Gordon-Shaag Ariela, Yosef Yael, Abd El-Latif Mahmoud, Oppenheim Ariella
Department of Hematology, The Hebrew University-Hadassah Medical School and Hadassah University Hospital, Ein Kerem, Jerusalem, Israel 91120.
J Virol. 2003 Apr;77(7):4273-82. doi: 10.1128/jvi.77.7.4273-4282.2003.
The abundant nuclear enzyme poly(ADP-ribose) polymerase (PARP) functions in DNA damage surveillance and repair and at the decision between apoptosis and necrosis. Here we show that PARP binds to simian virus 40 (SV40) capsid proteins VP1 and VP3. Furthermore, its enzymatic activity is stimulated by VP3 but not by VP1. Experiments with purified mutant proteins demonstrated that the PARP binding domain in VP3 is localized to the 35 carboxy-terminal amino acids, while a larger peptide of 49 amino acids was required for full stimulation of its activity. The addition of 3-aminobenzamide (3-AB), a known competitive inhibitor of PARP, demonstrated that PARP participates in the SV40 life cycle. The titer of SV40 propagated on CV-1 cells was reduced by 3-AB in a dose-dependent manner. Additional experiments showed that 3-AB did not affect viral DNA replication or capsid protein production. PARP did not modify the viral capsid proteins in in vitro poly(ADP-ribosylation) assays, implying that it does not affect SV40 infectivity. On the other hand, it greatly reduced the magnitude of the host cytopathic effects, a hallmark of SV40 infection. Additional experiments suggested that the stimulation of PARP activity by VP3 leads the infected cell to a necrotic pathway, characterized by the loss of membrane integrity, thus facilitating the release of mature SV40 virions from the cells. Our studies identified a novel function of the minor capsid protein VP3 in the recruitment of PARP for the SV40 lytic process.
丰富的核酶聚(ADP - 核糖)聚合酶(PARP)在DNA损伤监测与修复以及细胞凋亡与坏死的抉择中发挥作用。在此我们表明,PARP与猿猴病毒40(SV40)衣壳蛋白VP1和VP3结合。此外,其酶活性受VP3刺激,但不受VP1刺激。对纯化的突变蛋白进行的实验表明,VP3中的PARP结合结构域定位于35个羧基末端氨基酸,而其活性的充分刺激则需要一个49个氨基酸的更大肽段。添加已知的PARP竞争性抑制剂3 - 氨基苯甲酰胺(3 - AB)表明,PARP参与SV40的生命周期。在CV - 1细胞上繁殖的SV40滴度因3 - AB呈剂量依赖性降低。额外的实验表明,3 - AB不影响病毒DNA复制或衣壳蛋白产生。在体外聚(ADP - 核糖基化)测定中,PARP未修饰病毒衣壳蛋白,这意味着它不影响SV40的感染性。另一方面,它极大地降低了宿主细胞病变效应的程度,这是SV40感染的一个标志。额外的实验表明,VP3对PARP活性的刺激使受感染细胞走向坏死途径,其特征是膜完整性丧失,从而促进成熟SV40病毒粒子从细胞中释放。我们的研究确定了小衣壳蛋白VP3在招募PARP参与SV40裂解过程中的新功能。