Jaramillo-Martinez Valeria, Dominguez Matthew J, Bell Gemma M, Souness Megan E, Carhart Anna H, Cuibus M Adriana, Masoumzadeh Elahe, Lantz Benjamin J, Adkins Aaron J, Latham Michael P, Ball K Aurelia, Stollar Elliott J
bioRxiv. 2023 Mar 22:2023.03.21.532811. doi: 10.1101/2023.03.21.532811.
Charged residues on the surface of proteins are critical for both protein stability and interactions. However, many proteins contain binding regions with a high net-charge that may destabilize the protein but are useful for binding to oppositely charged targets. We hypothesized that these domains would be marginally stable, as electrostatic repulsion would compete with favorable hydrophobic collapse during folding. Furthermore, by increasing the salt concentration we predict that these protein folds would be stabilized by mimicking some of the favorable electrostatic interactions that take place during target binding. We varied the salt and urea concentrations to probe the contributions of electrostatic and hydrophobic interactions for the folding of the 60-residue yeast SH3 domain found in Abp1p. The SH3 domain was significantly stabilized with increased salt concentrations according to the Debye-Huckel limiting law. Molecular dynamics and NMR show that sodium ions interact with all 15 acidic residues but do little to change backbone dynamics or overall structure. Folding kinetics experiments show that the addition of urea or salt primarily affects the folding rate, indicating that almost all the hydrophobic collapse and electrostatic repulsion occurs in the transition state. After the transition state formation, modest yet favorable short-range salt-bridges are formed along with hydrogen bonds, as the native state fully folds. Thus, hydrophobic collapse offsets electrostatic repulsion to ensure this highly charged binding domain can still fold and be ready to bind to its charged peptide targets, a property that is likely evolutionarily conserved over one billion years.
Some protein domains are highly charged because they are adapted to bind oppositely charged proteins and nucleic acids. However, it is unknown how these highly charged domains fold as during folding there will be significant repulsion between like-charges. We investigate how one of these highly charged domains folds in the presence of salt, which can screen the charge repulsion and make folding easier, allowing us to understand how folding occurs despite the protein’s high charge.
Supplementary material document containing additional details on protein expression methods, thermodynamics and kinetics equations, and the effect of urea on electrostatic interactions, as well as 4 supplemental figures and 4 supplemental data tables. ( ), 15 pages Supplemental excel file containing covariation data across AbpSH3 orthologs ( ).
蛋白质表面的带电残基对于蛋白质稳定性和相互作用都至关重要。然而,许多蛋白质含有净电荷较高的结合区域,这可能会使蛋白质不稳定,但对与带相反电荷的靶标结合很有用。我们推测这些结构域稳定性较低,因为在折叠过程中静电排斥会与有利的疏水塌缩相互竞争。此外,我们预测通过增加盐浓度,这些蛋白质折叠会因模拟靶标结合过程中发生的一些有利静电相互作用而得到稳定。我们改变盐和尿素浓度,以探究静电和疏水相互作用对在Abp1p中发现的60个残基的酵母SH3结构域折叠的贡献。根据德拜-休克尔极限定律,随着盐浓度增加,SH3结构域显著稳定。分子动力学和核磁共振表明,钠离子与所有15个酸性残基相互作用,但对主链动力学或整体结构影响很小。折叠动力学实验表明,添加尿素或盐主要影响折叠速率,这表明几乎所有的疏水塌缩和静电排斥都发生在过渡态。在过渡态形成后,随着天然态完全折叠,会形成适度但有利的短程盐桥以及氢键。因此,疏水塌缩抵消了静电排斥,以确保这个高电荷结合结构域仍能折叠并准备好与带电荷的肽靶标结合,这一特性在超过十亿年的时间里可能在进化上得以保留。
一些蛋白质结构域带高电荷是因为它们适于与带相反电荷的蛋白质和核酸结合。然而,尚不清楚这些高电荷结构域如何折叠,因为在折叠过程中相同电荷之间会有显著排斥。我们研究其中一个高电荷结构域在盐存在下如何折叠,盐可以屏蔽电荷排斥并使折叠更容易,从而让我们了解尽管蛋白质带高电荷折叠是如何发生的。
补充材料文档包含有关蛋白质表达方法、热力学和动力学方程以及尿素对静电相互作用影响的更多详细信息,以及4个补充图和4个补充数据表。( ),15页包含AbpSH3直系同源物协变数据的补充Excel文件( )。
