中华实验外科杂志
中華實驗外科雜誌
중화실험외과잡지
Chinese Journal of Experimental Surgery
2015年
9期
2064-2067
,共4页
马可%周海霞%田男%田宇%韩亮
馬可%週海霞%田男%田宇%韓亮
마가%주해하%전남%전우%한량
胶质瘤%同源异形盒基因家族成员B1%微小RNA-3175
膠質瘤%同源異形盒基因傢族成員B1%微小RNA-3175
효질류%동원이형합기인가족성원B1%미소RNA-3175
Glioma%Homeobox B1%MicroRNA-3175
目的 观察在人胶质瘤细胞中微小RNA(miRNA,miR)-3175通过3'端非编码区(3'-UTR)对同源异形盒基因家族成员B1(HOXB1)表达的调控作用.方法 通过生物信息学可见miR-3175与HOXB1基因3'-UTR相互配对,构建HOXB1基因3'-UTR野生型和变异型荧光素酶载体,生物合成miR-3175 mimics、miR-3175 inhibitor和各自阴性对照.采用Lipofectamine 2000转染和双荧光素酶报告基因系统检测人胶质瘤细胞株(A172、U87)中miR-3175对HOXB1基因3'-UTR的调控作用.寡核苷酸转染24、48、72 h后,通过实时定量反转录聚合酶链反应(RT-qPCR)和Western blot分析miR-3175在人胶质瘤细胞株(A172、U251、U87)对HOXB1基因的表达调控.结果 双荧光素酶报告基因系统提示共转染HOXB1基因野生型载体和miR-3175 mimics后荧光素酶活性明显下降(P<0.05),A172细胞株荧光素酶活性下降(37.38±10.98)%,U87细胞株荧光索酶活性下降(24.62±3.22)%.与对照组比较miR-3175 mimics可下调HOXB1基因的表达,转染72h后HOXB1 mRNA表达水平在A172细胞株中下降(42.57±5.52)%,U251细胞株中下降(71.06±0.41)%,U87细胞株中下降(55.54±7.57)%;miR-3175 inhibitor可上调HOXB1基因的表达,转染72 h后HOXB1 mRNA表达水平在A172细胞株中升高(92.39±31.88)%,U251细胞株中升高(250.25±60.37)%,U87细胞株中升高(128.44±25.11)%.转染后HOXB1蛋白水平的变化也得出了相类似的结果.结论 HOXB1基因3'-UTR为miR-3175调控直接靶点,并且miR-3175 mimics为靶向负调控,miR-3175 inhibitor为靶向正调控.
目的 觀察在人膠質瘤細胞中微小RNA(miRNA,miR)-3175通過3'耑非編碼區(3'-UTR)對同源異形盒基因傢族成員B1(HOXB1)錶達的調控作用.方法 通過生物信息學可見miR-3175與HOXB1基因3'-UTR相互配對,構建HOXB1基因3'-UTR野生型和變異型熒光素酶載體,生物閤成miR-3175 mimics、miR-3175 inhibitor和各自陰性對照.採用Lipofectamine 2000轉染和雙熒光素酶報告基因繫統檢測人膠質瘤細胞株(A172、U87)中miR-3175對HOXB1基因3'-UTR的調控作用.寡覈苷痠轉染24、48、72 h後,通過實時定量反轉錄聚閤酶鏈反應(RT-qPCR)和Western blot分析miR-3175在人膠質瘤細胞株(A172、U251、U87)對HOXB1基因的錶達調控.結果 雙熒光素酶報告基因繫統提示共轉染HOXB1基因野生型載體和miR-3175 mimics後熒光素酶活性明顯下降(P<0.05),A172細胞株熒光素酶活性下降(37.38±10.98)%,U87細胞株熒光索酶活性下降(24.62±3.22)%.與對照組比較miR-3175 mimics可下調HOXB1基因的錶達,轉染72h後HOXB1 mRNA錶達水平在A172細胞株中下降(42.57±5.52)%,U251細胞株中下降(71.06±0.41)%,U87細胞株中下降(55.54±7.57)%;miR-3175 inhibitor可上調HOXB1基因的錶達,轉染72 h後HOXB1 mRNA錶達水平在A172細胞株中升高(92.39±31.88)%,U251細胞株中升高(250.25±60.37)%,U87細胞株中升高(128.44±25.11)%.轉染後HOXB1蛋白水平的變化也得齣瞭相類似的結果.結論 HOXB1基因3'-UTR為miR-3175調控直接靶點,併且miR-3175 mimics為靶嚮負調控,miR-3175 inhibitor為靶嚮正調控.
