Yamano S, Tokino T, Yasuda M, Kaneuchi M, Takahashi M, Niitsu Y, Fujinaga K, Yamashita T
Department of Molecular Biology, Cancer Research Institute, Sapporo Medical University School of Medicine, Chuo-ku, Japan.
J Virol. 1999 Dec;73(12):10095-103. doi: 10.1128/JVI.73.12.10095-10103.1999.
Adenovirus (Ad) E4orf6/7, one of the early gene products of human Ads, forms a stable complex with the cellular transcription factor E2F to activate transcription from the Ad E2 promoter. E2F cDNAs have growth-promoting and apoptosis-inducing activities when overexpressed in cells. We cloned Ad5 E4orf6/7 cDNA in both simian virus 40- and human cytomegalovirus-based expression vectors to examine its transforming and apoptotic activities. The cloned E4orf6/7 collaborated with a retinoblastoma protein (RB)-nonbinding and therefore E2F-nonreleasing mutant of Ad5 E1A (dl922/947) to morphologically transform primary rat cells, suggesting that E2F is an important cellular protein functioning downstream of E1A for transformation. In a G418 colony formation assay, E4orf6/7 was shown to suppress growth of untransformed rat cells. Moreover, a recombinant Ad expressing Ad5 E4orf6/7 induced apoptosis in rat cells when coinfected with wild-type p53-expressing Ad. Mutational analysis of E4orf6/7 revealed that both of the domains required for growth inhibition and transformation by E4orf6/7 lay in the C-terminal region, which is essential for transactivation from the upstream sequence of an E2a promoter containing E2F-binding sites. However, the smallest mutant of E4orf6/7, encoding the C-terminal 59 amino acids, failed to complement the RB-nonbinding dl922/947 mutant despite showing growth inhibition and E2F transactivation activities. Thus, it is suggested that a subregion of E4orf6/7 which is required for growth inhibition and transformation in collaboration with dl922/947 overlaps the transactivation domain of E4orf6/7.
腺病毒(Ad)E4orf6/7是人类腺病毒的早期基因产物之一,它与细胞转录因子E2F形成稳定复合物,以激活腺病毒E2启动子的转录。当在细胞中过表达时,E2F cDNA具有促进生长和诱导凋亡的活性。我们将Ad5 E4orf6/7 cDNA克隆到基于猿猴病毒40和人巨细胞病毒的表达载体中,以检测其转化和凋亡活性。克隆的E4orf6/7与腺病毒5型E1A的视网膜母细胞瘤蛋白(RB)非结合且因此E2F非释放突变体(dl922/947)协同作用,使原代大鼠细胞发生形态转化,这表明E2F是E1A下游发挥转化功能的重要细胞蛋白。在G418集落形成试验中,E4orf6/7被证明可抑制未转化大鼠细胞的生长。此外,表达Ad5 E4orf6/7的重组腺病毒在与表达野生型p53的腺病毒共感染时可诱导大鼠细胞凋亡。对E4orf6/7的突变分析表明,E4orf6/7抑制生长和转化所需的两个结构域均位于C末端区域,该区域对于从含有E2F结合位点的E2a启动子上游序列进行反式激活至关重要。然而,编码C末端59个氨基酸的E4orf6/7最小突变体,尽管具有生长抑制和E2F反式激活活性,但未能补充RB非结合的dl922/947突变体。因此,提示E4orf6/7与dl922/947协同作用时抑制生长和转化所需的一个亚区域与E4orf6/7的反式激活结构域重叠。