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阻抗谱揭示了表面活性剂诱导的人血清白蛋白展开和随后的折叠。

Impedance Spectroscopy Unveiled the Surfactant-Induced Unfolding and Subsequent Refolding of Human Serum Albumin.

机构信息

Biophysics and Soft Matter Laboratory, Department of Physics, IIT Kharagpur, Kharagpur 721302, India.

出版信息

Langmuir. 2024 Sep 10;40(36):19022-19031. doi: 10.1021/acs.langmuir.4c01886. Epub 2024 Aug 27.

DOI:10.1021/acs.langmuir.4c01886
PMID:39189867
Abstract

Protein-surfactant interaction is a dynamic interplay of electrostatic and hydrophobic forces that ensues from the folding of a protein. We employ impedance spectroscopy (IS), a label-free method, to investigate the unfolding and refolding of human serum albumin (HSA), a globular plasma protein, in the presence of two surfactants: polysorbate-20 (Tween-20), a nonionic surfactant, and sodium dodecyl sulfate (SDS), an anionic surfactant. The equivalent electrical analog circuit was predicted from impedance spectra of HSA in an aqueous solution at physiological pH and room temperature, focusing on varying the concentration of codissolved surfactants. A change in the dielectric constant (ε) and ionic conductivity (κ) is observed by comparing the surfactant-treated protein samples to the bare surfactant solutions to assess the conformational changes induced by surfactants in HSA. Far-UV circular dichroism analysis revealed a decrease in α-helices and an increase in β-sheets and random coils upon SDS addition, which were reversed by Tween-20. Dynamic light scattering supported the findings by measuring changes in the hydrodynamic diameter () of HSA. Unfolding and refolding of HSA with surfactants were also observed through photoluminescence spectroscopy by examining the microenvironment surrounding the single tryptophan () within the protein, and the thermodynamic parameters were obtained using the modified Stern-Volmer equation. Our research explores the intriguing domain of protein-surfactant interactions, offering insights with promising applications across diverse biological processes and IS as a suitable alternative technique for investigating protein conformational changes by studying the electrical response of the samples.

摘要

蛋白质-表面活性剂相互作用是一种静电和疏水相互作用的动态相互作用,源自蛋白质的折叠。我们采用阻抗谱(IS),一种无标记的方法,研究了人血清白蛋白(HSA)在两种表面活性剂存在下的展开和折叠:聚山梨酯 20(吐温 20),一种非离子表面活性剂,和十二烷基硫酸钠(SDS),一种阴离子表面活性剂。在生理 pH 值和室温下,在水溶液中预测了 HSA 的等效电模拟电路,重点是改变共溶解表面活性剂的浓度。通过将处理过的蛋白质样品与裸表面活性剂溶液进行比较,观察到介电常数(ε)和离子电导率(κ)的变化,以评估表面活性剂在 HSA 中引起的构象变化。远紫外圆二色性分析表明,SDS 加入后α-螺旋减少,β-折叠和无规卷曲增加,而 Tween-20 则使其逆转。动态光散射通过测量 HSA 水动力直径()的变化支持了这些发现。通过检查蛋白质中单个色氨酸()周围的微环境,还通过荧光光谱研究了 HSA 与表面活性剂的展开和折叠,使用改进的 Stern-Volmer 方程获得了热力学参数。我们的研究探索了蛋白质-表面活性剂相互作用的有趣领域,提供了有前途的应用,涉及到各种生物过程和 IS,作为研究蛋白质构象变化的合适替代技术,通过研究样品的电响应来研究。

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