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从紧密枝孢中纯化和表征洛伐他汀酯酶。

Purification and Characterization of a Lovastatin Esterase from Clonostachys compactiuscula.

出版信息

Appl Environ Microbiol. 1997 Apr;63(4):1307-11. doi: 10.1128/aem.63.4.1307-1311.1997.

Abstract

An esterase from the fungus Clonostachys compactiuscula selectively hydrolyzes lovastatin, a clinically useful antihypercholesterolemic agent. Lovastatin or lovastatin-related compounds were required to induce the activity of the lovastatin 8(prm1)-((alpha)-methylbutyryloxy) esterase. The 46-kDa esterase was purified from mycelial extracts by centrifugation and a single anion-exchange chromatographic separation. Maximal lovastatin esterase activity was found at pH 9.0 to 9.6 and at 25 to 30(deg)C. The addition of 5 to 20% methanol resulted in greater lovastatin hydrolysis, while the addition of other solvents (ethanol, isopropanol, butanol, ethyl acetate, isopropyl acetate, or tetrahydrofuran) decreased hydrolysis. Lovastatin was selectively hydrolyzed even in the presence of an excess of simvastatin, another antihypercholesterolemic agent that is structurally very similar to lovastatin. This lovastatin 8(prm1)-((alpha)-methylbutyryloxy) esterase can be used to prepare a core intermediate for the generation of novel antihypercholesterolemic agents or to purify simvastatin prepared by C methylation of the 2(S)-methylbutyryloxy side chain of lovastatin.

摘要

一种来自真菌紧密链格孢的酯酶,能够选择性地水解洛伐他汀,这是一种临床有用的抗高胆固醇血症药物。洛伐他汀或与洛伐他汀相关的化合物是诱导洛伐他汀 8(prm1)-((alpha)-甲基丁酰氧基)酯酶活性所必需的。该 46 kDa 的酯酶可通过离心和单一阴离子交换色谱分离从菌丝体提取物中纯化得到。洛伐他汀酯酶的最大活性在 pH 9.0 至 9.6 和 25 至 30(deg)C 时发现。添加 5%至 20%甲醇可导致更多的洛伐他汀水解,而添加其他溶剂(乙醇、异丙醇、丁醇、乙酸乙酯、乙酸异丙酯或四氢呋喃)则会降低水解。即使存在过量的辛伐他汀(另一种结构与洛伐他汀非常相似的抗高胆固醇血症药物),洛伐他汀也能被选择性地水解。这种洛伐他汀 8(prm1)-((alpha)-甲基丁酰氧基)酯酶可用于制备新型抗高胆固醇血症药物的核心中间体,或用于纯化通过洛伐他汀 2(S)-甲基丁酰氧基侧链的 C 甲基化制备的辛伐他汀。

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本文引用的文献

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Bacterial penicillin amidase.细菌青霉素酰胺酶
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Enzymatic synthesis of hydrophobic penicillins.疏水性青霉素的酶促合成。
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Pleurotus fungi produce mevinolin, an inhibitor of HMG CoA reductase.
FEMS Microbiol Lett. 1993 Nov 1;113(3):333-7. doi: 10.1111/j.1574-6968.1993.tb06536.x.

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