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鉴定出负责使柄型取代烷基和烷氧基苯酚的黄素单加氧酶在斯氏假单胞菌 TTNP3 和噬拜拉姆鞘氨醇单胞菌中的作用。

Identification of the flavin monooxygenase responsible for ipso substitution of alkyl and alkoxyphenols in Sphingomonas sp. TTNP3 and Sphingobium xenophagum Bayram.

机构信息

Department of Microbiology, Cornell University, Ithaca, New York, NY, USA.

出版信息

Appl Microbiol Biotechnol. 2012 Apr;94(1):261-72. doi: 10.1007/s00253-011-3621-8. Epub 2011 Oct 20.

DOI:10.1007/s00253-011-3621-8
PMID:22012340
Abstract

We previously showed that opdA from Sphingomonas sp. PWE1 encodes a putative flavin monooxygenase capable of transforming octylphenol (OP) via type II ipso substitution. Here, we demonstrate that an opdA homolog is responsible for OP and related alkyl/alkoxyphenol degradation in the nonylphenol degrader Sphingomonas sp. TTNP3. PCR and Southern blot analyses revealed that TTNP3 contained an opdA homolog, while a TTNP3 derivative unable to grow on nonylphenol (TTNP3d) did not. OpdA expression was confirmed in wild-type TTNP3 via two dimensional gel electrophoresis. Activity was restored to TTNP3d following complementation with opdA. Sequence analysis of an opdA homolog from another nonylphenol degrader, Sphingobium xenophagum Bayram, revealed that the predicted protein sequences from PWE1 and Bayram were identical, but differed from TTNP3 by four amino acids. In order to assess differences, we heterologously expressed the two unique opdA homologs and compared their effect on the disappearance of five alkyl/alkoxyphenol substrates and subsequent appearance of hydroquinone. For all substrates, except OP, the levels of substrate disappearance and hydroquinone appearance were significantly lower in cultures expressing odpA (TTNP3) than those expressing opdA (PWE1/Bayram). These differences in substrate specificity were consistent with an in silico model which predicted that two of the amino acid differences between odpA (TTNP3) and opdA (PWE1/Bayram) lay in a putative substrate binding pocket. While these strains are known to use the same type II ipso substitution mechanism for alkylphenol degradation, this work provides the first preliminary evidence that opdA homologs also encode the type I ipso substitution activity responsible for the degradation of alkoxyphenols.

摘要

我们之前表明,来自鞘氨醇单胞菌 PWE1 的 opdA 编码一种可能的黄素单加氧酶,能够通过 II 型邻位取代转化辛基酚(OP)。在这里,我们证明 opdA 同源物负责壬基酚降解菌鞘氨醇单胞菌 TTNP3 中 OP 和相关的烷基/烷氧基苯酚的降解。PCR 和 Southern 印迹分析表明,TTNP3 含有一个 opdA 同源物,而不能在壬基酚上生长的 TTNP3 衍生物(TTNP3d)则没有。通过二维凝胶电泳证实了野生型 TTNP3 中的 OpdA 表达。用 opdA 互补后,TTNP3d 的活性得以恢复。来自另一种壬基酚降解菌食酚鞘氨醇单胞菌的 opdA 同源物的序列分析表明,PWE1 和 Bayram 的预测蛋白序列完全相同,但与 TTNP3 有四个氨基酸的差异。为了评估差异,我们异源表达了这两个独特的 opdA 同源物,并比较了它们对五种烷基/烷氧基苯酚底物消失和随后对氢醌出现的影响。除了 OP,表达 odpA(TTNP3)的培养物中底物消失和氢醌出现的水平明显低于表达 opdA(PWE1/Bayram)的培养物。这些底物特异性的差异与一个计算机模型一致,该模型预测 odpA(TTNP3)和 opdA(PWE1/Bayram)之间的两个氨基酸差异位于一个假定的底物结合口袋中。虽然这些菌株已知使用相同的 II 型邻位取代机制来降解烷基酚,但这项工作首次提供了初步证据,表明 opdA 同源物还编码负责降解烷氧基苯酚的 I 型邻位取代活性。

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