浙江医学
浙江醫學
절강의학
ZHEJIANG MEDICAL JOURNAL
2015年
9期
747-749,761
,共4页
张财明%季一鸣%朱敏%吕尚东%王爱东
張財明%季一鳴%硃敏%呂尚東%王愛東
장재명%계일명%주민%려상동%왕애동
Livin基因%RNA干扰%转染%panc-1细胞
Livin基因%RNA榦擾%轉染%panc-1細胞
Livin기인%RNA간우%전염%panc-1세포
Livin gene%RNA interference%Transfection%panc- 1 cell
目的:构建Livin shRNA真核表达载体,探讨干扰质粒稳定转染的胰腺癌panc-1细胞系效应。方法合成Livin基因干扰序列并定向插入到RNA干扰(RNAi)真核表达载体pGCsilencerTM U6/Neo/GFP/RNAi质粒,通过测序进行鉴定。干扰质粒经脂质体Lipofectamine 2000介导转染panc-1细胞。经G418持续压力选择和有限稀释法获得稳定转染的细胞系。定量RT- PCR检测所筛选克隆Livin mRNA的转录水平,采用western blot验证Livin蛋白表达水平改变。结果测序证明Livin干扰序列及读码框正确,干扰质粒稳定转染的panc-1细胞在倒置荧光显微镜下呈明亮绿色荧光,定量RT- PCR和western blot检测结果显示Livin shRNA序列对胰腺癌细胞系Livin mRNA及蛋白表达均有抑制作用。结论成功构建Livin shRNA真核表达载体,建立Livin shRNA质粒稳定转染的panc-1细胞系可为进一步研究Livin在胰腺癌细胞中的作用奠定基础。
目的:構建Livin shRNA真覈錶達載體,探討榦擾質粒穩定轉染的胰腺癌panc-1細胞繫效應。方法閤成Livin基因榦擾序列併定嚮插入到RNA榦擾(RNAi)真覈錶達載體pGCsilencerTM U6/Neo/GFP/RNAi質粒,通過測序進行鑒定。榦擾質粒經脂質體Lipofectamine 2000介導轉染panc-1細胞。經G418持續壓力選擇和有限稀釋法穫得穩定轉染的細胞繫。定量RT- PCR檢測所篩選剋隆Livin mRNA的轉錄水平,採用western blot驗證Livin蛋白錶達水平改變。結果測序證明Livin榦擾序列及讀碼框正確,榦擾質粒穩定轉染的panc-1細胞在倒置熒光顯微鏡下呈明亮綠色熒光,定量RT- PCR和western blot檢測結果顯示Livin shRNA序列對胰腺癌細胞繫Livin mRNA及蛋白錶達均有抑製作用。結論成功構建Livin shRNA真覈錶達載體,建立Livin shRNA質粒穩定轉染的panc-1細胞繫可為進一步研究Livin在胰腺癌細胞中的作用奠定基礎。
목적:구건Livin shRNA진핵표체재체,탐토간우질립은정전염적이선암panc-1세포계효응。방법합성Livin기인간우서렬병정향삽입도RNA간우(RNAi)진핵표체재체pGCsilencerTM U6/Neo/GFP/RNAi질립,통과측서진행감정。간우질립경지질체Lipofectamine 2000개도전염panc-1세포。경G418지속압력선택화유한희석법획득은정전염적세포계。정량RT- PCR검측소사선극륭Livin mRNA적전록수평,채용western blot험증Livin단백표체수평개변。결과측서증명Livin간우서렬급독마광정학,간우질립은정전염적panc-1세포재도치형광현미경하정명량록색형광,정량RT- PCR화western blot검측결과현시Livin shRNA서렬대이선암세포계Livin mRNA급단백표체균유억제작용。결론성공구건Livin shRNA진핵표체재체,건립Livin shRNA질립은정전염적panc-1세포계가위진일보연구Livin재이선암세포중적작용전정기출。
Objective To construct LivinshRNA eukaryotic expression vectors and to investigate its effect on ex-pression of Livin mRNA and protein in pancreatic cancer cel line panc- 1. Methods Livin gene interference sequence was synthesized and inserted into pGCsilencerTM U6/Neo/GFP/RNAi vector,which was confirmed by sequencing. The recombi-nant RNAi vector was transfected into pancreatic cancer panc- 1cel s by Lipofectamine 2000. The cel s containing stable transformants were selected by G418, and isolated with limited dilution. The mRNA expression of Livin in the selected clones was detected by RT- PCR, the protein expression of Livin was detected by Western blot. Results The successful construction of RNAi eukaryotic expression vectors targeting Livin was confirmed by sequencing, which was expressed in panc- 1 cel s after transfection as showed by green fluorescence under inverted fluorescence microscope. RT- PCR and West-ern blot revealed that the expression of Livin mRNA and protein was down- regulated in panc- 1 cel s. Conclusion Livin shRNA eukaryotie expression vector was successful y constructed and the transfected pancreatic cancer panc- 1 cel s show a down- regulated expression of Livin mRNA and protein.
