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地衣半绿黄髓盘衣中一个非还原型聚酮合酶基因的克隆与序列特征分析

Cloning and sequence characterization of a non-reducing polyketide synthase gene from the lichen Xanthoparmelia semiviridis.

作者信息

Chooi Yit-Heng, Stalker David M, Davis Meryl A, Fujii Isao, Elix John A, Louwhoff Simone H J J, Lawrie Ann C

机构信息

School of Applied Sciences, RMIT University, Bundoora Campus, PO Box 71, Bundoora VIC 3083, Australia.

出版信息

Mycol Res. 2008 Feb;112(Pt 2):147-61. doi: 10.1016/j.mycres.2007.08.022. Epub 2007 Sep 15.

DOI:10.1016/j.mycres.2007.08.022
PMID:18280724
Abstract

Lichens produce a diverse array of secondary metabolites that have shown various biological activities. Of particular interest are the coupled phenolics that originate from polyketide pathways, such as depsides, depsidones and usnic acids, which are produced almost solely by lichens. Based on the presumed catalytic domains required for the synthesis of the key intermediates beta-orsellinic acid and methylphloroacetophenone, two pairs of degenerate primers were designed to target specifically the beta-ketoacylsynthase (KS) and C-methyltransferase (CMeT) domains of fungal non-reducing polyketide synthase (NR-PKS) genes with CMeT domains. These primers were used to explore the genome of the lichen Xanthoparmelia semiviridis, which produces beta-orcinol depsidones and usnic acid. One of the two KS domains amplified from genomic DNA of field-collected X. semiviridis was used as a probe to recover the candidate PKS gene. A 13 kb fragment containing an intact putative PKS gene (xsepks1) of 6555 bp was recovered from a partial genomic library. The inferred amino acid sequence indicated that xsepks1 encodes a protein of 2164 amino acids and contains KS, acyltransferase (AT), acyl carrier protein (ACP) and CMeT domains as expected. This demonstrated a successful strategy for targeting non-reducing PKS genes with CMeT domains. Integration of the 5' fragment of xsepks1, including the native promoter, into Aspergillus nidulans by cotransformation resulted in the transcription of the 5'xsepks1 and the splicing of a 63 bp intron, suggesting that A. nidulans could be a suitable heterologous host for xsepks1 expression.

摘要

地衣能产生一系列具有多种生物活性的次生代谢产物。特别令人感兴趣的是源自聚酮化合物途径的偶联酚类,如缩酚酸、缩酚酮和松萝酸,它们几乎仅由地衣产生。基于合成关键中间体β - 苔黑酚酸和甲基氯代苯乙酮所需的假定催化结构域,设计了两对简并引物,专门靶向具有C - 甲基转移酶(CMeT)结构域的真菌非还原型聚酮合酶(NR - PKS)基因的β - 酮酰基合酶(KS)和C - 甲基转移酶(CMeT)结构域。这些引物被用于探索地衣半绿黄髓盘衣(Xanthoparmelia semiviridis)的基因组,该物种能产生β - 苔黑酚缩酚酮和松萝酸。从野外采集的半绿黄髓盘衣基因组DNA中扩增出的两个KS结构域之一被用作探针来回收候选PKS基因。从一个部分基因组文库中获得了一个13 kb的片段,其中包含一个6555 bp的完整假定PKS基因(xsepks1)。推断的氨基酸序列表明,xsepks1编码一个2164个氨基酸的蛋白质,并且如预期那样包含KS、酰基转移酶(AT)、酰基载体蛋白(ACP)和CMeT结构域。这证明了一种针对具有CMeT结构域的非还原型PKS基因的成功策略。通过共转化将xsepks1的5'片段(包括天然启动子)整合到构巢曲霉中,导致5'xsepks1的转录以及一个63 bp内含子的剪接,这表明构巢曲霉可能是xsepks1表达的合适异源宿主。

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