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O6-methylguanine induces altered proteins at the level of transcription in human cells.

机译:O6-甲基鸟嘌呤在人类细胞的转录水平上诱导蛋白质的改变。

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摘要

O(6)-Methylguanine (O(6)-meG), which is produced in DNA following exposure to methylating agents, instructs human RNA polymerase II to mis-insert bases opposite the lesion during transcription. In this study, we examined the effect of O(6)-meG on transcription in human cells and investigated the subsequent effects on protein function following translation of the resulting mRNA. In HEK293 cells, O(6)-meG induced incorporation of uridine or cytidine in nascent RNA opposite the adduct. In cells containing active O(6)-alkylguanine-DNA alkyltransferase (AGT), which repairs O(6)-meG, 3% misincorporation of uridine was observed opposite the lesion. In cells where AGT function was compromised by addition of the AGT inhibitor O(6)-benzylguanine, ~ 58% of the transcripts contained a uridine misincorporation opposite the lesion. Furthermore, the altered mRNA induced changes to protein function as demonstrated through recovery of functional red fluorescent protein (RFP) from DNA coding for a non-fluorescent variant of RFP. These data show that O(6)-meG is highly mutagenic at the level of transcription in human cells, leading to an altered protein load, especially when AGT is inhibited.
机译:暴露于甲基化剂后在DNA中产生的O(6)-甲基鸟嘌呤(O(6)-meG)指示人类RNA聚合酶II在转录过程中错误插入与病灶相对的碱基。在这项研究中,我们检查了O(6)-meG对人类细胞转录的影响,并研究了所得mRNA的翻译对蛋白质功能的后续影响。在HEK293细胞中,O(6)-meG诱导尿苷或胞苷掺入与加合物相反的新生RNA中。在含有活性O(6)-烷基鸟嘌呤-DNA烷基转移酶(AGT),可修复O(6)-meG的细胞中,在病变对面观察到3%的尿苷错误掺入。在其中通过添加AGT抑制剂O(6)-苄基鸟嘌呤损害AGT功能的细胞中,约58%的转录本包含与病灶相对的尿苷错误掺入。此外,改变的mRNA诱导了蛋白质功能的改变,如通过从编码RFP的非荧光变体的DNA中恢复功能性红色荧光蛋白(RFP)所证明的。这些数据表明,O(6)-meG在人类细胞中的转录水平上具有很高的致突变性,从而导致蛋白质负载的改变,尤其是当AGT被抑制时。

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