Metabolomic Coverage of Chemical-Group-Submetabolome Analysis: Group Classification and Four-Channel Chemical Isotope Labeling LC-MS

化学 代谢组 代谢组学 质谱法 群(周期表) 衍生化 功能群 色谱法 化学电离 有机化学 离子 电离 聚合物
作者
Shuang Zhao,Hao Li,Wei Han,Wan Chan,Liang Li
出处
期刊:Analytical Chemistry [American Chemical Society]
卷期号:91 (18): 12108-12115 被引量:102
标识
DOI:10.1021/acs.analchem.9b03431
摘要

Chemical isotope labeling (CIL) liquid chromatography mass spectrometry (LC-MS) is a powerful technique for in-depth metabolome analysis with high quantification accuracy. Unlike conventional LC-MS, it analyzes chemical-group-based submetabolomes and uses the combined results to represent the whole metabolome. Due to analysis time and cost constraint, not all submetabolomes can be profiled and thus knowledge of chemical group classification is important in guiding submetabolome selection. Herein we report a study of determining the distribution of functional groups of compounds in a database and then examine how well we can experimentally analyze the major chemical groups in two representative samples (i.e., human plasma and yeast). We developed a computer algorithm to classify chemical structures according to their functional groups. After removing lipids which are targeted molecules in lipidomic analysis, inorganic species and other molecules that are unique to drug, food, plant, and environmental origins, five groups (i.e., amine, phenol, hydroxyl, carboxyl, and carbonyl) are found to be the dominant classes. In the databases of MCID (2683 filtered metabolites), HMDB (5506), KEGG (11598), YMDB (1107), and ECMDB (1462), 94.7%, 85.7%, 86.4%, 85.7%, and 95.8% of the filtered metabolites belong to one or more of the five groups, respectively. These groups can be analyzed in four-channel CIL LC-MS where hydroxyls (H), amines and phenols (A), carboxyls (C), and carbonyls or ketones/aldehydes (K) are separately profiled as individual channels using dansyl and DmPA labeling reagents. A total of 7431 peak pairs were detected with 6109 unique-mass pairs from plasma, while 5629 pairs with 4955 unique-mass pairs were detected in yeast. Compared to group distributions of database compounds, hydroxyl-containing metabolites were severely underdetected, which might indicate that the current method is less than optimal for analyzing this group of metabolites. As a result, the overall experimental coverage is likely significantly lower than the database-derived coverage. In short, this study has shown that high metabolome coverage is theoretically attainable by analyzing only the H, A, C, and K submetabolomes and the group classification information should be helpful in guiding future analytical method development and choices of submetabolomes to be analyzed.
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