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表达猿猴病毒 40 大 T 抗原的细胞中的复制应激和有丝分裂功能障碍。

Replication stress and mitotic dysfunction in cells expressing simian virus 40 large T antigen.

机构信息

Molecular Oncology Research Institute, Tufts Medical Center, Boston, Massachusetts, USA.

出版信息

J Virol. 2013 Dec;87(24):13179-92. doi: 10.1128/JVI.02224-13. Epub 2013 Sep 25.

DOI:10.1128/JVI.02224-13
PMID:24067972
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3838287/
Abstract

We previously demonstrated that simian virus 40 (SV40) large T antigen (LT) binds to the Bub1 kinase, a key regulator of the spindle checkpoint and chromosome segregation. Bub1 mutations or altered expression patterns are linked to chromosome missegregation and are considered to be a driving force in some human cancers. Here we report that LT, dependent on Bub1 binding, causes micronuclei, lagging chromatin, and anaphase bridges, which are hallmarks of chromosomal instability (CIN) and Bub1 insufficiency. Using time-lapse microscopy, we demonstrate that LT imposes a Bub1 binding-dependent delay in the metaphase-to-anaphase transition. Kinetochore fibers reveal that LT, via Bub1 binding, causes aberrant kinetochore (KT)-microtubule (MT) attachments and a shortened interkinetochore distance, consistent with a lack of tension. Previously, we showed that LT also induces the DNA damage response (DDR) via Bub1 binding. Using inducible LT cell lines, we show that an activated DDR was observed before the appearance of anaphase bridges and micronuclei. Furthermore, LT induction in serum-starved cells demonstrated γ-H2AX accumulation in cells that had not yet entered mitosis. Thus, DDR activation can occur independently of chromosome segregation defects. Replication stress pathways may be responsible, because signatures of replication stress were observed, which were attenuated by exogenous supplementation with nucleosides. Our observations allow us to propose a model that explains and integrates the diverse manifestations of genomic instability induced by LT.

摘要

我们之前已经证明,猿猴病毒 40(SV40)大 T 抗原(LT)与 Bub1 激酶结合,后者是纺锤体检查点和染色体分离的关键调节因子。Bub1 突变或表达模式改变与染色体错误分离有关,被认为是某些人类癌症的驱动因素。在这里,我们报告 LT 通过依赖于 Bub1 结合导致微核、滞后染色质和后期桥,这些都是染色体不稳定性(CIN)和 Bub1 不足的标志。通过延时显微镜,我们证明 LT 对中期到后期的转变施加了 Bub1 结合依赖性的延迟。着丝粒纤维表明,LT 通过与 Bub1 结合导致异常的着丝粒(KT)-微管(MT)附着和缩短的动粒间距离,这与缺乏张力一致。此前,我们还表明 LT 通过与 Bub1 结合诱导 DNA 损伤反应(DDR)。通过诱导 LT 细胞系,我们发现 DDR 在出现后期桥和微核之前被激活。此外,在血清饥饿的细胞中诱导 LT 显示 γ-H2AX 在尚未进入有丝分裂的细胞中积累。因此,DDR 的激活可以独立于染色体分离缺陷发生。复制应激途径可能是负责的,因为观察到复制应激的特征,并且通过外源性核苷酸补充可以减弱这些特征。我们的观察结果使我们能够提出一个模型,该模型解释并整合了 LT 诱导的基因组不稳定性的多种表现。

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