Kaur Anupamjeet, Goyal Deepti, Goyal Bhupesh
Department of Chemistry, Faculty of Basic and Applied Sciences, Sri Guru Granth Sahib World University, Fatehgarh Sahib-140406, Punjab, India.
Phys Chem Chem Phys. 2020 Dec 23;22(48):28055-28073. doi: 10.1039/d0cp04672h.
Alzheimer's disease (AD), an epidemic growing worldwide due to no effective medical aid available in the market, is a neurological disorder. AD is known to be directly associated with the toxicity of amyloid-β (Aβ) aggregates. In search of potent inhibitors of Aβ aggregation, Hamilton and co-workers reported an α-helix mimetic, ADH-31, which acts as a powerful antagonist of Aβ42 aggregation. To identify the key interactions between protein-ligand complexes and to gain insights into the inhibitory mechanism of ADH-31 against Aβ42 aggregation, molecular dynamics (MD) simulations were performed in the present study. The MD simulations highlighted that ADH-31 showed distinct binding capabilities with residues spanning from the N-terminal to the central hydrophobic core (CHC) region of Aβ42 and restricted the conformational transition of the helix-rich structure of Aβ42 into another form of secondary structures (coil/turn/β-sheet). Hydrophobic contacts, hydrogen bonding and π-π interaction contribute to the strong binding between ADH-31 and Aβ42 monomer. The Dictionary of Secondary Structure of Proteins (DSSP) analysis highlighted that the probability of helical content increases from 38.5% to 50.2% and the turn content reduces from 14.7% to 6.2% with almost complete loss of the β-sheet structure (4.5% to 0%) in the Aβ42 monomer + ADH-31 complex. The per-residue binding free energy analysis demonstrated that Arg5, Tyr10, His14, Gln15, Lys16, Val18, Phe19 and Lys28 residues of Aβ42 are responsible for the favourable binding free energy in Aβ42 monomer + ADH-31 complex, which is consistent with the 2D HSQC NMR of the Aβ42 monomer that depicted a change in the chemical shift of residues spanning from Glu11 to Phe20 in the presence of ADH-31. The MD simulations highlighted the prevention of sampling of amyloidogenic β-strand conformations in Aβ42 trimer in the presence of ADH-31 as well as the ability of ADH-31 to destabilize Aβ42 trimer and protofibril structures. The lower binding affinity between Aβ42 trimer chains in the presence of ADH-31 highlights the destabilization of the Aβ42 trimer structure. Overall, MD results highlighted that ADH-31 inhibited Aβ42 aggregation by constraining Aβ peptides into helical conformation and destabilized Aβ42 trimer as well as protofibril structures. The present study provides a theoretical insight into the atomic level details of the inhibitory mechanism of ADH-31 against Aβ42 aggregation as well as protofibril destabilization and could be implemented in the structure-based drug design of potent therapeutic agents for AD.
阿尔茨海默病(AD)是一种神经系统疾病,由于市场上没有有效的医疗救助手段,其在全球范围内呈流行趋势。已知AD与淀粉样β蛋白(Aβ)聚集体的毒性直接相关。为了寻找Aβ聚集的有效抑制剂,汉密尔顿及其同事报道了一种α-螺旋模拟物ADH-31,它是Aβ42聚集的强大拮抗剂。为了确定蛋白质-配体复合物之间的关键相互作用,并深入了解ADH-31对Aβ42聚集的抑制机制,本研究进行了分子动力学(MD)模拟。MD模拟突出显示,ADH-31与Aβ42从N端到中央疏水核心(CHC)区域的残基具有明显的结合能力,并限制了Aβ42富含螺旋结构向另一种二级结构形式(卷曲/转角/β-折叠)的构象转变。疏水接触、氢键和π-π相互作用有助于ADH-31与Aβ42单体之间的强结合。蛋白质二级结构词典(DSSP)分析突出显示,在Aβ42单体+ADH-31复合物中,螺旋含量的概率从38.5%增加到50.2%,转角含量从14.7%降低到6.2%,β-折叠结构几乎完全丧失(从4.5%降至0%)。每个残基的结合自由能分析表明,Aβ42的Arg5、Tyr10、His14、Gln15、Lys16、Val18、Phe19和Lys28残基负责Aβ42单体+ADH-31复合物中有利的结合自由能,这与Aβ42单体的二维异核单量子相干核磁共振(2D HSQC NMR)结果一致,该结果表明在存在ADH-31的情况下,从Glu11到Phe20的残基化学位移发生了变化。MD模拟突出显示,在存在ADH-31的情况下,可防止Aβ42三聚体中淀粉样β链构象的采样,以及ADH-31破坏Aβ42三聚体和原纤维结构的能力。在存在ADH-31的情况下,Aβ42三聚体链之间较低的结合亲和力突出显示了Aβ42三聚体结构的不稳定。总体而言,MD结果突出显示,ADH-31通过将Aβ肽限制为螺旋构象来抑制Aβ42聚集,并破坏Aβ42三聚体以及原纤维结构。本研究为ADH-31对Aβ42聚集以及原纤维不稳定的抑制机制的原子水平细节提供了理论见解,并可应用于AD有效治疗剂的基于结构的药物设计。
