首页> 外文期刊>Journal of proteome research >Tackling the Peak Overlap Issue in NMR Metabolomics Studies: 1D Projected Correlation Traces from Statistical Correlation Analysis on Nontilted 2D H-1 NMR J-Resolved Spectra
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Tackling the Peak Overlap Issue in NMR Metabolomics Studies: 1D Projected Correlation Traces from Statistical Correlation Analysis on Nontilted 2D H-1 NMR J-Resolved Spectra

机译:在NMR代谢组学研究中解决峰值重叠问题:1D投影相关痕量从统计相关性分析对Nontivered 2D H-1 NMR J-Solated Spectra

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摘要

The identification of metabolites in complex biological matrices is a challenging task in 1D H-1-NMR-based metabolomics studies. Statistical total correlation spectroscopy (STOCSY) has emerged for aiding the structural elucidation by revealing the peaks that present a high correlation to a driver peak of interest (which would likely belong to the same molecule). However, in these studies, the signals from metabolites are normally present as a mixture of overlapping resonances, limiting the performance of STOCSY. As an alternative to avoid the overlap issue, 2D H-1 homonuclear J-resolved (JRES) spectra were projected, in their usual tilted and symmetrized processed form, and STOCSY was applied on these ID projections (p-JRES-STOCSY). Nonetheless, this approach suffers in cases where the signals are very close. In addition, STOCSY was applied to the whole JRES spectra (also tilted) to identify correlated multiplets, although the overlap issue in itself was not addressed directly and the subsequent search in databases is complicated in cases of higher order coupling. With these limitations in mind, in the present work, we propose a new methodology based on the application of STOCSY on a set of nontilted JRES spectra, detecting peaks that would overlap in 1D spectra of the same sample set. Correlation comparison analysis for peak overlap detection (COCOA-POD) is able to reconstruct projected 1D STOCSY traces that result in more suitable database queries, as all peaks are summed at their f2 resonances instead of the resonance corresponding to the multiplet center in the tilted JRES spectra. (The peak dispersion and resolution enhancement gained are not sacrificed by the projection.) Besides improving database queries with better peak lists obtained from the projections of the 2D STOCSY analysis, the overlap region is examined, and the multiplet itself is analyzed from the correlation trace at 45 degrees to obtain a cleaner multiplet profile, free from contributions from
机译:复杂生物学基质中代谢物的鉴定是基于1DH-1-NMR的代谢组研究中的一个具有挑战性的任务。统计总相关光谱(Stocsy)揭示了通过揭示与驾驶员的驾驶员峰值(可能属于同一分子)的高相关性的峰值来实现结构阐明。然而,在这些研究中,来自代谢物的信号通常作为重叠共振的混合物存在,限制了Stocsy的性能。作为替代避免重叠问题的替代方案,将2D H-1同时核J-DEARTAVEVED(JRES)光谱以通常的倾斜和对称的加工形式投射,并且在这些ID投影(P-JRES-STOCSY)上应用Stocsy。尽管如此,这种方法在信号非常接近的情况下遭受。此外,STOCSY应用于整个JRES光谱(也倾斜)以识别相关的多重,尽管本身的重叠问题未直接解决,并且在高阶耦合的情况下,数据库中的后续搜索复杂。在目前的工作中,通过这些局限性,我们提出了一种基于STOCSY在一组Nontivered的JRES光谱上应用的新方法,检测在相同样本集的1D光谱中重叠的峰值。峰值重叠检测的相关比较分析(Cocoa-Pod)能够重建导致更合适的数据库查询的投影1D Stocsy迹线,因为所有峰值都在其F2谐振中求和而不是倾斜的JRE中的多功能中心对应的谐振光谱。 (通过投影不牺牲所获得的峰分散和分辨率增强。)除了从2D Stocsy分析的投影获得的更好的峰列表改进数据库查询之外,检查重叠区域,并且从相关迹线分析了多功能本身45度以获得清洁的多重配置文件,免于来自贡献

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