Exploiting a precise design of universal synthetic modular regulatory elements to unlock the microbial natural products in
 Streptomyces

Bai, Chaoxian; Zhang, Yang; Zhao, Xuejin; Hu, Yiling; Xiang, Sihai; Miao, Junwei; Lou, Chunbo; Zhang, Lixin

doi:10.1073/pnas.1511027112

Cited by 163 publications

(199 citation statements)

References 41 publications

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“…The oligonucleotides FadD-F-KasO*-RBS-BamHI and FadD-R-EcoRI were used to amplify the fadD1 gene using genomic DNA of S. coelicolor as template. The FadD-F-KasO*-RBS-BamHI forward primer contains a BamHI site (underlined), the RBS of helicase (italics) from phage ϕC31 [Smith et al, 1999], and a kasOp* (bold) strong promoter [Bai et al, 2015], which controls the expression of fadD1 and fadE. The FadD-R-EcoRI reverse primer contains an EcoRI site (underlined).…”

Section: Construction Of the Recombinantmentioning

confidence: 99%

Improvement of Spinosad Production upon Utilization of Oils and Manipulation of β-Oxidation in a High-Producing Saccharopolyspora spinosa Strain

et al. 2018

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Spinosad, a member of polyketide-derived macrolides produced in the actinomycete Saccharopolyspora spinosa, has been developed as a broad-spectrum and effective insecticide. The β-oxidation pathway could be an important source of building blocks for the biosynthesis of spinosad, thus the effect of vegetable oils on the production of spinosad in a high-yield strain was investigated. The spinosad production increased significantly with the addition of strawberry seed oil (511.64 mg/L) and camellia oil (520.07 mg/L) compared to the control group without oil (285.76 mg/L) and soybean oil group (398.11 mg/L). It also revealed that the addition of oils would affect the expression of genes involved in fatty acid metabolism, precursor supply, and oxidative stress. The genetically engineered strain, in which fadD1 and fadE genes of Streptomyces coelicolor were inserted, produced spinosad up to 784.72 mg/L in the medium containing camellia oil, while a higher spinosad production level (843.40 mg/L) was detected with the addition of 0.01 mM of thiourea.

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Section: Construction Of the Recombinantmentioning

confidence: 99%

Improvement of Spinosad Production upon Utilization of Oils and Manipulation of β-Oxidation in a High-Producing Saccharopolyspora spinosa Strain

et al. 2018

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“…When fused to regulatory elements, reporter genes provide quantifiable signals that can be used to monitor the performance of genetic parts and entire genetic circuits. Quantitative reporter genes shown to work in actinomycetes include gfp encoding the green fluorescent protein (GFP), 21 xylE encoding for catechol 2,3-dioxygenase that converts colorless catechol to yellow hydroxymuconic semialdehyde, 33 luxAB and luxCDABE operons encoding luciferases, 25, 34 and gusA encoding for a beta-glucuronidase that converts different substrates for chromogenic, fluorescent, spectroscopic or chemiluminescent readouts. 32 When selecting the appropriate reporter gene, important considerations include the scalability, sensitivity (signal-to-noise) and dynamic range of the assay in the host of interest, as well as the option of a real-time or end-point assay.…”

Section: Advances In Genetic Engineering Of Actinomycetesmentioning

confidence: 99%

Engineering microbial hosts for production of bacterial natural products

et al. 2016

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Microbial fermentation provides as an attractive alternative to chemical synthesis for the production of structurally complex natural products. In most cases, however, production titers are low and need to be improved for compound characterization and/or commercial production. Owing to advances in functional genomics and genetic engineering technologies, microbial hosts can be engineered to overproduce a desired natural product, greatly accelerating the traditionally time-consuming strain improvement process. This review covers recent developments and challenges in the engineering of native and heterologous microbial hosts for production of bacterial natural products, focusing on the genetic tools and strategies for strain improvement. Special emphasis is placed on bioactive secondary metabolites from actinomycetes. The considerations for the choice of host systems will also be discussed in this review.

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“…Recently, many synthetic and natural promoters were developed for use in various Streptomyces strains. [29][30][31][32] Luo, Zhang and coworkers 33 , using a fluorescence-activated cell sorting-based high-throughput screening with a fluorescent protein reporter, characterized ca. 200 native or synthetic promoters and ca.…”

Section: Production Hostmentioning

confidence: 99%

Bio-based production of fuels and industrial chemicals by repurposing antibiotic-producing type I modular polyketide synthases: opportunities and challenges

2016

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Complex polyketides comprise a large number of natural products that have broad application in medicine and agriculture. They are produced in bacteria and fungi from large enzyme complexes named type I modular polyketide synthases (PKSs) that are composed of multifunctional polypeptides containing discrete enzymatic domains organized into modules. The modular nature of PKSs has enabled a multitude of efforts to engineer the PKS genes to produce novel polyketides of predicted structure. We have repurposed PKSs to produce a number of short-chain mono-and di-carboxylic acids and ketones that could have applications as fuels or industrial chemicals.

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Exploiting a precise design of universal synthetic modular regulatory elements to unlock the microbial natural products in Streptomyces

Cited by 163 publications

References 41 publications

Improvement of Spinosad Production upon Utilization of Oils and Manipulation of β-Oxidation in a High-Producing <b><i>Saccharopolyspora spinosa</i></b> Strain

Improvement of Spinosad Production upon Utilization of Oils and Manipulation of β-Oxidation in a High-Producing <b><i>Saccharopolyspora spinosa</i></b> Strain

Engineering microbial hosts for production of bacterial natural products

Bio-based production of fuels and industrial chemicals by repurposing antibiotic-producing type I modular polyketide synthases: opportunities and challenges

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