Improving the catalytic performance of carbonyl reductase based on the functional loops engineering

化学 基质(水族馆) 立体化学 催化作用 非对映体 立体选择性 还原酶 催化循环 生物催化 亲核细胞 酶催化 反应机理 有机化学 海洋学 地质学
作者
Tao‐Shun Zhou,Xiangyang Li,Xiao‐Jian Zhang,Xue Cai,Zhi‐Qiang Liu,Yu‐Guo Zheng
出处
期刊:Biotechnology and Bioengineering [Wiley]
标识
DOI:10.1002/bit.28864
摘要

Abstract Vibegron functions as a potent and selective β 3 ‐adrenergic receptor agonist, with its chiral precursor ( 2S , 3R )‐aminohydroxy ester ( 1b) being crucial to its synthesis. In this study, loop engineering was applied to the carbonyl reductase ( Ea SDR6) from Exiguobacterium algae to achieve an asymmetric reduction of the ( rac )‐aminoketone ester 1a . The variant M5 (A138L/A190V/S193A/Y201F/N204A) was obtained and demonstrated an 868‐fold increase in catalytic efficiency ( k cat / K m = 260.3 s −1 mM −1 ) and a desirable stereoselectivity (>99% enantiomeric excess, e.e. ; >99% diastereomeric excess, d.e. ) for the target product 1b in contrast to the wild‐type Ea SDR6 (WT). Structural alignment with WT indicated that loops 137–154 and 182–210 potentially play vital roles in facilitating catalysis and substrate binding. Moreover, molecular dynamics (MD) simulations of WT‐ 1a and M5‐ 1a complex illustrated that M5‐ 1a exhibits a more effective nucleophilic attack distance and more readily adopts a pre‐reaction state. The interaction analysis unveiled that M5 enhanced hydrophobic interactions with substrate 1a on cavities A and B while diminishing unfavorable hydrophilic interactions on cavity C. Computational analysis of binding free energies indicated that M5 displayed heightened affinity towards substrate 1a compared to the WT, aligning with its decreased K m value. Under organic‐aqueous biphasic conditions, the M5 mutant showed >99% conversion within 12 h with 300 g/L substrate 1a (highest substrate loading as reported). This study enhanced the catalytic performance of carbonyl reductase through functional loops engineering and established a robust framework for the large‐scale biosynthesis of the vibegron intermediate.
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