Murata Takeshi, Yasuda Satoshi, Hayashi Tomohiko, Kinoshita Masahiro
Graduate School of Science, Chiba University, 1-33 Yayoi-cho, Inage, Chiba, 263-8522, Japan.
Molecular Chirality Research Center, Chiba University, 1-33 Yayoi-cho, Inage, Chiba, 263-8522, Japan.
Biophys Rev. 2020 Apr;12(2):323-332. doi: 10.1007/s12551-020-00678-5. Epub 2020 Apr 8.
Thermostabilization of a membrane proteins, especially G-protein-coupled receptors (GPCRs), is often necessary for biochemical applications and pharmaceutical studies involving structure-based drug design. Here we review our theoretical, physics-based method for identifying thermostabilizing amino acid mutations. Its novel aspects are the following: The entropic effect originating from the translational displacement of hydrocarbon groups within the lipid bilayer is treated as a pivotal factor; a reliable measure of thermostability is introduced and a mutation which enlarges the measure to a significant extent is chosen; and all the possible mutations can be examined with moderate computational effort. It was shown that mutating the residue at a position of N = 3.39 (N is the Ballesteros-Weinstein number) to Arg or Lys leads to the stabilization of significantly many different GPCRs of class A in the inactive state. Up to now, we have been successful in stabilizing several GPCRs and newly solving three-dimensional structures for the muscarinic acetylcholine receptor 2 (M2R), prostaglandin E receptor 4 (EP4), and serotonin 2A receptor (5-HTR) using X-ray crystallography. The subjects to be pursued in future studies are also discussed.
对于涉及基于结构的药物设计的生化应用和药物研究而言,膜蛋白尤其是G蛋白偶联受体(GPCR)的热稳定性化通常是必要的。在此,我们综述了我们基于物理学的理论方法,用于识别热稳定性化氨基酸突变。其新颖之处如下:源自脂质双层内烃基平移位移的熵效应被视为关键因素;引入了热稳定性的可靠度量,并选择能将该度量显著增大的突变;并且可以通过适度的计算量来检查所有可能的突变。结果表明,将N = 3.39位置(N为巴列斯特罗斯 - 温斯坦编号)的残基突变为精氨酸或赖氨酸会导致许多不同的A类GPCR在非活性状态下显著稳定。到目前为止,我们已成功地稳定了几种GPCR,并利用X射线晶体学新解析了毒蕈碱型乙酰胆碱受体2(M2R)、前列腺素E受体4(EP4)和5-羟色胺2A受体(5-HTR)的三维结构。还讨论了未来研究中有待探讨的主题。