목적 관찰재인효질류세포중미소RNA(miRNA,miR)-3175통과3'단비편마구(3'-UTR)대동원이형합기인가족성원B1(HOXB1)표체적조공작용.방법 통과생물신식학가견miR-3175여HOXB1기인3'-UTR상호배대,구건HOXB1기인3'-UTR야생형화변이형형광소매재체,생물합성miR-3175 mimics、miR-3175 inhibitor화각자음성대조.채용Lipofectamine 2000전염화쌍형광소매보고기인계통검측인효질류세포주(A172、U87)중miR-3175대HOXB1기인3'-UTR적조공작용.과핵감산전염24、48、72 h후,통과실시정량반전록취합매련반응(RT-qPCR)화Western blot분석miR-3175재인효질류세포주(A172、U251、U87)대HOXB1기인적표체조공.결과 쌍형광소매보고기인계통제시공전염HOXB1기인야생형재체화miR-3175 mimics후형광소매활성명현하강(P<0.05),A172세포주형광소매활성하강(37.38±10.98)%,U87세포주형광색매활성하강(24.62±3.22)%.여대조조비교miR-3175 mimics가하조HOXB1기인적표체,전염72h후HOXB1 mRNA표체수평재A172세포주중하강(42.57±5.52)%,U251세포주중하강(71.06±0.41)%,U87세포주중하강(55.54±7.57)%;miR-3175 inhibitor가상조HOXB1기인적표체,전염72 h후HOXB1 mRNA표체수평재A172세포주중승고(92.39±31.88)%,U251세포주중승고(250.25±60.37)%,U87세포주중승고(128.44±25.11)%.전염후HOXB1단백수평적변화야득출료상유사적결과.결론 HOXB1기인3'-UTR위miR-3175조공직접파점,병차miR-3175 mimics위파향부조공,miR-3175 inhibitor위파향정조공.
Objective To explore the regulation of homeobox B1 (HOXB1) gene by microRNA (miRNA,miR)-3175 targeting 3' untranslated region (3'-UTR) in the human glioma cell line.Methods Bioinformatics analysis was applied to predict the HOXB1 gene 3'-UTR targeted miRNA.The wild-type and mutation-type of HOXB1 gene 3'-UTR luciferase vectors were constructed.MiR-3175 mimics,miR-3175 inhibitor and their negative controls were bio-synthetized.Lipofectamine 2000 transfection and the Dual Luciferase Reporter Gene System were applied to detect the effect of miR-3175 on the HOXB1 gene 3'-UTR in the human glioma cell lines (A172 and U87).Real-time quantitative reverse transcriptase-polymerase chain reaction (RT-qPCR) and Western blotting were performed to analyze the regulation of HOXB1 gene expression by miR-3175 in the human glioma cell lines (A172,U251 and U87) after oligonucleotide transfection in 24,48,and 72 h.Results The luciferase assay revealed that miR-3175 mimics could significantly down-regulate the luciferase activity of the wild-type HOXB1 gene vector.The luciferase activity of A172 cell line was declined by (37.38 ± 10.98)% and that of U87 cell line by (24.62 ± 3.22)% respectively.MiR-3175 mimics could decrease the expression of HOXB1 gene.After transfection over 72 h,the HOXB1 mRNA expression levels were decreased by (42.57 ± 5.52) % in A172 cell line,(71.06 ± 0.41) % in U251 cell line,and (55.54 ± 7.57) % in U87 cell line.MiR-3175 inhibitor increased the expression of HOXB1 gene.After transfection over 72 h,HOXB1 mRNA expression levels were elevated by (92.39 ±31.88)% in A172 cell line,(250.25 ±60.37)% in U251 cell line,and (128.44 ± 25.11)% in U87 cell line.The similar results were obtained about the change of HOXB1 protein levels.Conclusion HOXB1 gene 3'-UTR is a direct target of rniR-3175.MiR-3175 mimics is negative regulation for target,and miR-3175 inhibitor is positive regulation.
