Over-expression and RNAi Vector Construction of Cattle FADD Gene and Its Expression in Bovine Fetal Fibroblasts

ZHAO Mao-xin;YU Hai-bin;LI Ao-nan;ZHAO Zhi-hui;YANG Run-jun;LU Chun-yan;College of Animal Science,Jilin University;Experimental Base of Agriculture,Jilin University;

FADD;;RNA interference(RNAi) vector;;pAcGFP-N1;;bovine fetal fibroblasts(BEF)

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 Lipofectamine 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.