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Positive Cofactor 4 (PC4) is critical for DNA repair pathway re-routing in DT40 cells

机译:辅助因子4(PC4)阳性对于DT40细胞中DNA修复途径的重新路由至关重要

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摘要

PC4 is an abundant single-strand DNA binding protein that has been implicated in transcription and DNA repair. Here, we show that PC4 is involved in the cellular DNA damage response. To elucidate the role, we used the DT40 chicken B cell model, which produces clustered DNA lesions at Ig loci via the action of activation-induced deaminase. Our results help resolve key aspects of immunoglobulin diversification and suggest an essential role of PC4 in repair pathway choice. We show that PC4 ablation in gene conversion (GC)-active cells significantly disrupts GC but has little to no effect on targeted homologous recombination. In agreement, the global double-strand break repair response, as measured by γH2AX foci analysis, is unperturbed 16 hours post irradiation. In cells with the pseudo-genes removed (GC inactive), PC4 ablation reduced the overall mutation rate while simultaneously increasing the transversion mutation ratio. By tagging the N-terminus of PC4, gene conversion and somatic hypermutation are all but abolished even when native non-tagged PC4 is present, indicating a dominant negative effect. Our data point to a very early and deterministic role for PC4 in DNA repair pathway re-routing.
机译:PC4是一种丰富的单链DNA结合蛋白,已参与转录和DNA修复。在这里,我们显示PC4参与细胞DNA损伤反应。为了阐明其作用,我们使用了DT40鸡B细胞模型,该模型通过激活诱导的脱氨酶的作用在Ig位点产生簇状DNA损伤。我们的结果有助于解决免疫球蛋白多样化的关键方面,并提示PC4在修复途径选择中的重要作用。我们显示,在基因转化(GC)-活性细胞中PC4消融可显着破坏GC,但对靶向同源重组几乎没有影响。一致的是,用γH2AX焦点分析法测得的整体双链断裂修复反应在辐照后16小时内不受干扰。在去除了假基因的细胞中(GC未激活),PC4消融降低了总突变率,同时增加了颠换突变率。通过标记PC4的N端,即使存在天然的未标记PC4,基因转换和体细胞超突变几乎都被取消,这表明了显性的负作用。我们的数据表明PC4在DNA修复途径重新路由中起着非常早期的决定性作用。

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