Voitenleitner Christian, Botchan Michael
Department of Molecular and Cell Biology, Division of Biochemistry and Molecular Biology, University of California, Berkeley, California 94720, USA.
J Virol. 2002 Apr;76(7):3440-51. doi: 10.1128/jvi.76.7.3440-3451.2002.
Eukaryotic viruses can maintain latency in dividing cells as extrachromosomal plasmids. It is therefore of vital importance for viruses to ensure nuclear retention and proper segregation of their viral DNA. The bovine papillomavirus (BPV) E2 enhancer protein plays a key role in these processes by tethering the viral DNA to the host cell chromosomes. Viral genomes that harbor phosphorylation mutations in the E2 gene are transformation defective, and for these mutant genomes, neither the viral DNA nor the E2 protein is detected on mitotic chromosomes, while other key functions of E2 in transcription and replication were wild type. Moreover, secondary mutations in both the E2 and E1 proteins lead to suppression of the phosphorylation mutant phenotype and resulted in reattachment of the viral DNA and the E2 protein onto mitotic chromosomes, suggesting that E1 also plays a role in viral genome partitioning. The E1 protein was cytologically always excluded from mitotic chromatin, either as a suppressor allele or as the wild type. In the absence of other viral proteins, an E2 protein containing alanine substitutions for phosphorylation substrates in the hinge region (E2-A4) was detected as wild-type on mitotic chromosomes. However, when wild-type E1 protein levels were increased in cells expressing either the A4 mutant E2 proteins or wild-type E2, the E2-A4 protein was much more sensitive to chromosomal dislocation than was the wild-type protein. In contrast, suppressor alleles of E1 were not capable of such abrogation of E2 binding (A4 or wild-type) to chromosomes. These results suggest that wild-type E1 can be a negative regulator of the chromosomal attachment of E2.
真核病毒可作为染色体外质粒在分裂细胞中维持潜伏状态。因此,对于病毒而言,确保其病毒DNA在细胞核内保留并正确分离至关重要。牛乳头瘤病毒(BPV)E2增强子蛋白通过将病毒DNA tether到宿主细胞染色体上,在这些过程中发挥关键作用。在E2基因中携带磷酸化突变的病毒基因组具有转化缺陷,对于这些突变基因组,在有丝分裂染色体上既检测不到病毒DNA,也检测不到E2蛋白,而E2在转录和复制中的其他关键功能为野生型。此外,E2和E1蛋白中的二次突变导致磷酸化突变体表型受到抑制,并导致病毒DNA和E2蛋白重新附着到有丝分裂染色体上,这表明E1在病毒基因组分配中也发挥作用。无论是作为抑制等位基因还是野生型,E1蛋白在细胞学上总是被排除在有丝分裂染色质之外。在没有其他病毒蛋白的情况下,在铰链区含有磷酸化底物丙氨酸替代物的E2蛋白(E2-A4)在有丝分裂染色体上被检测为野生型。然而,当在表达A4突变E2蛋白或野生型E2的细胞中野生型E1蛋白水平增加时,E2-A4蛋白比野生型蛋白对染色体错位更敏感。相比之下,E1的抑制等位基因不能消除E2(A4或野生型)与染色体的结合。这些结果表明野生型E1可能是E2与染色体附着的负调节因子。