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一种改良的培养佐久间链霉菌的方法:阿齐霉素B烯醇片段的生物合成起源

An improved method for culturing Streptomyces sahachiroi: biosynthetic origin of the enol fragment of azinomycin B.

作者信息

Kelly Gilbert T, Sharma Vasudha, Watanabe Coran M H

机构信息

Department of Chemistry, Texas A&M University, P.O. Box 30012, College Station, TX 77843, USA.

出版信息

Bioorg Chem. 2008 Feb;36(1):4-15. doi: 10.1016/j.bioorg.2007.08.002. Epub 2007 Sep 27.

Abstract

Azinomycin B is an environmental DNA crosslinking agent produced by the soil microorganism Streptomyces sahachiroi. While the agent displays potent cytotoxic activities against leukemic cell lines and animal mouse models, the lack of a consistent supply of the natural product has hampered detailed biological investigations on the compound, including its mode of action and biosynthesis. We report here a significant methodological improvement in the culturing of the bacterium, which allows reliable and steady production of the natural product in good yields. The key experimental step involves the culturing of the strain on dehydrated plates, followed by the generation of a two-stage starter culture and subsequent fermentation of the strain under nutrient-starved conditions. We illustrate use of this culture system by investigating the formation of the enol fragment of the molecule in isotopic labeling experiments with threonine and several advanced precursors (beta-ketoamino acid 3, beta-hydroxyamino aldehyde 4, and beta-ketoaminoaldehyde 5). The results unequivocally show that threonine is the most advanced precursor accepted by the NRPS (non-ribosomal peptidyl synthetase) machinery for final processing and construction of the enol moiety of the natural product.

摘要

阿齐霉素B是一种由土壤微生物佐久间链霉菌产生的环境DNA交联剂。虽然该试剂对白血病细胞系和动物小鼠模型显示出强大的细胞毒性活性,但天然产物缺乏稳定供应阻碍了对该化合物的详细生物学研究,包括其作用方式和生物合成。我们在此报告了该细菌培养方法的重大改进,这使得天然产物能够以良好的产量可靠且稳定地生产。关键实验步骤包括在脱水平板上培养菌株,随后生成两阶段起始培养物,并在营养饥饿条件下对菌株进行后续发酵。我们通过在苏氨酸和几种高级前体(β-酮氨基酸3、β-羟基氨基醛4和β-酮氨基醛5)的同位素标记实验中研究分子烯醇片段的形成来说明该培养系统的用途。结果明确表明,苏氨酸是NRPS(非核糖体肽基合成酶)机制接受的用于最终加工和构建天然产物烯醇部分的最先进前体。

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