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Assembly of the Five-Way Junction in the Ribosomal Small Subunit Using Hybrid MD-Go Simulations

机译:使用混合MD-Go模拟在核糖体小亚基中的五向连接

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摘要

Assembly of the bacterial ribosomal small subunit (SSU) begins with the folding of the five-way junction upon interaction with the primary binding protein S4. This complex contains the largest contiguous molecular signature, which is a conserved feature in all bacterial 16S rRNAs. In a previous study, we used all-atom molecular dynamics simulations to demonstrate that the co-evolving signature in the N-terminus of S4 is intrinsically disordered and capable of accelerating the binding process through a fly casting mechanism. In this paper, comparisons between the all-atom MD simulations and FRET experiments identify multiple metastable conformations of the naked five-way junction without the presence of S4. Furthermore, we capture the simultaneous folding and binding of the five-way junction and r-protein S4 by use of a structure-based Gō potential implemented within the framework of the all-atom molecular dynamics CHARMM force field. Different folding pathways are observed for the refolding of the five-way junction upon partial binding of S4. Our simulations illustrate the complex nature of RNA folding in the presence of a protein binding partner and provide insight into the role of population shift and the induced fit mechanisms in the protein:RNA folding and binding process.
机译:细菌核糖体小亚基(SSU)的组装始于与主要结合蛋白S4相互作用时五向接头的折叠。该复合物包含最大的连续分子标记,这是所有细菌16S rRNA的保守特征。在先前的研究中,我们使用了全原子分子动力学模拟来证明S4的N末端的共同进化特征本质上是无序的,并且能够通过飞铸机制加速结合过程。在本文中,全原子MD模拟和FRET实验之间的比较确定了在不存在S4的情况下,裸五通结的多个亚稳构象。此外,我们通过使用在所有原子分子动力学CHARMM力场框架内实现的基于结构的Gō势,捕获了五向联结和r蛋白S4的同时折叠和结合。观察到S4部分结合后五向连接的重折叠的不同折叠途径。我们的模拟说明了存在蛋白质结合伴侣的情况下RNA折叠的复杂性质,并提供了对种群迁移的作用以及蛋白质:RNA折叠和结合过程中诱导的适应机制的了解。

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