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L1 retrotransposition requires rapid ORF1p oligomerization a novel coiled coil-dependent property conserved despite extensive remodeling

机译:L1逆转座需要快速的ORF1p寡聚尽管进行了广泛的改建但仍保留了一种新型的卷曲螺旋依赖性结构

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摘要

Detailed mechanistic understanding of L1 retrotransposition is sparse, particularly with respect to ORF1p, a coiled coil-mediated homotrimeric nucleic acid chaperone that can form tightly packed oligomers on nucleic acids. Although the coiled coil motif is highly conserved, it is uniquely susceptible to evolutionary change. Here we studied three ORF1 proteins: a modern human one (111p), its resuscitated primate ancestor (555p) and a mosaic modern protein (151p) wherein 9 of the 30 coiled coil substitutions retain their ancestral state. While 111p and 555p equally supported retrotransposition, 151p was inactive. Nonetheless, they were fully active in bulk assays of nucleic acid interactions including chaperone activity. However, single molecule assays showed that 151p trimers form stably bound oligomers on ssDNA at <1/10th the rate of the active proteins, revealing that oligomerization rate is a novel critical parameter of ORF1p activity in retrotransposition conserved for at least the last 25 Myr of primate evolution.
机译:对L1逆转座的详细机械理解稀疏,特别是对于ORF1p而言,ORF1p是卷曲的螺旋介导的同源三聚体核酸伴侣,可以在核酸上形成紧密堆积的寡聚物。尽管盘绕的线圈图案高度保守,但它极易受到进化变化的影响。在这里,我们研究了三种ORF1蛋白:一种现代人类蛋白(111p),其复苏的灵长类动物祖先(555p)和一种镶嵌现代蛋白(151p),其中30个卷曲螺旋取代物中的9个保持其祖先状态。虽然111p和555p同样支持逆转座,但151p无效。但是,它们在核酸相互作用(包括伴侣活性)的大量测定中具有完全的活性。然而,单分子分析表明,151p三聚体在ssDNA上形成稳定结合的寡聚体,其活性蛋白的比率小于活性蛋白质的1/10,表明寡聚化率是ORF1p活性的一个新的关键参数,在逆转录中至少保留了25 Myr。灵长类动物进化。

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