吉林农业大学学报
吉林農業大學學報
길임농업대학학보
JOURNAL OF JILIN AGRICUL TURAL UNIVERSITY
2014年
2期
199-204,212
,共7页
赵茂鑫%于海滨%李傲楠%赵志辉%杨润军%芦春艳
趙茂鑫%于海濱%李傲楠%趙誌輝%楊潤軍%蘆春豔
조무흠%우해빈%리오남%조지휘%양윤군%호춘염
FADD%RNAi载体%pAcGFP-N1%牛胎儿成纤维细胞
FADD%RNAi載體%pAcGFP-N1%牛胎兒成纖維細胞
FADD%RNAi재체%pAcGFP-N1%우태인성섬유세포
FADD%RNA interference(RNAi)vector%pAcGFP-N1%bovine fetal fibroblasts(BEF)
FADD(Fas-associated death domain protein)存在于 Fas/FasL系统中,是信号传导通路的一个信号连接蛋白,FADD通过传递凋亡信号,从而介导细胞凋亡。为进一步验证FADD基因抑制细胞增殖和促进细胞凋亡的作用,从牛卵巢组织中扩增 FADD基因,将 FADD基因连接到带有绿色荧光蛋白报告基因的真核表达载体pAcGFP-N1中,构建过表达FADD基因载体,并构建FADD基因的RNAi载体;用脂质体介导法将FADD基因RNAi载体、真核表达载体转染到牛胎儿成纤维细胞中,观察有无荧光的表达,并使用 Real-Time qPCR和West-ern blot方法检测FADD基因mRNA、蛋白水平的表达情况。结果表明:成功构建出FADD基因RNAi载体和高表达载体,重组质粒转染牛胎儿成纤维细胞24 h后在荧光显微镜下可观察到绿色荧光,转染效率可达50%。
FADD(Fas-associated death domain protein)存在于 Fas/FasL繫統中,是信號傳導通路的一箇信號連接蛋白,FADD通過傳遞凋亡信號,從而介導細胞凋亡。為進一步驗證FADD基因抑製細胞增殖和促進細胞凋亡的作用,從牛卵巢組織中擴增 FADD基因,將 FADD基因連接到帶有綠色熒光蛋白報告基因的真覈錶達載體pAcGFP-N1中,構建過錶達FADD基因載體,併構建FADD基因的RNAi載體;用脂質體介導法將FADD基因RNAi載體、真覈錶達載體轉染到牛胎兒成纖維細胞中,觀察有無熒光的錶達,併使用 Real-Time qPCR和West-ern blot方法檢測FADD基因mRNA、蛋白水平的錶達情況。結果錶明:成功構建齣FADD基因RNAi載體和高錶達載體,重組質粒轉染牛胎兒成纖維細胞24 h後在熒光顯微鏡下可觀察到綠色熒光,轉染效率可達50%。
FADD(Fas-associated death domain protein)존재우 Fas/FasL계통중,시신호전도통로적일개신호련접단백,FADD통과전체조망신호,종이개도세포조망。위진일보험증FADD기인억제세포증식화촉진세포조망적작용,종우란소조직중확증 FADD기인,장 FADD기인련접도대유록색형광단백보고기인적진핵표체재체pAcGFP-N1중,구건과표체FADD기인재체,병구건FADD기인적RNAi재체;용지질체개도법장FADD기인RNAi재체、진핵표체재체전염도우태인성섬유세포중,관찰유무형광적표체,병사용 Real-Time qPCR화West-ern blot방법검측FADD기인mRNA、단백수평적표체정황。결과표명:성공구건출FADD기인RNAi재체화고표체재체,중조질립전염우태인성섬유세포24 h후재형광현미경하가관찰도록색형광,전염효솔가체50%。
Fas-associated death domain protein(FADD)is connected to a signal protein signaling pathway in Fas/FasL system which mediates apoptosis guide by passing apoptotic signals .To further verify the function of FADD gene in inhibiting cell proliferation and promoting apoptosis,we cloned FADD gene in bovine ovary tissue with molecular cloning technique,directionally cloned the amplified FADD gene into eukaryotic expression vector pAcGFP-Nl including AcGFP and constructed the fusion protein recombinant plasmid .Using gene-silencing technology,we constructed RNA interference(RNAi)vector .And then we transfected pAcGFP-N1-FADD and RNAi into bovine fetal fibroblasts(BEF)cell mediated by Lipofec-tamine 2000,observed the expression of AcGFP and detected the mRNA and protein level of FADD by Real-Time qPCR and Western blot .The results showed that cattle FADD gene was successfully cloned, and RNAi vectors and pAcGFP-N1-FADD fusion protein eukaryotic expression vector were successfully constructed .Recombinant plasmid bovine fetal fibroblasts (BEF)under a fluorescence microscope after 24 h green fluorescence were observed,and the transfection efficiency was up to 50%.In this study,we used Real-Time qPCR and Western blot methods to verify the changes of FADD in gene expression level after transfection,and provided an experimental basis for the subsequent induction of apoptosis gene and further study of FADD materials .
