Structure basis of the caffeic acid O-methyltransferase from Ligusiticum chuanxiong to understand its selective mechanism

咖啡酸 化学 立体化学 氢键 对接(动物) 三元络合物 活动站点 羧酸盐 基质(水族馆) 生物化学 有机化学 分子 抗氧化剂 生物 医学 生态学 护理部
作者
Simin Song,Anqi Chen,Jianquan Zhu,Zicheng Yan,Qiuju An,Jiayu Zhou,Hai Liao,Yamei Yu
出处
期刊:International Journal of Biological Macromolecules [Elsevier BV]
卷期号:194: 317-330 被引量:16
标识
DOI:10.1016/j.ijbiomac.2021.11.135
摘要

Caffeic acid O-methyltransferase from Ligusticum chuanxiong (LcCOMT) showed strict regiospecificity despite a relative degree of preference. Compared with caffeic acid, methyl caffeate was the preferential substrate by its low Km and high Kcat. In this study, we obtained the SAM binary (1.80 Å) and SAH binary (1.95 Å) complex LcCOMT crystal structures, and established the ternary complex structure with methyl caffeate by molecular docking. The active site of LcCOMT included phenolic substrate pocket, SAM/SAH ligand pocket and conserved catalytic residues as well. The regiospecificity of LcCOMT that permitted only 3-hydroxyl group to be methylated arise from the interactions between the active site and the phenyl ring. However, the propanoid tail governed the relative preference of LcCOMT. The ester group in methyl caffeate stabilized the anionic intermediate caused by His268-Asp269 pair, whereas caffeic acid was unable to stabilize the anionic intermediate due to the adjacent carboxylate anion in the propanoid tail. Ser183 residue formed an additional hydrogen bond with SAH and its role was identified by S183A mutation. Ile318 residue might be a potential site for determination of substrate preference, and its mutation led to the change of tertiary conformation. The results supported the selective mechanism of LcCOMT.
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