基础医学与临床
基礎醫學與臨床
기출의학여림상
Basic & Clinical Medicine
2015年
1期
12-16
,共5页
张汝益%何方%王静%邓芳%李琪英%施琼
張汝益%何方%王靜%鄧芳%李琪英%施瓊
장여익%하방%왕정%산방%리기영%시경
miR-30a%人骨肉瘤细胞%RUNX2
miR-30a%人骨肉瘤細胞%RUNX2
miR-30a%인골육류세포%RUNX2
miR-30a%human osteosarcoma cell line%RUNX2
目的:探讨miR-30a对人骨肉瘤细胞143B侵袭、迁移和细胞活力的影响。方法过表达或抑制miR-30a分别处理人骨肉瘤细胞143B。划痕实验观察细胞划痕愈合能力;Transwell 实验检测143B细胞迁移和侵袭能力;MTT实验检测细胞活力;定量PCR实验确认过表达miR-30a腺病毒有效性并且检测RUNX2 mRNA表达;Western blot检测细胞中RUNX2总蛋白表达。结果过表达miR-30a抑制了骨肉瘤细胞143B迁移和侵袭(P<0.05),在72 h时, miR-30a明显抑制细胞活力( P<0.01);抑制miR-30a的内源性表达后,143B细胞的迁移和侵袭能力增加( P<0.05),细胞活力也表现出上升水平( P<0.01);同时过表达miR-30 a可以抑制RUNX2的蛋白表达,抑制内源性miR-30a后RUNX2蛋白水平表达增加(P<0.05)。荧光素酶活性检测,miR-30a可以靶向于RUNX2(P<0.01)。结论 miR-30a抑制骨肉瘤细胞143B的迁移、侵袭和活力,其作用可以能是通过抑制RUNX2的表达来实现。
目的:探討miR-30a對人骨肉瘤細胞143B侵襲、遷移和細胞活力的影響。方法過錶達或抑製miR-30a分彆處理人骨肉瘤細胞143B。劃痕實驗觀察細胞劃痕愈閤能力;Transwell 實驗檢測143B細胞遷移和侵襲能力;MTT實驗檢測細胞活力;定量PCR實驗確認過錶達miR-30a腺病毒有效性併且檢測RUNX2 mRNA錶達;Western blot檢測細胞中RUNX2總蛋白錶達。結果過錶達miR-30a抑製瞭骨肉瘤細胞143B遷移和侵襲(P<0.05),在72 h時, miR-30a明顯抑製細胞活力( P<0.01);抑製miR-30a的內源性錶達後,143B細胞的遷移和侵襲能力增加( P<0.05),細胞活力也錶現齣上升水平( P<0.01);同時過錶達miR-30 a可以抑製RUNX2的蛋白錶達,抑製內源性miR-30a後RUNX2蛋白水平錶達增加(P<0.05)。熒光素酶活性檢測,miR-30a可以靶嚮于RUNX2(P<0.01)。結論 miR-30a抑製骨肉瘤細胞143B的遷移、侵襲和活力,其作用可以能是通過抑製RUNX2的錶達來實現。
목적:탐토miR-30a대인골육류세포143B침습、천이화세포활력적영향。방법과표체혹억제miR-30a분별처리인골육류세포143B。화흔실험관찰세포화흔유합능력;Transwell 실험검측143B세포천이화침습능력;MTT실험검측세포활력;정량PCR실험학인과표체miR-30a선병독유효성병차검측RUNX2 mRNA표체;Western blot검측세포중RUNX2총단백표체。결과과표체miR-30a억제료골육류세포143B천이화침습(P<0.05),재72 h시, miR-30a명현억제세포활력( P<0.01);억제miR-30a적내원성표체후,143B세포적천이화침습능력증가( P<0.05),세포활력야표현출상승수평( P<0.01);동시과표체miR-30 a가이억제RUNX2적단백표체,억제내원성miR-30a후RUNX2단백수평표체증가(P<0.05)。형광소매활성검측,miR-30a가이파향우RUNX2(P<0.01)。결론 miR-30a억제골육류세포143B적천이、침습화활력,기작용가이능시통과억제RUNX2적표체래실현。
Objective To investigate the effect of miR-30a on human osteosarcoma cell 143B in migration,invasion andcellviability.Methods 143BcellswereinfectedortransfectedwithrecombinantadenovirusmiR-30a(Ad-miR30a) and miR-30a inhibitor respectively .Wound healing assay was performed to detect the cell healing ability ( P<0.05 ) .Cell migration and invasion ability were determined by Transwell assay ( P<0.05 ) .The cell viability was analyzed by MTT assay ( P<0.01 ) .Real-time quantitative PCR was performed to analyze the expression of RUNX2 mRNA level and confirmed the adenovirus miR-30a expressed in 143B cells.The expression of RUNX2 was analyzed by Western blot .miR-30a target to RUNX2 was verified by luciferase reported gene assay .Results The ability of migration and invasion was suppressed in osteosarcoma cell 143B by overexpression miR-30a,and the cell viability also decreased .After the endogenous miR-30 a being inhibited , the cell motility and invasion enhanced and the cell viability was promoted .The RUNX2 protein decreased after overexpression miR-30 a as compared with controlgroup.TheluciferaseactivityofRUNX2decreasedbyaddingmiR-30a.Conclusions 143Bcellmigration, invasion and viability were suppressed by miR-30a,and this process is potentially achieved via suppressing RUNX 2 protein expression .
