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Lattice simulations of cotranslational folding of single domain proteins.

机译:单域蛋白共翻译折叠的晶格模拟。

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摘要

We use lattice protein models and Monte Carlo simulations to study cotranslational folding of small single domain proteins. We show that the assembly of native structure begins during late extrusion stages, but final formation of native state occurs during de novo folding, when all residues are extruded. There are three main results in our study. First, for the sequences displaying two-state refolding mechanism de novo cotranslational folding pathway differs from that sampled in in vitro refolding. The change in folding pathways is due to partial assembly of native interactions during extrusion that results in different starting conditions for in vitro refolding and for de novo cotranslational folding. For small single domain proteins cotranslational folding is slower than in vitro refolding, but is generally fast enough to be completed before the release from a ribosome. Second, we found that until final stages of biosynthesis cotranslational folding is essentially equilibrium. This observation is explained by low stability of structured states for partially extruded chains. Finally, our data suggest that the proteins, which refold in vitro slowly via intermediates, complete their de novo folding after the release from a ribosome. Comparison of our lattice cotranslational simulations with recent experimental and computational studies is discussed.
机译:我们使用晶格蛋白模型和蒙特卡洛模拟研究小单域蛋白的共翻译折叠。我们表明天然结构的组装开始于后期挤出阶段,但当所有残基均被挤出时,原始状态的最终形成发生在从头折叠期间。我们的研究有三个主要结果。首先,对于显示两种状态重折叠机制的序列,从头共翻译折叠路径与体外重折叠中所采样的不同。折叠途径的变化归因于挤出过程中天然相互作用的部分组装,这导致体外重折叠和从头共翻译折叠的起始条件不同。对于小的单结构域蛋白,共翻译折叠比体外重折叠慢,但通常足够快,可以在从核糖体释放之前完成。其次,我们发现直到生物合成的最后阶段,共翻译折叠基本上是平衡的。对于部分挤出的链,结构态的稳定性较低,可以解释此现象。最后,我们的数据表明,通过中间体在体外缓慢重折叠的蛋白质在从核糖体释放后完成了从头折叠。讨论了我们的晶格共翻译模拟与最近的实验和计算研究的比较。

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