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Breaking the speed limit with multimode fast scanning of DNA by Endonuclease V

机译:通过核酸内切酶V对DNA进行多模式快速扫描打破了速度限制

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摘要

In order to preserve genomic stability, cells rely on various repair pathways for removing DNA damage. The mechanisms how enzymes scan DNA and recognize their target sites are incompletely understood. Here, by using high-localization precision microscopy along with 133 Hz high sampling rate, we have recorded EndoV and OGG1 interacting with 12-kbp elongated λ-DNA in an optical trap. EndoV switches between three distinct scanning modes, each with a clear range of activation energy barriers. These results concur with average diffusion rate and occupancy of states determined by a hidden Markov model, allowing us to infer that EndoV confinement occurs when the intercalating wedge motif is involved in rigorous probing of the DNA, while highly mobile EndoV may disengage from a strictly 1D helical diffusion mode and hop along the DNA. This makes EndoV the first example of a monomeric, single-conformation and single-binding-site protein demonstrating the ability to switch between three scanning modes.
机译:为了保持基因组稳定性,细胞依靠各种修复途径消除DNA损伤。酶如何扫描DNA并识别其靶位的机制尚不完全清楚。在这里,通过使用高定位精度显微镜和133 Hz的高采样率,我们已经在一个光阱中记录了EndoV和OGG1与12-kbp细长λ-DNA相互作用。 EndoV在三种不同的扫描模式之间切换,每种扫描模式都有清晰的激活能垒范围。这些结果与隐马尔可夫模型确定的平均扩散速率和状态占有率一致,从而使我们可以推断,当嵌入楔形基序参与DNA的严格探测时,会发生EndoV限制,而高度活动的EndoV可能会脱离严格的1D螺旋扩散模式并沿着DNA跳跃。这使EndoV成为单体,单一构型和单一结合位点蛋白的第一个实例,证明了在三种扫描模式之间切换的能力。

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