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基于独立氨酰化结构域对反应底物的不专一性对非核糖体肽合成系统进行的化学衍生化研究。

Chemical Diversification Based on Substrate Promiscuity of a Standalone Adenylation Domain in a Reconstituted NRPS System.

机构信息

State Key Laboratory of Agricultural Microbiology, College of Life Science and Technology , Huazhong Agricultural University , Wuhan 430070 , China.

CAS Key Laboratory of Tropical Marine Bio-resources and Ecology, RNAM Center for Marine Microbiology, Guangdong Key Laboratory of Marine Materia Medica , South China Sea Institute of Oceanology, Chinese Academy of Sciences , 164 West Xingang Road , Guangzhou 510301 , P. R. China.

出版信息

ACS Chem Biol. 2019 Feb 15;14(2):256-265. doi: 10.1021/acschembio.8b00938. Epub 2019 Feb 4.

DOI:10.1021/acschembio.8b00938
PMID:30673204
Abstract

A nonribosomal peptide synthetase (NRPS) assembly line ( sfa) in Streptomyces thioluteus that directs the formation of the diisonitrile chalkophore SF2768 (1) has been characterized by heterologous expression and directed gene knockouts. Herein, differential metabolic analysis of the heterologous expression strain and the original host led to the isolation of an SF2768 analogue (2, a byproduct of sfa) that possesses N-isovaleryl rather than 3-isocyanobutyryl side chains. The proposed biosynthetic logic of sfa and the structural difference between 1 and 2 suggested substrate promiscuity of the adenylate-forming enzyme SfaB. Further substrate scope investigation of SfaB and a successfully reconstituted NRPS system including a four-enzyme cascade enabled incorporation of diverse carboxylic acid building blocks into peptide scaffolds, and 30 unnatural products were thus generated. This structural diversification strategy based on substrate flexibility of the adenylation domain and in vitro reconstitution can be applied to other adenylation-priming pathways, thus providing a supplementary method for diversity-oriented total synthesis. Additionally, the biocatalytic process of the putative lysine δ-hydroxylase SfaE was validated through the derivatization of two key aldehyde intermediates (2a and 2b), thereby expanding the toolkit of enzymatic C-H bond activation.

摘要

链霉菌硫丝菌素中一种非核糖体肽合成酶 (NRPS) 装配线 (sfa) 负责形成二异腈 chalkophore SF2768(1),其通过异源表达和定向基因敲除进行了表征。在此,通过对异源表达菌株和原始宿主的差异代谢分析,分离到 SF2768 类似物 (2),它具有 N-异戊酰基而不是 3-异氰基丁酰基侧链,这是 sfa 的副产物。sfa 的提议生物合成逻辑和 1 与 2 的结构差异表明了腺苷酸形成酶 SfaB 的底物混杂性。进一步对 SfaB 和成功重建的 NRPS 系统(包括四酶级联)的底物范围进行研究,使各种羧酸构建块能够掺入肽支架中,从而生成了 30 种非天然产物。这种基于腺苷酸化结构域底物灵活性和体外重建的结构多样化策略可以应用于其他腺苷酸化引发途径,从而为多样性导向的全合成提供了一种补充方法。此外,通过对两个关键醛中间体 (2a 和 2b) 的衍生化,验证了假定赖氨酸 δ-羟化酶 SfaE 的生物催化过程,从而扩展了酶 C-H 键活化的工具包。

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