Promoter tools for further development of Aspergillus oryzae as a platform for fungal secondary metabolite production.

Q1 Agricultural and Biological Sciences Fungal Biology and Biotechnology Pub Date : 2020-03-23 eCollection Date: 2020-01-01 DOI:10.1186/s40694-020-00093-1
Maiko Umemura, Kaoru Kuriiwa, Linh Viet Dao, Tetsuya Okuda, Goro Terai
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引用次数: 14

Abstract

Background: The filamentous fungus Aspergillus oryzae is widely used for secondary metabolite production by heterologous expression; thus, a wide variety of promoter tools is necessary to broaden the application of this species. Here we built a procedure to survey A. flavus genes constitutively highly expressed in 83 transcriptome datasets obtained under various conditions affecting secondary metabolite production, to find promoters useful for heterologous expression of genes in A. oryzae.

Results: To test the ability of the promoters of the top 6 genes to induce production of a fungal secondary metabolite, ustiloxin B, we inserted the promoters before the start codon of ustR, which encodes the transcription factor of the gene cluster responsible for ustiloxin B biosynthesis, in A. oryzae. Four of the 6 promoters induced ustiloxin B production in all tested media (solid maize, liquid V8 and PDB media), and also ustR expression. Two of the 4 promoters were those of tef1 and gpdA, which are well characterized in A. oryzae and A. nidulans, respectively, whereas the other two, those of AFLA_030930 and AFLA_113120, are newly reported here and show activities comparable to that of the gpdA promoter with respect to induction of gene expression and ustiloxin B production.

Conclusion: We newly reported two sequences as promoter tools for secondary metabolite production in A. oryzae. Our results demonstrate that our simple strategy of surveying for constitutively highly expressed genes in large-scale transcriptome datasets is useful for finding promoter sequences that can be used as heterologous expression tools in A. oryzae.

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进一步开发米曲霉作为真菌次生代谢物生产平台的启动子工具。
背景:丝状真菌米曲霉(Aspergillus oryzae)被广泛应用于异源表达产生次生代谢物;因此,需要多种多样的启动子工具来扩大该物种的应用。在此,我们建立了一个程序来调查在影响次级代谢物产生的各种条件下获得的83个转录组数据集中组成性高表达的a . flavus基因,以寻找对a . oryzae基因异源表达有用的启动子。结果:为了测试前6个基因启动子诱导真菌次生代谢产物ustiloxin B产生的能力,我们将启动子插入到a . oryzae中编码ustiloxin B生物合成基因簇转录因子的ustR起始密码子之前。6个启动子中的4个在所有测试培养基(固体玉米、液体V8和PDB培养基)中诱导了ustiloxin B的产生,并诱导了ustR的表达。在这4个启动子中,tef1和gpdA两个启动子分别在a.m oryzae和a.n idulans中得到了很好的表征,而另外两个启动子AFLA_030930和AFLA_113120是本文新报道的,在诱导基因表达和ustiloxin B产生方面显示出与gpdA启动子相当的活性。结论:我们新报道了两个序列作为m.o ryzae次级代谢物产生的启动子工具。我们的研究结果表明,我们在大规模转录组数据集中测量组成型高表达基因的简单策略对于寻找可作为水稻芽孢杆菌异源表达工具的启动子序列是有用的。
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来源期刊
Fungal Biology and Biotechnology
Fungal Biology and Biotechnology Agricultural and Biological Sciences-Ecology, Evolution, Behavior and Systematics
CiteScore
10.20
自引率
0.00%
发文量
17
审稿时长
9 weeks
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