P<0.01).(5)재전염siRNA 24 h후급여10μg/ml순박작용24 h,가사세포적조망솔증가지17.95%(P<0.05),병사Bcl-2단백적표체수평하조.결론 통과RNAi기술가유효억제IGF1R기인재전록화번역수평적표체,억제종류세포적증식,출현G2기조체,명현제고세포대순박화료적민감성.
Objective To assess the effect of suppression of insulin-like growth factor-1 receptor (IGF1R)in HO8910PM cell line by small interference RNA(siRNA).Methods Transfection of siRNA using liporectamine 2000 was conducted to silence IGF1R gene expression,the expression levels of IGF1R mRNA and protein were evaluated,and the effects on the cell cycles at 48 hours of transfection were assessed by real-time PCR,western blot and flow cytometry(FCM)assay respectively.The cell growth was detected by cell counting kit-8(CCK-8)at 24,48,72,96 hours of transfection.After 24 hours of transfection,the cells were cuhured with difierent concentrations of cisplatin(DDP)for 24 hours,the cell growth inhibition rate Was evaluated by CCK-8.Following incubation with 10μg/ml DDP for 24 hours after 24 hours of transfection,the apoptosis cells and the protein expression level of apoptosis-related gene,B cell leukemia/lymphoma 2(Bcl-2),were identified by FCM and western blot respectively.Resuits (1)Expression levels of IGF1R mRNA and protein were markedly decreased respectively at 48 hours of transfection IGF1R siRNA.(2)Suppression of IGF1R accompanied the reduction of cell growth at 48,72,96 hours of transfection with IGF1R siRNA,absorbance were 1.71±0.13,2.32±0.23,2.79±0.28 respectively (P<0.01).(3)IGF1R siRNA induces arrest of G2 phase,the G2 phase rate of cells were 24.37%(P<0.05).(4)Following treatment with 2.5,5,10,20μg/ml DDP for 24 hours after 24 hours of transfection,the cell growth inhibition rates were(25.94±0.08)%,(40.25±0.05)%,(59.48±0.03)%and(74.18±0.08)%respectively(P<0.01).(5)Treatment with 10μg/ml DDP for 24 hours after 24 hours of transfection,induces 17.95%of cells apoptosis(P<0.05),and decreases Bcl-2 protein level.Conclusion RNA interference of IGF1R gene induces the IGF1R silence in HO8910PM cell line significantly,inhibits cell growth in vitro, arrests the G2 phase, and enhances the chemosensitization to DDP.
