Department of Biochemistry and Molecular Biology, School of Basic Medical Sciences and the Affiliated Hospital, Key Laboratory of Aging and Cancer Biology of Zhejiang Province, Hangzhou Normal University , Hangzhou, China.
Photosynthesis Research Center, College of Life and Environmental Sciences, Hangzhou Normal University , Hangzhou, China.
mBio. 2023 Aug 31;14(4):e0323322. doi: 10.1128/mbio.03233-22. Epub 2023 Jun 6.
Malonyl-CoA reductase (MCR) is a NADPH-dependent bi-functional enzyme that performs alcohol dehydrogenase and aldehyde dehydrogenase (CoA-acylating) activities in the N- and C-terminal fragments, respectively. It catalyzes the two-step reduction of malonyl-CoA to 3-hydroxypropionate (3-HP), a key reaction in the autotrophic CO fixation cycles of green non-sulfur bacteria and the archaea . However, the structural basis underlying substrate selection, coordination, and the subsequent catalytic reactions of full-length MCR is largely unknown. For the first time, we here determined the structure of full-length MCR from the photosynthetic green non-sulfur bacterium (MCR) at 3.35 Å resolution. Furthermore, we determined the crystal structures of the N- and C-terminal fragments bound with reaction intermediates NADP and malonate semialdehyde (MSA) at 2.0 Å and 2.3 Å, respectively, and elucidated the catalytic mechanisms using a combination of molecular dynamics simulations and enzymatic analyses. Full-length MCR was a homodimer of two cross-interlocked subunits, each containing four tandemly arranged short-chain dehydrogenase/reductase (SDR) domains. Only the catalytic domains SDR1 and SDR3 incorporated additional secondary structures that changed with NADP-MSA binding. The substrate, malonyl-CoA, was immobilized in the substrate-binding pocket of SDR3 through coordination with Arg1164 and Arg799 of SDR4 and the extra domain, respectively. Malonyl-CoA was successively reduced through protonation by the Tyr743-Arg746 pair in SDR3 and the catalytic triad (Thr165-Tyr178-Lys182) in SDR1 after nucleophilic attack from NADPH hydrides. IMPORTANCE The bi-functional MCR catalyzes NADPH-dependent reduction of malonyl-CoA to 3-HP, an important metabolic intermediate and platform chemical, from biomass. The individual MCR-N and MCR-C fragments, which contain the alcohol dehydrogenase and aldehyde dehydrogenase (CoA-acylating) activities, respectively, have previously been structurally investigated and reconstructed into a malonyl-CoA pathway for the biosynthetic production of 3-HP. However, no structural information for full-length MCR has been available to illustrate the catalytic mechanism of this enzyme, which greatly limits our capacity to increase the 3-HP yield of recombinant strains. Here, we report the cryo-electron microscopy structure of full-length MCR for the first time and elucidate the mechanisms underlying substrate selection, coordination, and catalysis in the bi-functional MCR. These findings provide a structural and mechanistic basis for enzyme engineering and biosynthetic applications of the 3-HP carbon fixation pathways.
丙二酰辅酶 A 还原酶 (MCR) 是一种依赖 NADPH 的双功能酶,在 N 端和 C 端片段中分别具有醇脱氢酶和醛脱氢酶(酰基辅酶 A 化)活性。它催化丙二酰辅酶 A 两步还原为 3-羟基丙酸(3-HP),这是绿色非硫细菌和古菌自养 CO 固定循环中的关键反应。然而,全长 MCR 的底物选择、配位和随后的催化反应的结构基础在很大程度上尚不清楚。我们首次在 3.35Å 分辨率下测定了来自光合绿色非硫细菌(MCR)的全长 MCR 结构。此外,我们还分别以 2.0Å 和 2.3Å 的分辨率测定了与反应中间体 NADP 和丙二酰半醛(MSA)结合的 N 端和 C 端片段的晶体结构,并通过分子动力学模拟和酶分析相结合阐明了催化机制。全长 MCR 是两个交叉互锁亚基的同源二聚体,每个亚基包含四个串联排列的短链脱氢酶/还原酶(SDR)结构域。只有催化结构域 SDR1 和 SDR3 包含了与 NADP-MSA 结合变化相关的额外二级结构。底物丙二酰辅酶 A 通过与 SDR4 的 Arg1164 和 Arg799 以及额外结构域的配位固定在 SDR3 的底物结合口袋中。丙二酰辅酶 A 依次通过 SDR3 中的 Tyr743-Arg746 对和 SDR1 中的催化三联体(Thr165-Tyr178-Lys182)进行质子化,然后在 NADPH 氢化物的亲核攻击后被还原。重要性双功能 MCR 催化 NADPH 依赖性还原丙二酰辅酶 A 生成 3-HP,3-HP 是一种重要的代谢中间产物和平台化学品,可从生物质中获得。单独的 MCR-N 和 MCR-C 片段分别包含醇脱氢酶和醛脱氢酶(酰基辅酶 A 化)活性,以前已经进行了结构研究,并被重建为用于 3-HP 生物合成生产的丙二酰辅酶 A 途径。然而,尚无全长 MCR 的结构信息来阐明该酶的催化机制,这极大地限制了我们提高重组菌株 3-HP 产量的能力。在这里,我们首次报道了全长 MCR 的冷冻电子显微镜结构,并阐明了双功能 MCR 中底物选择、配位和催化的机制。这些发现为 3-HP 碳固定途径的酶工程和生物合成应用提供了结构和机制基础。
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