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Single-molecule spectroscopy of the unexpected collapse of an unfolded protein at low pH

机译:单分子光谱法在低pH下未折叠蛋白质的意外崩溃

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The dimensions of intrinsically disordered and unfolded proteins critically depend on the solution conditions, such as temperature, pH, ionic strength, and osmolyte or denarurant concentration. However, a quantitative understanding of how the complex combination of chain-chain and chain-solvent interactions is affected by the solvent is still missing. Here, we take a step towards this goal by investigating the combined effect of pH and denaturants on the dimensions of an unfolded protein. We use single-molecule fluorescence spectroscopy to extract the dimensions of unfolded cold shock protein (CspTm) in mixtures of the denaturants urea and guanidinium chloride (GdmCl) at neutral and acidic pH. Surprisingly, even though a change in pH from 7 to 2.9 increases the net charge of CspTm from -3.8 to +10.2, the radius of gyration of the chain is very similar under both conditions, indicating that protonation of acidic side chains at low pH results in additional hydrophobic interactions. We use a simple shared binding site model that describes the joint effect of urea and GdmCl, together with polyampholyte theory and an ion cloud model that includes the chemical free energy of counterion interactions and side chain protonation, to quantify this effect.
机译:本质上无序和未折叠的蛋白质的尺寸主要取决于溶液的条件,例如温度,pH,离子强度,渗透压或纳莫尔浓度。然而,仍然缺少对链-链和链-溶剂相互作用的复杂组合如何受溶剂影响的定量理解。在这里,我们通过研究pH和变性剂对未折叠蛋白质尺寸的综合影响,朝着这一目标迈出了一步。我们使用单分子荧光光谱法提取变性尿素和氯化胍(GdmCl)在中性和酸性pH值下的混合物中未折叠的冷激蛋​​白(CspTm)的尺寸。出人意料的是,即使pH值从7变为2.9,CspTm的净电荷也将从-3.8增至+10.2,但是在两种条件下,链的回转半径都非常相似,这表明在低pH值下酸性侧链的质子化在其他疏水相互作用中。我们使用一个简单的共享结合位点模型(该模型描述了尿素和GdmCl的联合作用),聚两性电解质理论和一个包含反离子相互作用和侧链质子化的化学自由能的离子云模型来量化这种作用。

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