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藤仓镰孢菌中红色色素比卡维林的生物合成:基因、其功能与调控

Biosynthesis of the red pigment bikaverin in Fusarium fujikuroi: genes, their function and regulation.

作者信息

Wiemann Philipp, Willmann Anita, Straeten Marcus, Kleigrewe Karin, Beyer Marita, Humpf Hans-Ulrich, Tudzynski Bettina

机构信息

Institut für Botanik, Schlossgarten 3, Westfälische Wilhelms-Universität Münster, D-48149 Münster, Germany.

出版信息

Mol Microbiol. 2009 May;72(4):931-46. doi: 10.1111/j.1365-2958.2009.06695.x. Epub 2009 Apr 14.

DOI:10.1111/j.1365-2958.2009.06695.x
PMID:19400779
Abstract

Fusarium secondary metabolites are structurally diverse, have a variety of activities and are generally poorly understood biosynthetically. The F. fujikuroi polyketide synthase gene bik1 was previously shown to be responsible for formation of the mycelial pigment bikaverin. Here we present the characterization of five genes adjacent to bik1 as encoding a putative FAD-dependent monooxygenase (bik2), an O-methyltransferase (bik3), an NmrA-like protein (bik4), a Zn(II)2Cys6 transcription factor (bik5) and an MFS transporter (bik6). Deletion of each gene resulted in total loss or significant reduction of bikaverin synthesis. Expression studies revealed that all bik genes are repressed by high amounts of nitrogen in an AreA-independent manner and are subject to a time- and pH-dependent regulation. Deletion of the pH regulatory gene pacC resulted in partial derepression while complementation with a dominant active allele resulted in repression of bik genes at acidic ambient pH. Transcription of all bik genes in strains lacking bik1, bik2 or bik3 was essentially eliminated, while transcription of some bik genes was detected in strains lacking bik4, bik5 or bik6. Thus, bikaverin synthesis is regulated by a complex regulatory network. Understanding how different factors influence the synthesis of this model secondary metabolite will aid understanding secondary metabolism in general.

摘要

镰刀菌的次生代谢产物结构多样,具有多种活性,但其生物合成过程通常还知之甚少。先前已表明,藤仓镰孢菌的聚酮合酶基因bik1负责菌丝色素比卡维林的形成。在此,我们描述了与bik1相邻的五个基因,它们分别编码一种假定的FAD依赖性单加氧酶(bik2)、一种O-甲基转移酶(bik3)、一种NmrA样蛋白(bik4)、一种Zn(II)2Cys6转录因子(bik5)和一种MFS转运蛋白(bik6)。每个基因的缺失都会导致比卡维林合成完全丧失或显著减少。表达研究表明,所有bik基因都以不依赖于AreA的方式被大量氮抑制,并且受到时间和pH依赖性调控。pH调节基因pacC的缺失导致部分去抑制,而用显性活性等位基因互补则导致在酸性环境pH下bik基因受到抑制。在缺乏bik1、bik2或bik3的菌株中,所有bik基因的转录基本消除,而在缺乏bik4、bik5或bik6的菌株中检测到一些bik基因的转录。因此,比卡维林的合成受复杂的调控网络调节。了解不同因素如何影响这种典型次生代谢产物的合成将有助于总体上理解次生代谢。

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