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大肠杆菌细胞表达来自恶臭假单胞菌 CA-3 的野生型和工程化苯乙烯单加氧酶对烷基芳基硫化物和苯并[b]噻吩的氧化作用。

The oxidation of alkylaryl sulfides and benzo[b]thiophenes by Escherichia coli cells expressing wild-type and engineered styrene monooxygenase from Pseudomonas putida CA-3.

机构信息

School of Biomolecular and Biomedical Sciences and Centre for Synthesis and Chemical Biology, University College Dublin, Belfield, Dublin 4, Ireland.

出版信息

Appl Microbiol Biotechnol. 2013 Jun;97(11):4849-58. doi: 10.1007/s00253-012-4332-5. Epub 2012 Aug 14.

DOI:10.1007/s00253-012-4332-5
PMID:22890778
Abstract

Nine different sulfur-containing compounds were biotransformed to the corresponding sulfoxides by Escherichia coli Bl21(DE3) cells expressing styrene monooxygenase (SMO) from Pseudomonas putida CA-3. Thioanisole was consumed at 83.3 μmoles min(-1) g cell dry weight(-1) resulting mainly in the formation of R-thioanisole sulfoxide with an enantiomeric excess (ee) value of 45 %. The rate of 2-methyl-, 2-chloro- and 2-bromo-thioanisole consumption was 2-fold lower than that of thioanisole. Surprisingly, the 2-methylthioanisole sulfoxide product had the opposite (S) configuration to that of the other 2-substituted thioanisole derivatives and had a higher ee value (84 %). The rate of oxidation of 4-substituted thioanisoles was higher than the corresponding 2-substituted substrates but the ee values of the products were consistently lower (10-23 %). The rate of benzo[b]thiophene and 2-methylbenzo[b]thiophene sulfoxidation was approximately 10-fold lower than that of thioanisole. The ee value of the benzo[b]thiophene sulfoxide could not be determined as the product racemized rapidly. E. coli cells expressing an engineered SMO (SMOeng R3-11) oxidised 2-substituted thioanisoles between 1.8- and 2.8-fold faster compared to cells expressing the wild-type enzyme. SMOeng R3-11 oxidised benzo[b]thiophene and 2-methylbenzo[b]thiophene 10.1 and 5.6 times faster that the wild-type enzyme. The stereospecificity of the reaction catalysed by SMOeng was unchanged from that of the wild type. Using the X-ray crystal structure of the P. putida S12 SMO, it was evident that the entrance of substrates into the SMO active site is limited by the binding pocket bottleneck formed by the side chains of Val-211 and Asn-46 carboxyamide group.

摘要

九种不同的含硫化合物被表达恶臭假单胞菌 CA-3 来源的苯乙烯单加氧酶(SMO)的大肠杆菌 BL21(DE3)细胞生物转化为相应的亚砜。硫代茴香醚的消耗速率为 83.3μmoles min(-1) g 细胞干重(-1),主要生成 R-硫代茴香醚亚砜,对映体过量(ee)值为 45%。2-甲基-、2-氯-和 2-溴-硫代茴香醚的消耗速率比硫代茴香醚低 2 倍。令人惊讶的是,2-甲基硫代茴香醚亚砜产物的构型与其他 2-取代硫代茴香醚衍生物相反,ee 值更高(84%)。4-取代硫代茴香醚的氧化速率高于相应的 2-取代底物,但产物的 ee 值始终较低(10-23%)。苯并[b]噻吩和 2-甲基苯并[b]噻吩的氧化速率比硫代茴香醚低约 10 倍。苯并[b]噻吩亚砜的 ee 值无法确定,因为产物迅速外消旋。表达工程化 SMO(SMOeng R3-11)的大肠杆菌细胞比表达野生型酶的细胞氧化 2-取代硫代茴香醚的速率快 1.8-2.8 倍。SMOeng R3-11 氧化苯并[b]噻吩和 2-甲基苯并[b]噻吩的速率分别比野生型酶快 10.1 倍和 5.6 倍。SMOeng 催化的反应的立体特异性与野生型酶相同。利用恶臭假单胞菌 S12 SMO 的 X 射线晶体结构,显然,底物进入 SMO 活性位点的入口受到由 Val-211 和 Asn-46 羧酰胺基团的侧链形成的结合口袋瓶颈的限制。

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