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质子化有利于溶菌酶与十二烷基硫酸钠的聚集。

Protonation favors aggregation of lysozyme with SDS.

作者信息

Khan Javed M, Chaturvedi Sumit K, Rahman Shah K, Ishtikhar Mohd, Qadeer Atiyatul, Ahmad Ejaz, Khan Rizwan H

机构信息

Interdisciplinary Biotechnology Unit, Aligarh Muslim University, Aligarh 202002, India.

出版信息

Soft Matter. 2014 Apr 21;10(15):2591-9. doi: 10.1039/c3sm52435c.

DOI:10.1039/c3sm52435c
PMID:24647567
Abstract

Different proteins have different amino acid sequences as well as conformations, and therefore different propensities to aggregate. Electrostatic interactions have an important role in the aggregation of proteins as revealed by our previous report (J. M. Khan et al., PLoS One, 2012, 7, e29694). In this study, we designed and executed experiments to gain knowledge of the role of charge variations on proteins during the events of protein aggregation with lysozyme as a model protein. To impart positive and negative charges to proteins, we incubated lysozyme at different pH values of below and above the pI (∼11). Negatively charged SDS was used to 'antagonize' positive charges on lysozyme. We examined the effects of pH variations on SDS-induced amyloid fibril formation by lysozyme using methods such as far-UV circular dichroism, Rayleigh scattering, turbidity measurements, dye binding assays and dynamic light scattering. We found that sub-micellar concentrations of SDS (0.1 to 0.6 mM) induced amyloid fibril formation by lysozyme in the pH range of 10.0-1.0 and maximum aggregation was observed at pH 1.0. The morphology of aggregates was fibrillar in structure, as visualized by transmission electron microscopy. Isothermal titration calorimetry studies demonstrated that fibril formation is exothermic. To the best of our current understanding of the mechanism of aggregation, this study demonstrates the crucial role of electrostatic interactions during amyloid fibril formation. The model proposed here will help in designing molecules that can prevent or reverse the amyloid fibril formation or the aggregation.

摘要

不同的蛋白质具有不同的氨基酸序列和构象,因此具有不同的聚集倾向。正如我们之前的报告(J.M. Khan等人,《公共科学图书馆·综合》,2012年,7卷,e29694)所揭示的,静电相互作用在蛋白质聚集中起着重要作用。在本研究中,我们设计并开展了实验,以了解电荷变化在以溶菌酶为模型蛋白的蛋白质聚集过程中对蛋白质的作用。为了给蛋白质赋予正电荷和负电荷,我们在低于和高于pI(约11)的不同pH值下孵育溶菌酶。带负电荷的十二烷基硫酸钠(SDS)被用来“对抗”溶菌酶上的正电荷。我们使用远紫外圆二色性、瑞利散射、浊度测量、染料结合测定和动态光散射等方法,研究了pH变化对SDS诱导溶菌酶形成淀粉样纤维的影响。我们发现,亚胶束浓度的SDS(0.1至0.6 mM)在pH值为10.0 - 1.0的范围内诱导溶菌酶形成淀粉样纤维,在pH 1.0时观察到最大聚集。通过透射电子显微镜观察,聚集体的形态为纤维状结构。等温滴定量热法研究表明,纤维形成是放热的。就我们目前对聚集机制的理解而言,本研究证明了静电相互作用在淀粉样纤维形成过程中的关键作用。这里提出的模型将有助于设计能够预防或逆转淀粉样纤维形成或聚集的分子。

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