四川医学
四川醫學
사천의학
SICHUAN MEDICAL JOURNAL
2015年
6期
827-830
,共4页
胃癌%CDK1%凋亡%增殖
胃癌%CDK1%凋亡%增殖
위암%CDK1%조망%증식
gastric cancer%CDKI%apoptosis%proliferation
目的:观察周期蛋白依赖性激酶1(CDK1)在胃癌细胞及永生化胃粘膜上皮细胞系中的表达,探讨其沉默对胃癌细胞恶性表型的影响。方法利用实时荧光定量PCR检测永生化胃粘膜上皮细胞系GES及胃癌细胞系SGC7901中CDK1的mRNA表达水平,应用RNA干扰技术沉默胃癌细胞系SGC7901的CDK1,运用流式细胞术检测沉默CDK1前后胃癌细胞的凋亡情况,绘制细胞的生长曲线,并通过克隆形成实验观察肿瘤细胞恶性表型的变化。结果 CDK1在胃癌细胞系SGC7901中表达明显高于永生化胃粘膜上皮细胞系GES。使用siRNA体外转染SGC7901细胞后胃癌细胞的凋亡率升高。 MTT结果显示与空白对照组和阴性对照相比,沉默CDK1后胃癌细胞增殖速度明显受到抑制( P<0.05)。克隆形成实验发现沉默CDK1后可明显减少胃癌细胞株的平板克隆数目。结论 CDK1在胃癌细胞中高表达,可能参与胃癌的发生发展,下调CDK1的表达可促进胃癌细胞凋亡、抑制胃癌细胞的恶性增殖。
目的:觀察週期蛋白依賴性激酶1(CDK1)在胃癌細胞及永生化胃粘膜上皮細胞繫中的錶達,探討其沉默對胃癌細胞噁性錶型的影響。方法利用實時熒光定量PCR檢測永生化胃粘膜上皮細胞繫GES及胃癌細胞繫SGC7901中CDK1的mRNA錶達水平,應用RNA榦擾技術沉默胃癌細胞繫SGC7901的CDK1,運用流式細胞術檢測沉默CDK1前後胃癌細胞的凋亡情況,繪製細胞的生長麯線,併通過剋隆形成實驗觀察腫瘤細胞噁性錶型的變化。結果 CDK1在胃癌細胞繫SGC7901中錶達明顯高于永生化胃粘膜上皮細胞繫GES。使用siRNA體外轉染SGC7901細胞後胃癌細胞的凋亡率升高。 MTT結果顯示與空白對照組和陰性對照相比,沉默CDK1後胃癌細胞增殖速度明顯受到抑製( P<0.05)。剋隆形成實驗髮現沉默CDK1後可明顯減少胃癌細胞株的平闆剋隆數目。結論 CDK1在胃癌細胞中高錶達,可能參與胃癌的髮生髮展,下調CDK1的錶達可促進胃癌細胞凋亡、抑製胃癌細胞的噁性增殖。
목적:관찰주기단백의뢰성격매1(CDK1)재위암세포급영생화위점막상피세포계중적표체,탐토기침묵대위암세포악성표형적영향。방법이용실시형광정량PCR검측영생화위점막상피세포계GES급위암세포계SGC7901중CDK1적mRNA표체수평,응용RNA간우기술침묵위암세포계SGC7901적CDK1,운용류식세포술검측침묵CDK1전후위암세포적조망정황,회제세포적생장곡선,병통과극륭형성실험관찰종류세포악성표형적변화。결과 CDK1재위암세포계SGC7901중표체명현고우영생화위점막상피세포계GES。사용siRNA체외전염SGC7901세포후위암세포적조망솔승고。 MTT결과현시여공백대조조화음성대조상비,침묵CDK1후위암세포증식속도명현수도억제( P<0.05)。극륭형성실험발현침묵CDK1후가명현감소위암세포주적평판극륭수목。결론 CDK1재위암세포중고표체,가능삼여위암적발생발전,하조CDK1적표체가촉진위암세포조망、억제위암세포적악성증식。
Objective The purpose of this study was to investigate the expression of cyclin dependent kinase 1(CDK1)in gastric cancer cell line SGC7901 and gastric epithelial cell line GES and study the effects of CDKl knockdown on the malignant be-havior of gastric cancer. Methods The expression of CDKl in gastric epithelial cell line GES and gastric cancer cell line SGC7901 were quantified using real-time quantitative polymerase chain reaction( Q-PCR) . The siRNA targeting the CDK1 gene was synthe-sized and transfected into SGC7901 cells by lipofectamine 2000. Cell apoptosis was detected by flow cytometry after the transfected for 48 or 60 h. MTT assay and colony formation assay were performed to examine the effect of CDKl on the cell growth and cell proliferation in vitro. Results CDK1 expression was significantly increased in gastric cancer cell line SGC7901 compared with gastric epithelial cell line GES. The ratio of apoptotic cell of transfected cells at 48h after transfection was increased significantly compared with control. Downregulation of CDK1 inhibited the growth and proliferation of gastric cancer cell compared with control, which was comfirmed by MTT and plate colony formation assays. Conclusion CDK1 expression was significantly increased in gas-tric cancer. Overexpression of CDK1 may promote oncogenesis and progression of human gastric cancer. Downregulation of CDK1 expression can prompt the apoptosis and inhibit the proliferation activities of human gastric cancer.
