安徽医科大学学报
安徽醫科大學學報
안휘의과대학학보
ACTA UNIVERSITY MEDICINALIS ANHUI
2015年
6期
740-743,744
,共5页
李佳%卞尔保%贺小军%马春春%宗钢%王洪亮%赵兵
李佳%卞爾保%賀小軍%馬春春%宗鋼%王洪亮%趙兵
리가%변이보%하소군%마춘춘%종강%왕홍량%조병
胶质瘤%基因%转染%细胞增殖
膠質瘤%基因%轉染%細胞增殖
효질류%기인%전염%세포증식
glioblastoma%DNMT1%transfection%cell proliferation
目的:应用靶向 DNA 甲基转移酶1(DNMT1)基因的小干扰 RNA(siRNA)重组质粒来转染体外培养的人脑胶质瘤细胞,观察其对胶质瘤细胞增殖活性的影响。方法实验组予以 siRNA-DNMT1序列进行转染,对照组仅予以 siRNA-阴性对照序列。应用 qRT-PCR 分析 DNMT1基因表达变化, Western blot 法分析 DNMT1、PCNA 和 Cyclin D1蛋白表达变化,MTT 法检测细胞增殖生长能力,细胞克隆法分析细胞增殖克隆形成能力。结果与对照组比较,qRT-PCR 结果表明实验组 DNMT1 mRNA 表达明显减少( P <0.01);Western blot 法表明实验组 DNMT1、PCNA 和 Cyclin D1蛋白表达水平明显降低(P <0.01);MTT 法检测表明实验组中活细胞数明显低于对照组(P <0.05);细胞克隆法表明实验组细胞的增殖克隆形成能力明显低于对照组( P <0.01)。结论靶向 DNMT1基因的 siRNA 重组质粒可减少人脑胶质瘤细胞内 DNMT1基因的表达,从而抑制胶质瘤细胞的增殖。
目的:應用靶嚮 DNA 甲基轉移酶1(DNMT1)基因的小榦擾 RNA(siRNA)重組質粒來轉染體外培養的人腦膠質瘤細胞,觀察其對膠質瘤細胞增殖活性的影響。方法實驗組予以 siRNA-DNMT1序列進行轉染,對照組僅予以 siRNA-陰性對照序列。應用 qRT-PCR 分析 DNMT1基因錶達變化, Western blot 法分析 DNMT1、PCNA 和 Cyclin D1蛋白錶達變化,MTT 法檢測細胞增殖生長能力,細胞剋隆法分析細胞增殖剋隆形成能力。結果與對照組比較,qRT-PCR 結果錶明實驗組 DNMT1 mRNA 錶達明顯減少( P <0.01);Western blot 法錶明實驗組 DNMT1、PCNA 和 Cyclin D1蛋白錶達水平明顯降低(P <0.01);MTT 法檢測錶明實驗組中活細胞數明顯低于對照組(P <0.05);細胞剋隆法錶明實驗組細胞的增殖剋隆形成能力明顯低于對照組( P <0.01)。結論靶嚮 DNMT1基因的 siRNA 重組質粒可減少人腦膠質瘤細胞內 DNMT1基因的錶達,從而抑製膠質瘤細胞的增殖。
목적:응용파향 DNA 갑기전이매1(DNMT1)기인적소간우 RNA(siRNA)중조질립래전염체외배양적인뇌효질류세포,관찰기대효질류세포증식활성적영향。방법실험조여이 siRNA-DNMT1서렬진행전염,대조조부여이 siRNA-음성대조서렬。응용 qRT-PCR 분석 DNMT1기인표체변화, Western blot 법분석 DNMT1、PCNA 화 Cyclin D1단백표체변화,MTT 법검측세포증식생장능력,세포극륭법분석세포증식극륭형성능력。결과여대조조비교,qRT-PCR 결과표명실험조 DNMT1 mRNA 표체명현감소( P <0.01);Western blot 법표명실험조 DNMT1、PCNA 화 Cyclin D1단백표체수평명현강저(P <0.01);MTT 법검측표명실험조중활세포수명현저우대조조(P <0.05);세포극륭법표명실험조세포적증식극륭형성능력명현저우대조조( P <0.01)。결론파향 DNMT1기인적 siRNA 중조질립가감소인뇌효질류세포내 DNMT1기인적표체,종이억제효질류세포적증식。
Objective To transfect the human glioblastoma cells in vitro with the siRNA sequence targeting to DNA methyltransferase 1(DNMT1)gene,and investigate its effect on proliferation of human glioblastoma cells. Methods The experimental group was transfected by siRNA-DNMT1 sequence and the control group was given the siRNA negative sequence. The expression of DNMT1 gene was confirmed by qRT-PCR. The expression of DNMT1,PCNA and Cyclin D1,which were usually used as cell proliferation markers,was analyzed by Western blot. Cell survival and proliferation rate were determined by MTT and colony formation assay. Results Compared with the control group,qRT-PCR results showed that DNMT1 mRNA level was significantly decreased in DNMT1 siRNA transfected cells(P < 0. 01). The protein expression levels of DNMT1,PCNA and Cyclin D1 were dramatically reduced in the experimental group as detected by Western blot( P < 0. 01). MTT and colony formation assay results suggested that,the experimental group had a much lower cell survival(P < 0. 05)and proliferation rate(P < 0. 01). Conclu-sion The expression of DNMT1 gene of human glioblastoma cells in vitro is decreased by siRNA sequence targeting to DNMT1 gene,and the proliferation of human glioblastoma cells is also inhibited.