4.7 Article

Metabolic profiles of human brain parenchyma and glioma for rapid tissue diagnosis by targeted desorption electrospray ionization mass spectrometry

Journal

ANALYTICAL AND BIOANALYTICAL CHEMISTRY
Volume 413, Issue 25, Pages 6213-6224

Publisher

SPRINGER HEIDELBERG
DOI: 10.1007/s00216-021-03593-0

Keywords

Metabolomics; Biomarker; Glioma; Ambient ionization; Multiple reaction monitoring; Tandem mass spectrometry

Funding

  1. National Cancer Institute [IR33CA240181-01A1]
  2. Waters Inc. [40002775]

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DESI-MS is a suitable method for intraoperative tissue analysis due to its minimal sample preparation and quick molecular diagnostics. Combining multiple metabolites, such as GABA, creatine, carnitine, and hexol, with the established biomarker NAA, allows for improved accuracy in distinguishing brain parenchyma from glioma. The implementation of diagnostic ion abundance ratios based on these metabolites can enhance method robustness and strengthen discriminatory power, leading to an improved DESI-MS method for glioma diagnosis.
Desorption electrospray ionization mass spectrometry (DESI-MS) is well suited for intraoperative tissue analysis since it requires little sample preparation and offers rapid and sensitive molecular diagnostics. Currently, intraoperative assessment of the tumor cell percentage of glioma biopsies can be made by measuring a single metabolite, N-acetylaspartate (NAA). The inclusion of additional biomarkers will likely improve the accuracy when distinguishing brain parenchyma from glioma by DESI-MS. To explore this possibility, mass spectra were recorded for extracts from 32 unmodified human brain samples with known pathology. Statistical analysis of data obtained from full-scan and multiple reaction monitoring (MRM) profiles identified discriminatory metabolites, namely gamma-aminobutyric acid (GABA), creatine, glutamic acid, carnitine, and hexane-1,2,3,4,5,6-hexol (abbreviated as hexol), as well as the established biomarker NAA. Brain parenchyma was readily differentiated from glioma based on these metabolites as measured both in full-scan mass spectra and by the intensities of their characteristic MRM transitions. New DESI-MS methods (5 min acquisition using full scans and MS/MS), developed to measure ion abundance ratios among these metabolites, were tested using smears of 29 brain samples. Ion abundance ratios based on signals for GABA, creatine, carnitine, and hexol all had sensitivities > 90%, specificities > 80%, and accuracies > 85%. Prospectively, the implementation of diagnostic ion abundance ratios should strengthen the discriminatory power of individual biomarkers and enhance method robustness against signal fluctuations, resulting in an improved DESI-MS method of glioma diagnosis.

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