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NF1 家族转录因子对 BK 病毒 DNA 复制的刺激作用。

Stimulation of BK virus DNA replication by NFI family transcription factors.

机构信息

Department of Biochemistry and Genetics Area Program, University of Missouri—Columbia, Columbia, Missouri, USA.

出版信息

J Virol. 2012 Mar;86(6):3264-75. doi: 10.1128/JVI.06369-11. Epub 2011 Dec 28.

Abstract

BK polyomavirus (BKV) establishes persistent, low-level, and asymptomatic infections in most humans and causes polyomavirus-associated nephropathy (PVAN) and other pathologies in some individuals. The activation of BKV replication following kidney transplantation, leading to viruria, viremia, and, ultimately, PVAN, is associated with immune suppression as well as inflammation and stress from ischemia-reperfusion injury of the allograft, but the stimuli and molecular mechanisms leading to these pathologies are not well defined. The replication of BKV DNA in cell cultures is regulated by the viral noncoding control region (NCCR) comprising the core origin and flanking sequences, to which BKV T antigen (Tag), cellular proteins, and small regulatory RNAs bind. Six nuclear factor I (NFI) binding sites occur in sequences flanking the late side of the core origin (the enhancer) of the archetype virus, and their mutation, either individually or in toto, reduces BKV DNA replication when placed in competition with templates containing intact BKV NCCRs. NFI family members interacted with the helicase domain of BKV Tag in pulldown assays, suggesting that NFI helps recruit Tag to the viral core origin and may modulate its function. However, Tag may not be the sole target of the replication-modulatory activities of NFI: the NFIC/CTF1 isotype stimulates BKV template replication in vitro at low concentrations of DNA polymerase-α primase (Pol-primase), and the p58 subunit of Pol-primase associates with NFIC/CTF1, suggesting that NFI also recruits Pol-primase to the NCCR. These results suggest that NFI proteins (and the signaling pathways that target them) activate BKV replication and contribute to the consequent pathologies caused by acute infection.

摘要

BK 多瘤病毒(BKV)在大多数人中建立持续的、低水平的无症状感染,并在某些个体中引起多瘤病毒相关肾病(PVAN)和其他病变。肾移植后 BKV 复制的激活导致尿病毒血症、病毒血症,并最终导致 PVAN,这与免疫抑制以及同种异体移植物缺血再灌注损伤引起的炎症和应激有关,但导致这些病变的刺激物和分子机制尚不清楚。BKV DNA 在细胞培养物中的复制受病毒非编码控制区(NCCR)调节,该区域由核心起点和侧翼序列组成,BKV T 抗原(Tag)、细胞蛋白和小调节 RNA 结合到该区域。原型病毒核心起点(增强子)侧翼的晚期侧有六个核因子 I(NFI)结合位点,当与包含完整 BKV NCCR 的模板竞争时,这些位点的突变(单独或全部)会降低 BKV DNA 复制。NFI 家族成员在下拉测定中与 BKV Tag 的解旋酶结构域相互作用,表明 NFI 有助于将 Tag 募集到病毒核心起点,并可能调节其功能。然而,Tag 可能不是 NFI 复制调节活性的唯一靶标:NFIC/CTF1 同工型在低浓度 DNA 聚合酶-α引发酶(Pol-primase)下体外刺激 BKV 模板复制,Pol-primase 的 p58 亚基与 NFIC/CTF1 结合,表明 NFI 也将 Pol-primase 募集到 NCCR。这些结果表明,NFI 蛋白(以及针对它们的信号通路)激活 BKV 复制,并导致急性感染引起的后续病变。

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