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Itinerary profiling to analyze a large number of protein-folding trajectories

机译:行程分析可分析大量蛋白质折叠轨迹

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摘要

Understanding how proteins fold through a vast number of unfolded states is a major subject in the study of protein folding. Herein, we present itinerary profiling as a simple method to analyze molecular dynamics trajectories, and apply this method to Trp-cage. In itinerary profiling, structural clusters included in a trajectory are represented by a bit sequence, and a number of trajectories, as well as the structural clusters, can be compared and classified. As a consequence, the structural clusters that characterize the foldability of trajectories were able to be identified. The connections between the clusters were then illustrated as a network and the structural features of the clusters were examined. We found that in the true folding funnel, Trp-cage formed a left-handed main-chain topology and the Trp6 side-chain was located at the front of the main-chain ring, even in the initial unfolded states. In contrast, in the false folding funnel of the pseudo-native states, in which the Trp6 side-chain is upside down in the protein core, Trp-cage had a right-handed main-chain topology and the Trp side-chain was at the back. The initial topological partition, as determined by the main-chain handedness and the location of the Trp residue, predetermines Trp-cage foldability and the destination of the trajectory to the native state or the pseudo-native states.
机译:了解蛋白质如何通过大量未折叠状态折叠是蛋白质折叠研究的主要课题。在本文中,我们提出了路线分析作为一种简单的方法来分析分子动力学轨迹,并将此方法应用于Trp笼。在行程分析中,轨迹中包含的结构簇由位序列表示,并且可以比较和分类许多轨迹以及结构簇。结果,能够确定表征轨迹可折叠性的结构簇。然后,将群集之间的连接图示为网络,并检查了群集的结构特征。我们发现,在真正的折叠漏斗中,Trp笼形成了左手主链拓扑结构,而Trp6侧链甚至在初始展开状态下也位于主链环的前端。相反,在假天然状态的假折叠漏斗中,Trp6侧链在蛋白质核心中上下颠倒,Trp笼具有右手主链拓扑,而Trp侧链位于背部。初始拓扑划分(由主链惯用性和Trp残基的位置确定)预先确定Trp笼的可折叠性以及轨迹到原始状态或伪原始状态的目的地。

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