Efficient Fas-ligand gene expression in rodent liver after intravenous injection of a recombinant adenovirus by the use of a Cre-mediated switching system

Cre重组酶 生物 分子生物学 Fas配体 转基因 遗传增强 转染 病毒载体 Jurkat细胞 基因表达 基因传递 基因 腺病毒科 互补DNA 重组DNA 重组酶 细胞凋亡 转基因小鼠 免疫学 程序性细胞死亡 遗传学 免疫系统 T细胞 重组
作者
Torayuki Okuyama,Masaie Fujino,Li Xk,Naoko Funeshima,Motomichi Kosuga,Izumu Saito,Seiichi Suzuki,Masahiro Yamada
出处
期刊:Gene Therapy [Springer Nature]
卷期号:5 (8): 1047-1053 被引量:49
标识
DOI:10.1038/sj.gt.3300704
摘要

An adenovirus vector AxCALNFasL was constructed in order to transduce a gene for rat Fas-ligand, requiring co-expression of Cre recombinase for its expression. In the cosmid cassette, pAxCALNFasL, a stuffer DNA fragment flanked with two loxP sequences was placed between the promoter and Fas-ligand cDNA to prevent its expression in transfected 293 cells. COS-7 cells infected with AxCALNFasL alone did not induce apoptosis in cocultivated Jurkat cells, but the cells treated with AxCALNFasL and AxCANCre (an adenovirus expressing Cre recombinase with the CAG promoter) did. BALB/c mice injected with 109 plaque-forming units of AxCALNFasL and with different doses of AxCANCre, developed lethal acute liver failure. The number of the apoptotic hepatocytes increased dramatically with increased doses of injected AxCANCre, indicating that the level of transgene expression in the rodent liver appeared to be adjustable. Based on these observations, we conclude that vectors expressing a gene to produce cytotoxic substances can be constructed by the use of a Cre-mediated switching system. Our system also demonstrated that efficient expression of the toxic gene in the rodent liver was achievable by co-infection of adenovirus vectors carrying the target gene and Cre recombinase.
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