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戈登氏菌 SoCg 中烷烃羟化酶系统在固体烷烃降解中的作用。

Involvement of an alkane hydroxylase system of Gordonia sp. strain SoCg in degradation of solid n-alkanes.

机构信息

Dipartimento di Biologia Cellulare e dello Sviluppo, Viale delle Scienze edif. 16, 90128 Palermo, Italy.

出版信息

Appl Environ Microbiol. 2011 Feb;77(4):1204-13. doi: 10.1128/AEM.02180-10. Epub 2010 Dec 23.

DOI:10.1128/AEM.02180-10
PMID:21183636
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3067205/
Abstract

Enzymes involved in oxidation of long-chain n-alkanes are still not well known, especially those in gram-positive bacteria. This work describes the alkane degradation system of the n-alkane degrader actinobacterium Gordonia sp. strain SoCg, which is able to grow on n-alkanes from dodecane (C(12)) to hexatriacontane (C(36)) as the sole C source. SoCg harbors in its chromosome a single alk locus carrying six open reading frames (ORFs), which shows 78 to 79% identity with the alkane hydroxylase (AH)-encoding systems of other alkane-degrading actinobacteria. Quantitative reverse transcription-PCR showed that the genes encoding AlkB (alkane 1-monooxygenase), RubA3 (rubredoxin), RubA4 (rubredoxin), and RubB (rubredoxin reductase) were induced by both n-hexadecane and n-triacontane, which were chosen as representative long-chain liquid and solid n-alkane molecules, respectively. Biotransformation of n-hexadecane into the corresponding 1-hexadecanol was detected by solid-phase microextraction coupled with gas chromatography-mass spectrometry (SPME/GC-MS) analysis. The Gordonia SoCg alkB was heterologously expressed in Escherichia coli BL21 and in Streptomyces coelicolor M145, and both hosts acquired the ability to transform n-hexadecane into 1-hexadecanol, but the corresponding long-chain alcohol was never detected on n-triacontane. However, the recombinant S. coelicolor M145-AH, expressing the Gordonia alkB gene, was able to grow on n-triacontane as the sole C source. A SoCg alkB disruption mutant that is completely unable to grow on n-triacontane was obtained, demonstrating the role of an AlkB-type AH system in degradation of solid n-alkanes.

摘要

参与长链正烷烃氧化的酶仍然知之甚少,特别是在革兰氏阳性菌中。本工作描述了正烷烃降解菌 Gordonia 属 sp. 菌株 SoCg 的烷烃降解系统,该菌株能够以十二烷(C(12))至三十六烷(C(36))正烷烃作为唯一碳源进行生长。SoCg 染色体上有一个单一的烷烃基因座,带有六个开放阅读框(ORFs),与其他烷烃降解放线菌的烷烃羟化酶(AH)编码系统具有 78%至 79%的同源性。定量反转录-PCR 显示,编码 AlkB(烷烃 1-单加氧酶)、RubA3(rubredoxin)、RubA4(rubredoxin)和 RubB(rubredoxin reductase)的基因均被 n-十六烷和 n-三十烷诱导,分别选择这两种代表长链液体和固体正烷烃分子。通过固相微萃取结合气相色谱-质谱联用(SPME/GC-MS)分析检测到 n-十六烷转化为相应的 1-十六醇。Gordonia SoCg alkB 在大肠杆菌 BL21 和链霉菌 M145 中异源表达,两种宿主均获得了将 n-十六烷转化为 1-十六醇的能力,但从未在 n-三十烷上检测到相应的长链醇。然而,表达 Gordonia alkB 基因的重组链霉菌 M145-AH 能够以 n-三十烷作为唯一碳源生长。获得了一株完全不能在 n-三十烷上生长的 SoCg alkB 缺失突变体,证明了 AlkB 型 AH 系统在固体正烷烃降解中的作用。

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