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利用宿主代谢在……中生产双去甲氧基姜黄素

Leveraging host metabolism for bisdemethoxycurcumin production in .

作者信息

Incha Matthew R, Thompson Mitchell G, Blake-Hedges Jacquelyn M, Liu Yuzhong, Pearson Allison N, Schmidt Matthias, Gin Jennifer W, Petzold Christopher J, Deutschbauer Adam M, Keasling Jay D

机构信息

Joint BioEnergy Institute, 5885 Hollis Street, Emeryville, CA, 94608, USA.

Biological Systems & Engineering Division, Lawrence Berkeley National Laboratory, Berkeley, CA, 94720, USA.

出版信息

Metab Eng Commun. 2019 Dec 17;10:e00119. doi: 10.1016/j.mec.2019.e00119. eCollection 2020 Jun.

Abstract

is a saprophytic bacterium with robust metabolisms and strong solvent tolerance making it an attractive host for metabolic engineering and bioremediation. Due to its diverse carbon metabolisms, its genome encodes an array of proteins and enzymes that can be readily applied to produce valuable products. In this work we sought to identify design principles and bottlenecks in the production of type III polyketide synthase (T3PKS)-derived compounds in . T3PKS products are widely used as nutraceuticals and medicines and often require aromatic starter units, such as coumaroyl-CoA, which is also an intermediate in the native coumarate catabolic pathway of . Using a randomly barcoded transposon mutant (RB-TnSeq) library, we assayed gene functions for a large portion of aromatic catabolism, confirmed known pathways, and proposed new annotations for two aromatic transporters. The 1,3,6,8-tetrahydroxynapthalene synthase of (RppA), a microbial T3PKS, was then used to rapidly assay growth conditions for increased T3PKS product accumulation. The feruloyl/coumaroyl CoA synthetase (Fcs) of was used to supply coumaroyl-CoA for the curcuminoid synthase (CUS) of , a plant T3PKS. We identified that accumulation of coumaroyl-CoA in this pathway results in extended growth lag times in . Deletion of the second step in coumarate catabolism, the enoyl-CoA hydratase-lyase (Ech), resulted in increased production of the type III polyketide bisdemethoxycurcumin.

摘要

是一种具有强大代谢能力和较强溶剂耐受性的腐生细菌,使其成为代谢工程和生物修复的有吸引力的宿主。由于其多样的碳代谢,其基因组编码了一系列蛋白质和酶,可很容易地用于生产有价值的产品。在这项工作中,我们试图确定在中生产III型聚酮合酶(T3PKS)衍生化合物的设计原则和瓶颈。T3PKS产品被广泛用作营养保健品和药物,通常需要芳香起始单元,如香豆酰辅酶A,它也是中天然香豆酸盐分解代谢途径的中间体。使用随机条形码转座子突变体(RB-TnSeq)文库,我们分析了大部分芳香族分解代谢的基因功能,确认了已知途径,并为两种芳香族转运蛋白提出了新的注释。然后使用微生物T3PKS(RppA)的1,3,6,8-四羟基萘合酶快速分析生长条件,以增加T3PKS产物的积累。的阿魏酰/香豆酰辅酶A合成酶(Fcs)用于为植物T3PKS的姜黄素合酶(CUS)提供香豆酰辅酶A。我们发现该途径中香豆酰辅酶A的积累导致生长延迟时间延长。删除香豆酸盐分解代谢的第二步,即烯酰辅酶A水合酶裂解酶(Ech),导致III型聚酮化合物双去甲氧基姜黄素的产量增加。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8a82/7136493/029c41f77b0d/gr1.jpg

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