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An UPLC-ESI-MS/MS Assay Using 6-Aminoquinolyl-N-Hydroxysuccinimidyl Carbamate Derivatization for Targeted Amino Acid Analysis: Application to Screening of Arabidopsis thaliana Mutants

机译:使用6-氨基喹啉基-N-羟基琥珀酰亚胺氨基甲酸酯衍生化的UPLC-ESI-MS / MS分析,用于目标氨基酸分析:在拟南芥突变体筛选中的应用

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In spite of the large arsenal of methodologies developed for amino acid assessment in complex matrices, their implementation in metabolomics studies involving wide-ranging mutant screening is hampered by their lack of high-throughput, sensitivity, reproducibility, and/or wide dynamic range. In response to the challenge of developing amino acid analysis methods that satisfy the criteria required for metabolomic studies, improved reverse-phase high-performance liquid chromatography-mass spectrometry (RPHPLC-MS) methods have been recently reported for large-scale screening of metabolic phenotypes. However, these methods focus on the direct analysis of underivatized amino acids and, therefore, problems associated with insufficient retention and resolution are observed due to the hydrophilic nature of amino acids. It is well known that derivatization methods render amino acids more amenable for reverse phase chromatographic analysis by introducing highly-hydrophobic tags in their carboxylic acid or amino functional group. Therefore, an analytical platform that combines the 6-aminoquinolyl-N-hydroxysuccinimidyl carbamate (AQC) pre-column derivatization method with ultra performance liquid chromatography-electrospray ionization-tandem mass spectrometry (UPLC-ESI-MS/MS) is presented in this article. For numerous reasons typical amino acid derivatization methods would be inadequate for large scale metabolic projects. However, AQC derivatization is a simple, rapid and reproducible way of obtaining stable amino acid adducts amenable for UPLC-ESI-MS/MS and the applicability of the method for high-throughput metabolomic analysis in Arabidopsis thaliana is demonstrated in this study. Overall, the major advantages offered by this amino acid analysis method include high-throughput, enhanced sensitivity and selectivity; characteristics that showcase its utility for the rapid screening of the preselected plant metabolites without compromising the quality of the metabolic data. The presented method enabled thirty-eight metabolites (proteinogenic amino acids and related compounds) to be analyzed within 10 min with detection limits down to 1.02 × 10−11 M (i.e., atomole level on column), which represents an improved sensitivity of 1 to 5 orders of magnitude compared to existing methods. Our UPLC-ESI-MS/MS method is one of the seven analytical platforms used by the Arabidopsis Metabolomics Consortium. The amino acid dataset obtained by analysis of Arabidopsis T-DNA mutant stocks with our platform is captured and open to the public in the web portal PlantMetabolomics.org. The analytical platform herein described could find important applications in other studies where the rapid, high-throughput and sensitive assessment of low abundance amino acids in complex biosamples is necessary.
机译:尽管开发了大量用于复杂基质中氨基酸评估的方法学,但由于它们缺乏高通量,灵敏度,可重复性和/或宽动态范围,因此难以在涉及广泛突变体筛选的代谢组学研究中实施。为响应开发满足代谢组学研究要求的标准的氨基酸分析方法的挑战,最近已报道了用于代谢表型的大规模筛选的改良型反相高效液相色谱-质谱(RPHPLC-MS)方法。但是,这些方法着重于未衍生氨基酸的直接分析,因此,由于氨基酸的亲水性,观察到与保留和分离度不足有关的问题。众所周知,衍生化方法是通过在其羧酸或氨基官能团中引入高度疏水性的标记,使氨基酸更适合于反相色谱分析。因此,本文提出了一种结合6-氨基喹啉基-N-羟基琥珀酰亚胺氨基甲酸酯(AQC)预柱衍生化方法与超高效液相色谱-电喷雾电离串联质谱(UPLC-ESI-MS / MS)的分析平台。由于许多原因,典型的氨基酸衍生化方法不足以用于大规模的代谢项目。但是,AQC衍生化是获得适合UPLC-ESI-MS / MS的稳定氨基酸加合物的简单,快速且可重现的方法,本研究证明了该方法在拟南芥中进行高通量代谢组学分析的适用性。总体而言,这种氨基酸分析方法的主要优点包括高通量,增强的灵敏度和选择性;以及这些特性展示了其可用于快速筛选预选植物代谢物的功能,而不会影响代谢数据的质量。所提出的方法能够在10分钟内分析38种代谢产物(蛋白原性氨基酸和相关化合物),检出限低至1.02×10 −11 M(即色谱柱上的原子水平)。代表与现有方法相比灵敏度提高了1-5个数量级。我们的UPLC-ESI-MS / MS方法是拟南芥代谢组学联盟使用的七个分析平台之一。通过使用我们的平台分析拟南芥属T-DNA突变体种群获得的氨基酸数据集已被捕获,并在门户网站PlantMetabolomics.org中向公众开放。本文所述的分析平台可在其他研究中找到重要的应用,在这些研究中,需要对复杂生物样品中的低丰度氨基酸进行快速,高通量和灵敏的评估。

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