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通过串联质谱和同位素标记对天然大肠杆菌素-核碱基加合物进行表征。支持环丙烷开环导致的DNA烷基化。

Characterization of Natural Colibactin-Nucleobase Adducts by Tandem Mass Spectrometry and Isotopic Labeling. Support for DNA Alkylation by Cyclopropane Ring Opening.

作者信息

Xue Mengzhao, Shine Emilee, Wang Weiwei, Crawford Jason M, Herzon Seth B

机构信息

Department of Chemistry , Yale University , New Haven , Connecticut 06520 , United States.

Chemical Biology Institute , Yale University , West Haven , Connecticut 06516 , United States.

出版信息

Biochemistry. 2018 Nov 13;57(45):6391-6394. doi: 10.1021/acs.biochem.8b01023. Epub 2018 Oct 31.

Abstract

Colibactins are genotoxic secondary metabolites whose biosynthesis is encoded in the clb gene cluster harbored by certain strains of gut commensal Escherichia coli. Using synthetic colibactin analogues, we previously provided evidence that colibactins alkylate DNA by addition of a nucleotide to an electrophilic cyclopropane intermediate. However, natural colibactin-nucleobase adducts have not been identified, to the best of our knowledge. Here we present the first identification of such adducts, derived from treatment of pUC19 DNA with clb E. coli. Previous biosynthetic studies established cysteine and methionine as building blocks in colibactin biosynthesis; accordingly, we used cysteine (Δ cysE) and methionine (Δ metA) auxotrophic strains cultured in media supplemented with l-[U-C]Cys or l-[U-C]Met to facilitate the identification of nucleobases bound to colibactins. Using MS and MS analysis, in conjunction with the known oxidative instability of colibactin cyclopropane-opened products, we were able to characterize adenine adducts derived from cyclopropane ring opening. This study provides the first reported detection of nucleobase adducts derived from clb E. coli and lends support to our earlier model suggesting DNA alkylation by addition of a nucleotide to an electrophilic cyclopropane.

摘要

大肠杆菌素是具有基因毒性的次级代谢产物,其生物合成由某些肠道共生大肠杆菌菌株所携带的clb基因簇编码。我们之前使用合成的大肠杆菌素类似物证明,大肠杆菌素通过将一个核苷酸添加到亲电环丙烷中间体上使DNA烷基化。然而,据我们所知,尚未鉴定出天然的大肠杆菌素-核碱基加合物。在此,我们首次鉴定了此类加合物,其源自用携带clb的大肠杆菌处理pUC19 DNA。先前的生物合成研究确定半胱氨酸和甲硫氨酸是大肠杆菌素生物合成的组成部分;因此,我们使用在补充有l-[U-C]半胱氨酸或l-[U-C]甲硫氨酸的培养基中培养的半胱氨酸(ΔcysE)和甲硫氨酸(ΔmetA)营养缺陷型菌株,以促进对与大肠杆菌素结合的核碱基的鉴定。结合已知的大肠杆菌素环丙烷开环产物的氧化不稳定性,通过质谱和质谱分析,我们能够表征源自环丙烷环开环的腺嘌呤加合物。本研究首次报道了对源自携带clb的大肠杆菌的核碱基加合物的检测,并支持了我们早期提出的通过将一个核苷酸添加到亲电环丙烷使DNA烷基化的模型。

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本文引用的文献

1
Colibactin: More Than a New Bacterial Toxin.肠细胞毒素:不止一种新型细菌毒素。
Toxins (Basel). 2018 Apr 10;10(4):151. doi: 10.3390/toxins10040151.
3
ClbS Is a Cyclopropane Hydrolase That Confers Colibactin Resistance.ClbS 是一种环丙烷水解酶,可赋予大肠杆菌素抗性。
J Am Chem Soc. 2017 Dec 13;139(49):17719-17722. doi: 10.1021/jacs.7b09971. Epub 2017 Nov 28.
7
A Mechanistic Model for Colibactin-Induced Genotoxicity.一种 colibactin 诱导遗传毒性的机制模型。
J Am Chem Soc. 2016 Dec 7;138(48):15563-15570. doi: 10.1021/jacs.6b10354. Epub 2016 Nov 28.
10
Escherichia coli ClbS is a colibactin resistance protein.大肠杆菌ClbS是一种大肠杆菌素抗性蛋白。
Mol Microbiol. 2016 Mar;99(5):897-908. doi: 10.1111/mmi.13272. Epub 2015 Dec 1.

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