Braithwaite A W, Cheetham B F, Li P, Parish C R, Waldron-Stevens L K, Bellett A J
J Virol. 1983 Jan;45(1):192-9. doi: 10.1128/JVI.45.1.192-199.1983.
Mutants dl312, dl314, hr1, and hr3 with mutations in region E1A of adenovirus type 5 were defective for the induction of cell cycle abnormalities detectable by flow cytometry, cell DNA replication, thymidine kinase production, and chromosome aberrations and did not synthesize the viral DNA-binding protein (E2A) in rat cells. dl311, a leaky E1A mutant, induced cell cycle effects at high multiplicity in only one of three experiments, and synthesized the DNA-binding protein. hr7 (E1B) gave a wild-type response in all tests. dl313 was also positive in all tests, although it induced fewer polyploid cells than did wild-type virus, probably because of the leftward extension of the dl313 E1B deletion into E1A. sub315 and sub316, with mutations which also span the E1A-E1B border, synthesized DNA-binding protein, but caused no cell cycle alterations detectable by flow cytometry in rat or mouse cells. Although the participation of other viral early regions cannot be completely excluded, our results suggest that alteration of cell cycle progression is a direct effect of E1A unrelated to its control of other viral early regions, and may be the function of E1A in transformation.
5型腺病毒E1A区域发生突变的突变体dl312、dl314、hr1和hr3,在通过流式细胞术检测细胞周期异常、细胞DNA复制、胸苷激酶产生以及染色体畸变方面存在缺陷,并且在大鼠细胞中不合成病毒DNA结合蛋白(E2A)。漏出型E1A突变体dl311仅在三个实验中的一个实验中以高感染复数诱导了细胞周期效应,并且合成了DNA结合蛋白。hr7(E1B)在所有测试中均给出野生型反应。dl313在所有测试中也呈阳性,尽管它诱导产生的多倍体细胞比野生型病毒少,这可能是因为dl313的E1B缺失向左延伸到了E1A区域。sub315和sub316的突变也跨越了E1A - E1B边界,它们合成了DNA结合蛋白,但在大鼠或小鼠细胞中通过流式细胞术未检测到细胞周期改变。尽管不能完全排除其他病毒早期区域的参与,但我们的结果表明,细胞周期进程的改变是E1A的直接作用,与其对其他病毒早期区域的控制无关,并且可能是E1A在转化中的功能。
