高效慢病毒整合不需要依赖DNA的蛋白激酶。
DNA-Dependent protein kinase is not required for efficient lentivirus integration.
作者信息
Baekelandt V, Claeys A, Cherepanov P, De Clercq E, De Strooper B, Nuttin B, Debyser Z
机构信息
Laboratory for Experimental Neurosurgery and Neuroanatomy, Katholieke Universiteit Leuven, Leuven, Belgium.
出版信息
J Virol. 2000 Dec;74(23):11278-85. doi: 10.1128/jvi.74.23.11278-11285.2000.
How DNA is repaired after retrovirus integration is not well understood. DNA-dependent protein kinase (DNA-PK) is known to play a central role in the repair of double-stranded DNA breaks. Recently, a role for DNA-PK in retroviral DNA integration has been proposed (R. Daniel, R. A. Katz, and A. M. Skalka, Science 284:644-647, 1999). Reduced transduction efficiency and increased cell death by apoptosis were observed upon retrovirus infection of cultured scid cells. We have used a human immunodeficiency virus (HIV) type 1 (HIV-1)-derived lentivirus vector system to further investigate the role of DNA-PK during integration. We measured lentivirus transduction of scid mouse embryonic fibroblasts (MEF) and xrs-5 or xrs-6 cells. These cells are deficient in the catalytic subunit of DNA-PK and in Ku, the DNA-binding subunit of DNA-PK, respectively. At low vector titers, efficient and stable lentivirus transduction was obtained, excluding an essential role for DNA-PK in lentivirus integration. Likewise, the efficiency of transduction of HIV-derived vectors in scid mouse brain was as efficient as that in control mice, without evidence of apoptosis. We observed increased cell death in scid MEF and xrs-5 or xrs-6 cells, but only after transduction with high vector titers (multiplicity of infection [MOI], >1 transducing unit [TU]/cell) and subsequent passage of the transduced cells. At an MOI of <1 TU/cell, however, transduction efficiency was even higher in DNA-PK-deficient cells than in control cells. Taken together, the data suggest a protective role of DNA-PK against cellular toxicity induced by high levels of retrovirus integrase or integration. Another candidate cellular enzyme that has been claimed to play an important role during retrovirus integration is poly(ADP-ribose) polymerase (PARP). However, no inhibition of lentivirus vector-mediated transduction or HIV-1 replication by 3-methoxybenzamide, a known PARP inhibitor, was observed. In conclusion, DNA-PK and PARP are not essential for lentivirus integration.
逆转录病毒整合后DNA如何修复尚未完全明确。已知DNA依赖性蛋白激酶(DNA-PK)在双链DNA断裂修复中起核心作用。最近,有人提出DNA-PK在逆转录病毒DNA整合中发挥作用(R. Daniel、R. A. Katz和A. M. Skalka,《科学》284:644 - 647,1999年)。在用逆转录病毒感染培养的严重联合免疫缺陷(scid)细胞后,观察到转导效率降低以及细胞凋亡导致的细胞死亡增加。我们使用了一种源自1型人类免疫缺陷病毒(HIV-1)的慢病毒载体系统,进一步研究DNA-PK在整合过程中的作用。我们检测了scid小鼠胚胎成纤维细胞(MEF)以及xrs-5或xrs-6细胞的慢病毒转导情况。这些细胞分别在DNA-PK的催化亚基以及DNA-PK的DNA结合亚基Ku方面存在缺陷。在低载体滴度下,获得了高效且稳定的慢病毒转导,排除了DNA-PK在慢病毒整合中的关键作用。同样,HIV衍生载体在scid小鼠脑中的转导效率与对照小鼠中的效率一样高,且没有细胞凋亡的迹象。我们在scid MEF和xrs-5或xrs-6细胞中观察到细胞死亡增加,但这仅发生在高载体滴度(感染复数[MOI],>1转导单位[TU]/细胞)转导以及转导后细胞传代之后。然而,在MOI <1 TU/细胞时,DNA-PK缺陷细胞中的转导效率甚至高于对照细胞。综合来看,数据表明DNA-PK对高水平逆转录病毒整合酶或整合所诱导的细胞毒性具有保护作用。另一种被认为在逆转录病毒整合过程中起重要作用的细胞酶是聚(ADP-核糖)聚合酶(PARP)。然而,未观察到已知的PARP抑制剂3-甲氧基苯甲酰胺对慢病毒载体介导的转导或HIV-1复制有抑制作用。总之,DNA-PK和PARP对慢病毒整合并非必不可少。
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