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Common determinants in DNA melting and helicase-catalysed DNA unwinding by papillomavirus replication protein E1

机译:乳头瘤病毒复制蛋白E1在DNA熔解和解旋酶催化的DNA解链中的常见决定因素

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摘要

E1 and T-antigen of the tumour viruses bovine papillomavirus (BPV-1) and Simian virus 40 (SV40) are the initiator proteins that recognize and melt their respective origins of replication in the initial phase of DNA replication. These proteins then assemble into processive hexameric helicases upon the single-stranded DNA that they create. In T-antigen, a characteristic loop and hairpin structure (the pre-sensor 1β hairpin, PS1βH) project into a central cavity generated by protein hexamerization. This channel undergoes large ATP-dependent conformational changes, and the loop/PS1βH is proposed to form a DNA binding site critical for helicase activity. Here, we show that conserved residues in BPV E1 that probably form a similar loop/hairpin structure are required for helicase activity and also origin (ori) DNA melting. We propose that DNA melting requires the cooperation of the E1 helicase domain (E1HD) and the origin binding domain (OBD) tethered to DNA. One possible mechanism is that with the DNA locked in the loop/PS1βH DNA binding site, ATP-dependent conformational changes draw the DNA inwards in a twisting motion to promote unwinding.
机译:肿瘤病毒牛乳头瘤病毒(BPV-1)和猿猴病毒40(SV40)的E1和T抗原是在DNA复制初期识别并融化其各自复制起点的起始蛋白。这些蛋白质然后在它们产生的单链DNA上组装成进行性六聚体解旋酶。在T抗原中,特征性的环和发夹结构(传感器前1β的发夹,PS1βH)突出到蛋白质六聚化产生的中央腔中。该通道经历了较大的ATP依赖性构象变化,并提出loop /PS1βH形成对解旋酶活性至关重要的DNA结合位点。在这里,我们显示了BPV E1中可能形成相似环/发夹结构的保守残基对于解旋酶活性以及起源(ori)DNA融解是必需的。我们建议DNA融化需要E1解旋酶域(E1HD)和拴在DNA上的起源结合域(OBD)的合作。一种可能的机制是,将DNA锁定在loop /PS1βHDNA结合位点中,ATP依赖的构象变化以扭转运动向内吸引DNA,以促进解开。

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