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Optimized sampling protocol for mass spectrometry-based metabolomics in Streptomyces

机译:用于链霉菌基于质谱的基于质谱的代谢组织的优化抽样方案

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摘要

Abstract In quantitative metabolomics studies, the most crucial step was arresting snapshots of all interesting metabolites. However, the procedure customized for Streptomyces was so rare that most studies consulted the procedure from other bacteria even yeast, leading to inaccurate and unreliable metabolomics analysis. In this study, a base solution (acetone: ethanol = 1:1, mol/mol) was added to a quenching solution to keep the integrity of the cell membrane. Based on the molar transition energy (E T) of the organic solvents, five solutions were used to carry out the quenching procedures. These were acetone, isoamylol, propanol, methanol, and 60% (v/v) methanol. To the best of our knowledge, this is the first report which has utilized a quenching solution with ET values. Three procedures were also adopted for extraction. These were boiling, freezing–thawing, and grinding ethanol. Following the analysis of the mass balance, amino acids, organic acids, phosphate sugars, and sugar alcohols were measured using gas chromatography with an isotope dilution mass spectrometry. It was found that using isoamylol with a base solution (5:1, v/v) as a quenching solution and that freezing–thawing in liquid nitrogen within 50% (v/v) methanol as an extracting procedure were the best pairing for the quantitative metabolomics of Streptomyces ZYJ-6, and resulted in average recoveries of close to 100%. The concentration of intracellular metabolites obtained from this new quenching solution was between two and ten times higher than that from 60% (v/v) methanol, which until now has been the most commonly used solution. Our findings are the first systematic quantitative metabolomics tools for Streptomyces ZYJ-6 and, therefore, will be important references for research in fields such as 13C based metabolic flux analysis, multi-omic research and genome-scale metabolic model establishment, as well as for other Streptomyces.
机译:摘要在定量代谢组学研究中,最关键的步骤是逮捕所有有趣的代谢物的快照。然而,为链霉菌定制的程序是如此罕见的是大多数研究甚至酵母甚至酵母的程序咨询了该程序,导致不准确和不可靠的代谢组科分析。在该研究中,将碱溶液(丙酮:乙醇= 1:1,mol / mol)加入到淬火溶液中以保持细胞膜的完整性。基于有机溶剂的摩尔过渡能量(E T),使用五种溶液进行猝灭程序。这些是丙酮,异戊酰胺,丙醇,甲醇和60%(v / v)甲醇。据我们所知,这是第一个已利用具有ET值的淬火解决方案的报告。还采用了三个程序进行提取。这些是沸腾,冷冻解冻和研磨乙醇。在分析质量平衡,使用气相色谱法测量氨基酸,有机酸,磷酸糖和糖醇,用同位素稀释质谱法测量。发现使用具有碱溶液(5:1,v / v)的异氰基醇作为淬火溶液,并且在50%(v / v)甲醇中的液氮中的冷冻解冻作为提取程序是最佳配对链霉菌ZYJ-6的定量代谢学,导致平均回收率接近100%。从这种新的淬火溶液获得的细胞内代谢物的浓度比从60%(v / v)甲醇高的2至10倍之间,直到现在现在是最常用的溶液。我们的研究结果是Streptomyces Zyj-6的第一种系统定量代谢工具,因此将是在基于13C的代谢通量分析,多OMIC研究和基因组代谢模型建立等领域研究的重要引用,以及其他链霉菌。

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