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紫杉醇途径10 - O - 乙酰转移酶对4 - 去乙酰紫杉醇的氧杂环丁烷羟基表现出区域选择性混杂。

The taxol pathway 10-O-acetyltransferase shows regioselective promiscuity with the oxetane hydroxyl of 4-deacetyltaxanes.

作者信息

Ondari Mark E, Walker Kevin D

机构信息

Department of Chemistry, Michigan State University, East Lansing, Michigan 48824, USA.

出版信息

J Am Chem Soc. 2008 Dec 17;130(50):17187-94. doi: 10.1021/ja8067534.

DOI:10.1021/ja8067534
PMID:19007225
Abstract

The 10-deacetylbaccatin III:10beta-O-acetyltransferase isolated from Taxus cuspidata regiospecifically transfers short-chain alkanoyl groups from their corresponding CoA thioesters to the C10 hydroxyl of 10-deacetylbaccatin III. This 10-O-acetyltransferase along with five other Taxus acyltransferases on the paclitaxel (Taxol) biosynthetic pathway and one additional Taxus-derived acyltransferases of unknown function were screened for 4-O-acetyltransferase activity against 4-deacetylbaccatin III, 7-acetyl-, 13-acetyl-, and 7,13-diacetyl-4-deacetylbaccatin III. These 4-deacyl derivatives were semisynthesized from the natural product baccatin III via silyl protecting group manipulation, regioselective reductive ester cleavage with sodium bis(2-methoxyethoxy)aluminum hydride, and regioselective acetylation with acetic anhydride. Assays with the 4-deacetylated diterpene substrates and acetyl CoA revealed the taxane 10beta-O-acetyltransferase was able to catalyze the 4-O-acetylation of 4-deacetylbaccatin III to baccatin III and 13-acetyl-4-deacetylbacatin III to 13-acetylbaccatin III, although each was converted at lesser efficiency than with the natural substrate. In contrast, this enzyme was unable to acetylate 7-acetyl-4-deacetylbaccatin III and 7,13-diacetyl-4-deacetylbaccatin III substrates at C4, suggesting that the C7 hydroxyl of baccatin III must remain deacylated for enzyme function. The biocatalytic transfer of an acyl group to the tertiary hydroxyl on the oxetane moiety at C4 of the taxane ring demonstrates that the regiochemistry of the 10beta-acetyltransferase is mutable.

摘要

从东北红豆杉中分离出的10 - 去乙酰浆果赤霉素III:10β - O - 乙酰转移酶能区域特异性地将短链烷酰基从其相应的辅酶A硫酯转移至10 - 去乙酰浆果赤霉素III的C10羟基上。针对4 - 去乙酰浆果赤霉素III、7 - 乙酰 - 、13 - 乙酰 - 和7,13 - 二乙酰 - 4 - 去乙酰浆果赤霉素III,对这条紫杉醇生物合成途径上的这种10 - O - 乙酰转移酶以及其他五种红豆杉酰基转移酶和一种功能未知的源自红豆杉的酰基转移酶进行了4 - O - 乙酰转移酶活性筛选。这些4 - 脱酰基衍生物是通过硅烷基保护基操作、用双(2 - 甲氧基乙氧基)氢化铝钠进行区域选择性还原酯裂解以及用乙酸酐进行区域选择性乙酰化,从天然产物浆果赤霉素III半合成得到的。用4 - 脱乙酰化二萜底物和乙酰辅酶A进行的测定表明,紫杉烷10β - O - 乙酰转移酶能够催化4 - 去乙酰浆果赤霉素III向浆果赤霉素III以及13 - 乙酰 - 4 - 去乙酰浆果赤霉素III向13 - 乙酰浆果赤霉素III的4 - O - 乙酰化反应,尽管与天然底物相比,每种底物的转化效率都较低。相比之下,这种酶无法在C4处将7 - 乙酰 - 4 - 去乙酰浆果赤霉素III和7,13 - 二乙酰 - 4 - 去乙酰浆果赤霉素III底物乙酰化,这表明浆果赤霉素III的C7羟基必须保持脱酰基状态才能发挥酶的功能。将酰基生物催化转移至紫杉烷环C4处氧杂环丁烷部分的叔羟基上,表明10β - 乙酰转移酶的区域化学性质是可变的。

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