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小分子蛋白折叠过程中连续收缩和亚稳定错误折叠状态的观察

Observation of Continuous Contraction and a Metastable Misfolded State during the Collapse and Folding of a Small Protein.

机构信息

National Centre for Biological Sciences, Tata Institute of Fundamental Research, Bengaluru 560 065, India.

Department of Biotechnology, Anna University, Chennai 600 025, India.

出版信息

J Mol Biol. 2019 Sep 6;431(19):3814-3826. doi: 10.1016/j.jmb.2019.07.024. Epub 2019 Jul 19.

DOI:10.1016/j.jmb.2019.07.024
PMID:31330152
Abstract

To obtain proper insight into how structure develops during a protein folding reaction, it is necessary to understand the nature and mechanism of the polypeptide chain collapse reaction, which marks the initiation of folding. Here, the time-resolved fluorescence resonance energy transfer technique, in which the decay of the fluorescence light intensity with time is used to determine the time evolution of the distribution of intra-molecular distances, has been utilized to study the folding of the small protein, monellin. It is seen that when folding begins, about one-third of the protein molecules collapse into a molten globule state (I), from which they relax by continuous further contraction to transit to the native state. The larger fraction gets trapped into a metastable misfolded state. Exit from this metastable state occurs via collapse to the lower free energy I state. This exit is slow, on a time scale of seconds, because of activation energy barriers. The trapped misfolded molecules as well as the I molecules contract continuously and slowly as structure develops. A phenomenological model of Markovian evolution of the polymer chain undergoing folding, incorporating these features, has been developed, which fits well the experimentally observed time evolution of distance distributions. The observation that the "wrong turn" to the misfolded state has not been eliminated by evolution belies the common belief that the folding of functional protein sequences is very different from that of a random heteropolymer, and the former have been selected by evolution to fold quickly.

摘要

为了深入了解蛋白质折叠反应过程中结构的发展,有必要理解多肽链折叠反应的本质和机制,这标志着折叠的开始。在这里,利用时间分辨荧光共振能量转移技术,其中荧光强度随时间的衰减用于确定分子内距离分布的时间演化,研究了小蛋白莫内林的折叠。可以看出,当折叠开始时,大约三分之一的蛋白质分子折叠成无规卷曲状态(I),它们从无规卷曲状态通过连续进一步收缩松弛过渡到天然状态。更大的部分陷入亚稳态错误折叠状态。从这个亚稳态中逸出是通过折叠到较低自由能的 I 态来实现的。由于活化能垒的存在,这种逸出过程非常缓慢,需要几秒钟的时间。由于折叠,被困的错误折叠分子以及 I 分子会连续且缓慢地收缩,从而形成结构。已经开发了一种聚合物链折叠的马尔可夫演化的唯象模型,其中包含了这些特征,该模型与实验观察到的距离分布的时间演化非常吻合。观察到错误折叠状态的“错误转弯”并没有被进化消除,这与普遍认为的功能蛋白序列的折叠与随机杂聚物的折叠非常不同的观点相矛盾,前者是通过进化选择快速折叠的。

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