Spatial-resolved metabolome imaging of petals for Forsythia viridissima and Jasminum nudiflorum using online extraction (OLE) coupled to LC-Qtof-MS.

J Chromatogr B Analyt Technol Biomed Life Sci

Modern Research Center for Traditional Chinese Medicine, Beijing Research Institute of Chinese Medicine, Beijing University of Chinese Medicine, Beijing 102401, China. Electronic address:

Published: January 2025

AI Article Synopsis

  • MS imaging (MSI) is effective for studying metabolites in biological samples but struggles with isomer identification and matrix effects due to the lack of liquid chromatography separation.
  • A new platform, OLE-LC-Qtof-MS, combines online extraction and liquid chromatography with mass spectrometry to address these limitations, allowing for better differentiation of isomers and improved quantification of metabolites.
  • In a study using flowers of Forsythia viridissima and Jasminum nudiflorum, this method successfully identified a total of 87 metabolites, demonstrating distinct spatial distributions and the ability to differentiate specific isomers like chlorogenic acids within the petal structure.

Article Abstract

MS imaging (MSI) is a powerful technique for investigating the spatial distribution of metabolites in complex biological samples. However, due to the absence of liquid chromatography (LC) separation in routine MSI analysis, matrix effect is obvious and isomers identification remains challenging. To overcome these shortcomings of classical MSI tools (e.g., DESI-MSI and MALDI-MSI) for isomer differentiation and insufficient datapoints for quantification, online extraction-liquid chromatogram-hybrid triple quadrupole-time-of-flight mass spectrometry (OLE-LC-Qtof-MS) platform has been developed for spatial metabolome. As a proof-of-concept, two species flowers namely Forsythia viridissima (FV) and Jasminum nudiflorum (JN) that bloom in early spring were collected, dried, and cut into small pieces (1.0 mm × 1.0 mm). All pieces successively underwent OLE-LC-Qtof-MS measurements. As a result, 46 and 41 metabolites were observed and identified from FV and JN petals, respectively. Particularly, each compound corresponded to a chromatographic peak and isomeric differentiation was achieved amongst a set of chlorogenic acid derivatives. The peak areas of high intensity metabolites were aligned and combined within either species. The datasets were individually converted into heatmaps for all compounds, 87 ones in total, and each grid of any heatmap was assigned to the original location in the petal. Then, the spatial-resolved distribution style of each compound crossing the petal was reflected by the re-organized heatmap bearing the petal shape. As expected, regio-specific occurrence and accumulation were observed for several compounds, particularly among the chlorogenic acid isomers. Above all, OLE-LC-Qtof-MS is an alternative tool for spatial-resolved metabolome attributing to the advantages of isomeric separation and reliable quantification.

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http://dx.doi.org/10.1016/j.jchromb.2024.124385DOI Listing

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  • MS imaging (MSI) is effective for studying metabolites in biological samples but struggles with isomer identification and matrix effects due to the lack of liquid chromatography separation.
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