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利用液相色谱-串联质谱法对吸水链霉菌中普拉地霉素类似物进行的表征和鉴定。

Characterization and identification of pradimicin analogs from Actinomadura hibisca using liquid chromatography-tandem mass spectrometry.

机构信息

Department of Pharmaceutical Engineering, Institute of Biomolecule Reconstruction, Sun Moon University, Chungnam, South Korea.

出版信息

J Chromatogr A. 2011 Apr 22;1218(16):2284-91. doi: 10.1016/j.chroma.2011.02.034. Epub 2011 Feb 19.

DOI:10.1016/j.chroma.2011.02.034
PMID:21376331
Abstract

Microbial cultures produce complex and potentially interesting mixtures of biosynthetic intermediates and derivatives of metabolites. These mixtures' reliable identification is important and so too is the development of techniques for their analysis. Here, a simple and highly selective method of detecting the biosynthetic congeners involved in the pentangular polyphenol pradimicin (PR) pathway from Actinomadura hibisca fermentation was developed. Solid-phase extraction (SPE) cleanup using an OASIS HLB cartridge was a simple and reliable tool for the extraction of PRs from a fermentation broth. The separation of each natural PR analog--eluted with a gradient system of aqueous acetonitrile through a reversed-phase C(18) column containing ammonium acetate and acetic acid as additives--allowed their simultaneous profiling. The combined use of SPE cleanup and chromatographic separation, coupled with electrospray ionization-tandem mass spectrometry (ESI-MS/MS) detection was demonstrated to be sufficiently accurate and reliable to analyze the natural PR analogs produced from A. hibisca. Ten natural PRs were identified: four alanine-containing (PRA, PRC, PRL, and PRB), two glycine-substituted (PRD and PRE), and four serine-substituted (PRFA-1, PRFA-2, PRFL, and PRFB). This report demonstrates the first use of both SPE cleanup and HPLC-ESI-MS/MS to profile a wide range of structurally closely related PRs in a bacterial fermentation broth.

摘要

微生物培养物会产生复杂且具有潜在有趣性的生物合成中间体和代谢物衍生物混合物。这些混合物的可靠鉴定非常重要,因此开发用于分析它们的技术也很重要。在这里,开发了一种从 Actinomadura hibisca 发酵中检测五角形多酚普拉迪霉素 (PR) 途径中涉及的生物合成同系物的简单且高度选择性方法。固相萃取 (SPE) 使用 OASIS HLB 小柱进行的净化是从发酵液中提取 PR 的简单可靠工具。通过在含有乙酸铵和乙酸作为添加剂的反相 C(18)柱上用含水乙腈梯度洗脱,可以分离出每个天然 PR 类似物,从而可以同时对其进行分析。事实证明,结合使用 SPE 净化和色谱分离,并结合电喷雾电离串联质谱 (ESI-MS/MS) 检测,足以准确可靠地分析从 A. hibisca 产生的天然 PR 类似物。鉴定了十种天然 PR:四种含有丙氨酸(PR A、PR C、PR L 和 PR B),两种甘氨酸取代(PR D 和 PR E)和四种丝氨酸取代(PR FA-1、PR FA-2、PR FL 和 PR FB)。本报告首次展示了同时使用 SPE 净化和 HPLC-ESI-MS/MS 来分析细菌发酵液中广泛存在的结构上密切相关的 PR 混合物。

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