Biosynthesis of Indole Diterpene Lolitrems: Radical‐Induced Cyclization of an Epoxyalcohol Affording a Characteristic Lolitremane Skeleton

Jiang, Yulu; Ozaki, Taro; Harada, Masatoshi; Miyasaka, Tadachika; Sato, Hajime; Miyamoto, Kazunori; Kanazawa, Junichiro; Li, Chengwei; Maruyama, Jun‐ichi; Adachi, Masaatsu; Nakazaki, Atsuo; Nishikawa, Toshio; Uchiyama, Masanobu; Minami, Atsushi; Oikawa, Hideaki

doi:10.1002/ange.202007280

Cited by 8 publications

(3 citation statements)

References 30 publications

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“…CRISPR-KI has been mostly used to integrate fragments that span few kilobases, and although recently it has been used for the integration of larger BGC fragments in Aspergilli, the efficiency of targeted integration is not reported. 20,21 In contrast, recombinase-mediated integration does not generate dsDNA breaks and is orthogonal to the host machinery. This makes recombinase-based systems a convenient and reliable alternative for the single-step integration of large DNA constructs, where the efficiency of HR declines.…”

Section: Discussionmentioning

confidence: 99%

Cre/lox-mediated chromosomal integration of biosynthetic gene clusters for heterologous expression in Aspergillus nidulans

Roux

Chooi

2021

Preprint

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Building strains for stable long-term heterologous expression of large biosynthetic pathways in filamentous fungi is limited by the low transformation efficiency or genetic stability of current methods. Here, we developed a system for targeted chromosomal integration of large biosynthetic gene clusters in Aspergillus nidulans based on site-specific recombinase mediated cassette exchange. We built A. nidulans strains harbouring a chromosomal landing pad for Cre/lox-mediated recombination and demonstrated efficient targeted integration of a 21.5 kb heterologous region in a single step. We further evaluated the integration at two loci by analysing the expression of a fluorescent reporter and the production of a heterologous polyketide. We compared chromosomal expression at those landing loci to episomal AMA1-based expression, which also shed light on uncharacterised aspects of episomal expression in filamentous fungi. This is the first demonstration of site-specific recombinase-mediated integration in filamentous fungi, setting the foundations for the further development of this tool.

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Section: Discussionmentioning

confidence: 99%

Cre/lox-mediated chromosomal integration of biosynthetic gene clusters for heterologous expression in Aspergillus nidulans

Roux

Chooi

2021

Preprint

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“…The P450 LtmQ, which is homologous to PaxQ and AtmQ, performs hydroxylation to provide terpendole E (131) [105,106]. Compound 131 is subsequently transformed into terpendole C (132) by four enzymes, and finally, 130 is synthesized by the prenyltransferase LtmE and the P450 LtmJ from 132 [107,108]. In Chaunopycnis alba, an uncharacterized dehydrogenase oxidizes 132 to yield terpendole K (133) [106].…”

Section: Meroterpenoidsmentioning

confidence: 99%

Branching and converging pathways in fungal natural product biosynthesis

Wei

Wang

Matsuda

2022

Fungal Biol Biotechnol

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In nature, organic molecules with great structural diversity and complexity are synthesized by utilizing a relatively small number of starting materials. A synthetic strategy adopted by nature is pathway branching, in which a common biosynthetic intermediate is transformed into different end products. A natural product can also be synthesized by the fusion of two or more precursors generated from separate metabolic pathways. This review article summarizes several representative branching and converging pathways in fungal natural product biosynthesis to illuminate how fungi are capable of synthesizing a diverse array of natural products.

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“…Tandem transformation utilizing two plasmids with the same selectable marker is efficient, requiring the use of fewer vectors and allowing a rapid introduction of biosynthetic genes to obtain TFs. By applying this simple method, we completely elucidated the detailed biosynthetic pathway of fungal indole diterpenes such as shearinine, 34) lolitrem, 35) and especially penitrem 36) whose biosynthesis requires 17 genes, one of the largest number of genes in the fungal metabolite biosynthesis (Fig. 5).…”

Section: Discovery Of Daases In Fungal Phytotoxin Biosynthesismentioning

confidence: 99%

Heterologous production of fungal natural products: Reconstitution of biosynthetic gene clusters in model host <i>Aspergillus oryzae</i>

Oikawa

2020

Proc. Jpn. Acad., Ser. B

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While exploring phytotoxic metabolites from phytopathogenic fungi in the 1970s, we became interested in biosynthetic enzymes that catalyze Diels–Alder reactions involving biosynthesis of several phytotoxins that we isolated. Target enzymes were successfully characterized, and this triggered the identification of various Diels–Alderases in a recent decade. Through our Diels–Alderase project in 1990s, we recognized a highly efficient expression system of various biosynthetic genes with Aspergillus oryzae as a host. With the development of tools such as genomic data and bioinformatics analysis to identify biosynthetic gene clusters for natural products, we developed a highly reliable methodology such as hot spot knock-in to elucidate the biosynthetic pathways of representative fungal metabolites including phytotoxic substances. This methodology allows total biosynthesis of natural products and genome mining using silent biosynthetic gene clusters to obtain novel bioactive metabolites. Further applications of this technology are discussed.

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Biosynthesis of Indole Diterpene Lolitrems: Radical‐Induced Cyclization of an Epoxyalcohol Affording a Characteristic Lolitremane Skeleton

Cited by 8 publications

References 30 publications

Cre/lox-mediated chromosomal integration of biosynthetic gene clusters for heterologous expression in Aspergillus nidulans

Cre/lox-mediated chromosomal integration of biosynthetic gene clusters for heterologous expression in Aspergillus nidulans

Branching and converging pathways in fungal natural product biosynthesis

Heterologous production of fungal natural products: Reconstitution of biosynthetic gene clusters in model host <i>Aspergillus oryzae</i>

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