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msPurity: Automated Evaluation of Precursor Ion Purity for Mass Spectrometry-Based Fragmentation in Metabolomics

机译:MSPURITY:对代谢物中的质谱基碎片的前体离子纯度的自动评价

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摘要

Tandem mass spectrometry (MS/MS or MS2) is a widely used approach for structural annotation and identification of metabolites in complex biological samples. The importance of assessing the contribution of the precursor ion within an isolation window for MS2 experiments has been previously detailed in proteomics, where precursor ion purity influences the quality and accuracy of matching to mass spectral libraries, but to date, there has been little attention to this data-processing technique in metabolomics. Here, we present msPurity, a vendor-independent R package for liquid chromatography (LC) and direct infusion (DI) MS2 that calculates a simple metric to describe the contribution of the selected precursor. The precursor purity metric is calculated as "intensity of a selected precursor divided by the summed intensity of the isolation window". The metric is interpolated at the recorded point of MS2 acquisition using bordering full-scan spectra. Isotopic peaks of the selected precursor can be removed, and low abundance peaks that are believed to have limited contribution to the resulting MS2 spectra are removed. Additionally, the isolation efficiency of the mass spectrometer can be taken into account. The package was applied to Data Dependent Acquisition (DDA)-based MS2 metabolomics data sets derived from three metabolomics data repositories. For the 10 LC-MS2 DDA data sets with > +/- 1 Da isolation windows, the median precursor purity score ranged from 0.67 to 0.96 (scale = 0 to +1). The R package was also used to assess precursor purity of theoretical isolation windows from LC MS data sets of differing sample types. The theoretical isolation windows being the same width used for an anticipated DDA experiment ( +/- 0.5 Da). The most complex sample had a median precursor purity score of 0.46 for the 64,498 XCMS determined features, in comparison to the less spectrally complex sample that had a purity score of 0.66 for 5071 XCMS features. It has been previously reported in proteomics that a purity score of <0.5 can produce unreliable spectra matching results. With this assumption, we show that for complex samples there will be a large number of metabolites where traditional DDA approaches will struggle to provide reliable annotations or accurate matches to mass spectral libraries.
机译:串联质谱(MS / MS或MS2)是广泛使用的综合生物样品中代谢物的结构注释和鉴定方法。在蛋白质组学中,在蛋白质组学中详述了评估前体离子在隔离窗口内的贡献的重要性,其中前体离子纯度会影响与质谱库匹配的质量和准确性,但到目前为止,还有很少关注这种数据处理技术在代谢组科中。在这里,我们呈现MSPUSTURY,用于液相色谱(LC)的供应商独立的R包装和直接输注(DI)MS2,用于描述所选前体的贡献。前体纯度度量计算为“所选前体的强度除以隔离窗口的总和”。使用接壤的全扫描光谱,在MS2采集的记录点处插入度量。可以去除所选前体的同位素峰,除去据信对所得MS2光谱有限贡献的低丰度峰。另外,可以考虑质谱仪的隔离效率。将包应用于数据依赖的采集(DDA) - 基于三个代谢组数据存储库的MS2代谢组数据集。对于具有> +/- 1DA隔离窗口的10 LC-MS2 DDA数据集,中位前体纯度分数范围为0.67至0.96(Scale = 0至+1)。 R包装还用于评估来自不同样品类型的LC MS数据集的理论隔离窗口的前体纯度。理论隔离窗口与预期的DDA实验相同的宽度(+/- 0.5Da)。对于64,498 XCMS测定的特征,最复杂的样品具有0.46的中值前体纯度得分为0.46,与纯度分数为0.66的纯度得分为5071 XCMS特征。以前在蛋白质组学中报道的是<0.5的纯度得分可以产生不可靠的光谱匹配结果。借此假设,我们表明,对于复杂的样本,将有大量代谢物,其中传统的DDA方法将努力提供可靠的注释或准确匹配质量谱库。

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  • 来源
    《Analytical chemistry》 |2017年第4期|共8页
  • 作者单位

    Univ Birmingham Sch Biosci Coll Life &

    Environm Sci Birmingham B15 2TT W Midlands England;

    Univ Birmingham Sch Biosci Coll Life &

    Environm Sci Birmingham B15 2TT W Midlands England;

    Univ Birmingham Sch Biosci Coll Life &

    Environm Sci Birmingham B15 2TT W Midlands England;

    Univ Birmingham Sch Biosci Coll Life &

    Environm Sci Birmingham B15 2TT W Midlands England;

    Univ Birmingham Sch Biosci Coll Life &

    Environm Sci Birmingham B15 2TT W Midlands England;

    Univ Birmingham Sch Biosci Coll Life &

    Environm Sci Birmingham B15 2TT W Midlands England;

    Univ Birmingham Sch Biosci Coll Life &

    Environm Sci Birmingham B15 2TT W Midlands England;

    Univ Birmingham Sch Biosci Coll Life &

    Environm Sci Birmingham B15 2TT W Midlands England;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 分析化学;
  • 关键词

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