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表皮短杆菌HCU菌株中参与环己酮氧化的两个基因簇的鉴定。

Identification of two gene clusters involved in cyclohexanone oxidation in Brevibacterium epidermidis strain HCU.

作者信息

Brzostowicz P C, Blasko M S, Rouvière P E

机构信息

E. I. du Pont de Nemours and Co., Central Research and Development, Wilmington, DE 19880-0328, USA.

出版信息

Appl Microbiol Biotechnol. 2002 May;58(6):781-9. doi: 10.1007/s00253-002-0968-x. Epub 2002 Mar 27.

Abstract

Brevibacterium epidermidis HCU can grow on cyclic ketones and alcohols as a sole carbon source. We have previously reported the identification of two cyclohexanone-induced Bayer-Villiger monooxygenase genes by mRNA differential display. Using the related technique of Out-PCR, we have amplified large DNA fragments flanking the two monooxygenase genes. Two large gene clusters were sequenced. Several ORFs in each gene cluster encoded proteins homologous to cyclohexanol and cyclohexanone oxidation enzymes from Acinetobacter. However, the structure of these two gene clusters differs significantly from that of Acinetobacter, where the complete pathway has been described. To assess activity of these genes, they were cloned and expressed in Escherichia coli. In vivo and in vitro assays enabled us to assign functions to the expressed ORFs. These ORFs included a cyclohexanol dehydrogenase, two different epsilon-caprolactone hydrolases and two 6-hydroxyhexanoate dehydrogenases belonging to different enzyme families. Because this environmental isolate is difficult to manipulate, we cannot determine at this time which cluster is involved in the degradation of cyclohexanone under physiological conditions. However, the original differential display experiments and some of the experiments reported here suggest the involvement of both gene clusters in the oxidation of cyclic ketones.

摘要

表皮短杆菌HCU能够以环酮和醇类作为唯一碳源生长。我们之前曾报道通过mRNA差异显示鉴定出两个环己酮诱导的拜耳-维利格单加氧酶基因。利用外显子PCR相关技术,我们扩增了这两个单加氧酶基因两侧的大片段DNA。对两个大的基因簇进行了测序。每个基因簇中的几个开放阅读框编码的蛋白质与不动杆菌属的环己醇和环己酮氧化酶同源。然而,这两个基因簇的结构与已描述完整代谢途径的不动杆菌属的基因簇结构有显著差异。为了评估这些基因的活性,将它们克隆并在大肠杆菌中表达。体内和体外试验使我们能够确定所表达开放阅读框的功能。这些开放阅读框包括一个环己醇脱氢酶、两种不同的ε-己内酯水解酶和两种属于不同酶家族的6-羟基己酸脱氢酶。由于这种环境分离株难以操作,我们目前无法确定在生理条件下哪个基因簇参与环己酮的降解。然而,最初的差异显示实验以及本文报道的一些实验表明这两个基因簇都参与环酮的氧化。

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