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一种来自快乐鼠尾草 Salvia sclarea 的二萜合酶催化香叶基香叶基二磷酸环化为(8R)-羟基-牻牛儿基二磷酸。

A diterpene synthase from the clary sage Salvia sclarea catalyzes the cyclization of geranylgeranyl diphosphate to (8R)-hydroxy-copalyl diphosphate.

机构信息

Donald Danforth Plant Science Center, St. Louis, MO 63132, USA.

出版信息

Phytochemistry. 2013 Jul;91:93-9. doi: 10.1016/j.phytochem.2012.07.019. Epub 2012 Sep 6.

DOI:10.1016/j.phytochem.2012.07.019
PMID:22959531
Abstract

The bicyclic diterpene (-)-sclareol is accumulated in glandular trichomes in Salvia sclarea (Schmiderer et al., 2008), and is a major terpenoid component of this plant species. It is used as the starting material for Ambrox synthesis, a synthetic ambergris analog used in the flavor and fragrance industry. In order to investigate the formation of sclareol, cDNA prepared from secretory cells of glandular trichomes from S. sclarea inflorescence were randomly sequenced. A putative copalyl diphosphate synthase encoding EST, SscTPS1, was functionally expressed in Escherichia coli. Whereas reaction of geranylgeranyl diphosphate with the putative copalyl diphosphate synthase followed by hydrolysis with alkaline phosphatase yielded a diastereomeric mixture of (13R)- and (13S)-manoyl oxide, HCl hydrolysis yielded (-)-sclareol (1) and 13-epi-sclareol as products. The product of the reaction of SscTPS1 with geranylgeranyl diphosphate was subjected to analysis by LC-negative ion ESI-MS/MS without prior hydrolysis. EPI scans were consistent with copalyl diphosphate to which 18 mass units had added (m/z 467 M+H). The enzymatic reaction was also carried out in the presence of 60% H2(18)O. LC-negative ion ESI-MS/MS analysis established an additional reaction product consistent with the incorporation of (18)O. Incubation in the presence of 60% (2)H2O resulted in the incorporation of one deuterium atom. These results suggest water capture of the carbocation intermediate, which is known to occur in reactions catalyzed by monoterpene synthases, but has been described only several times for diterpene synthases.

摘要

双环二萜(-)-喇叭醇在香紫苏(Schmiderer 等人,2008)的腺毛中积累,是该植物物种的主要萜烯成分。它被用作 Ambrox 合成的起始原料,一种用于香料和香精行业的合成龙涎香类似物。为了研究喇叭醇的形成,从香紫苏花序腺毛的分泌细胞中制备 cDNA,并对其进行随机测序。从香紫苏花序腺毛的分泌细胞中制备 cDNA,并对其进行随机测序。从香紫苏花序腺毛的分泌细胞中制备 cDNA,并对其进行随机测序。一个假定的牻牛儿基焦磷酸合酶编码 EST,SscTPS1,在大肠杆菌中功能表达。当用碱性磷酸酶水解法用香叶基香叶基二磷酸与假定的牻牛儿基焦磷酸合酶反应后,得到(13R)-和(13S)-马诺氧化物的非对映异构体混合物,用 HCl 水解得到(-)-喇叭醇(1)和 13-表-喇叭醇作为产物。用 SscTPS1 与香叶基香叶基二磷酸反应的产物不经水解直接进行 LC-负离子 ESI-MS/MS 分析。EPI 扫描与添加了 18 个质量单位的牻牛儿基焦磷酸一致(m/z 467 M+H)。该酶促反应也在 60% H2(18)O 的存在下进行。LC-负离子 ESI-MS/MS 分析确定了一个与(18)O 掺入一致的额外反应产物。在 60%(2)H2O 的存在下孵育导致一个氘原子的掺入。这些结果表明,在单萜合酶催化的反应中已知发生的碳正离子中间体的水捕获,但仅几次描述过二萜合酶。

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