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细胞质芳香醛脱氢酶为贯叶连翘中黄烷酮生物合成提供苯甲酸。

Cytosolic aromatic aldehyde dehydrogenase provides benzoic acid for xanthone biosynthesis in Hypericum.

机构信息

Technische Universität Braunschweig, Institute of Pharmaceutical Biology, Mendelssohnstraße 1, Braunschweig, 38106, Germany.

Technische Universität Braunschweig, Institute of Plant Biology, Humboldtstraße 1, Braunschweig, 38106, Germany.

出版信息

Plant Physiol Biochem. 2021 Mar;160:82-93. doi: 10.1016/j.plaphy.2021.01.011. Epub 2021 Jan 12.

DOI:10.1016/j.plaphy.2021.01.011
PMID:33482582
Abstract

Benzoic acid is a building block of a multitude of well-known plant natural products, such as paclitaxel and cocaine. Its simple chemical structure contrasts with its complex biosynthesis. Hypericum species are rich in polyprenylated benzoic acid-derived xanthones, which have received attention due to their biological impact on human health. The upstream biosynthetic sequence leading to xanthones is still incomplete. To supply benzoic acid for xanthone biosynthesis, Hypericum calycinum cell cultures use the CoA-dependent non-β-oxidative pathway, which starts with peroxisomal cinnamate CoA-ligase (HcCNL). Here, we use the xanthone-producing cell cultures to identify the transcript for benzaldehyde dehydrogenase (HcBD), a pivotal player in the non-β-oxidative pathways. In addition to benzaldehyde, the enzyme efficiently catalyzes the oxidation of trans-cinnamaldehyde in vitro. The enzymatic activity is strictly dependent on the presence of NAD as co-factor. HcBD is localized to the cytosol upon ectopic expression of reporter fusion constructs. HcBD oxidizes benzaldehyde, which moves across the peroxisome membrane, to form benzoic acid. Increases in the HcCNL and HcBD transcript levels precede the elicitor-induced xanthone accumulation. The current work addresses a crucial step in the yet incompletely understood CoA-dependent non-β-oxidative route of benzoic acid biosynthesis. Addressing this step may offer a new biotechnological tool to enhance product formation in biofactories.

摘要

苯甲酸是许多著名植物天然产物的结构单元,如紫杉醇和可卡因。其简单的化学结构与复杂的生物合成形成鲜明对比。贯叶金丝桃属植物富含多聚异戊烯基苯甲酸衍生的呫吨酮,由于其对人类健康的生物学影响而受到关注。导致呫吨酮生物合成的上游生物合成序列仍然不完整。为了提供用于呫吨酮生物合成的苯甲酸,贯叶金丝桃细胞培养物使用 CoA 依赖性非β-氧化途径,该途径始于过氧化物酶体肉桂酸 CoA 连接酶(HcCNL)。在这里,我们使用产生呫吨酮的细胞培养物来鉴定苯甲醛脱氢酶(HcBD)的转录物,苯甲醛脱氢酶是非β-氧化途径中的关键酶。除了苯甲醛外,该酶在体外还能有效地催化反式肉桂醛的氧化。酶活性严格依赖 NAD 作为辅酶。HcBD 在异位表达报告融合构建体时定位于细胞质。HcBD 将穿过过氧化物酶体膜的苯甲醛氧化形成苯甲酸。HcCNL 和 HcBD 转录物水平的增加先于诱导子诱导的呫吨酮积累。目前的工作解决了 CoA 依赖性非β-氧化途径中苯甲酸生物合成中一个关键步骤,该步骤的阐明可能为增强生物工厂中产物形成提供新的生物技术工具。

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