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SDS 诱导的蛋白质变性:SDS 与蛋白质组装体的微观机制和性质。

Protein unfolding by SDS: the microscopic mechanisms and the properties of the SDS-protein assembly.

机构信息

Center for the Physics of Living Cells, University of Illinois at Urbana-Champaign, Urbana, IL, USA.

出版信息

Nanoscale. 2020 Mar 7;12(9):5422-5434. doi: 10.1039/c9nr09135a. Epub 2020 Feb 21.

DOI:10.1039/c9nr09135a
PMID:32080694
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7291819/
Abstract

The effects of detergent sodium dodecyl sulfate (SDS) on protein structure and dynamics are fundamental to the most common laboratory technique used to separate proteins and determine their molecular weights: polyacrylamide gel electrophoresis. However, the mechanism by which SDS induces protein unfolding and the microstructure of protein-SDS complexes remain largely unknown. Here, we report a detailed account of SDS-induced unfolding of two proteins-I27 domain of titin and β-amylase-obtained through all-atom molecular dynamics simulations. Both proteins were found to spontaneously unfold in the presence of SDS at boiling water temperature on the time scale of several microseconds. The protein unfolding was found to occur via two distinct mechanisms in which specific interactions of individual SDS molecules disrupt the protein's secondary structure. In the final state of the unfolding process, the proteins are found to wrap around SDS micelles in a fluid necklace-and-beads configuration, where the number and location of bound micelles changes dynamically. The global conformation of the protein was found to correlate with the number of SDS micelles bound to it, whereas the number of SDS molecules directly bound to the protein was found to define the relaxation time scale of the unfolded protein. Our microscopic characterization of SDS-protein interactions sets the stage for future refinement of SDS-enabled protein characterization methods, including protein fingerprinting and sequencing using a solid-state nanopore.

摘要

十二烷基硫酸钠(SDS)对蛋白质结构和动力学的影响是最常用的实验室技术,用于分离蛋白质并确定其分子量:聚丙烯酰胺凝胶电泳的基础。然而,SDS 诱导蛋白质展开的机制以及蛋白质-SDS 复合物的微观结构在很大程度上仍然未知。在这里,我们通过全原子分子动力学模拟,详细描述了 SDS 诱导的两种蛋白质——肌联蛋白 I27 结构域和β-淀粉酶的展开。发现在 SDS 存在下,这两种蛋白质在沸水温度下都会自发展开,在几微秒的时间尺度上。发现蛋白质的展开是通过两种不同的机制发生的,其中 SDS 分子的特定相互作用破坏了蛋白质的二级结构。在展开过程的最终状态下,发现蛋白质在 SDS 胶束周围形成流体项链和珠子的配置,其中结合胶束的数量和位置动态变化。发现蛋白质的整体构象与其结合的 SDS 胶束数量相关,而直接结合到蛋白质上的 SDS 分子数量则定义了展开蛋白质的弛豫时间尺度。我们对 SDS-蛋白质相互作用的微观描述为未来改进 SDS 增强的蛋白质特性分析方法奠定了基础,包括使用固态纳米孔进行蛋白质指纹图谱和测序。

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Unfolding and partial refolding of a cellulase from the SDS-denatured state: From β-sheet to α-helix and back.从 SDS 变性状态下展开和部分重折叠纤维素酶:从β-折叠到α-螺旋再到β-折叠。
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Simulation of single-protein nanopore sensing shows feasibility for whole-proteome identification.模拟单蛋白纳米孔传感显示了用于全蛋白质组鉴定的可行性。
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