Targeting unique biological signals on the fly to improve MS/MS coverage and identification efficiency in metabolomics

Kevin Cho; Michaela Schwaiger-Haber; Fuad J Naser; Ethan Stancliffe; Miriam Sindelar; Gary J Patti

doi:10.1016/j.aca.2021.338210

Targeting unique biological signals on the fly to improve MS/MS coverage and identification efficiency in metabolomics

Anal Chim Acta. 2021 Mar 8:1149:338210. doi: 10.1016/j.aca.2021.338210. Epub 2021 Jan 12.

Authors

Kevin Cho¹, Michaela Schwaiger-Haber¹, Fuad J Naser¹, Ethan Stancliffe¹, Miriam Sindelar¹, Gary J Patti²

Affiliations

¹ Department of Chemistry, Washington University in St. Louis, St. Louis, MO, USA; Department of Medicine, Washington University in St. Louis, St. Louis, MO, USA.
² Department of Chemistry, Washington University in St. Louis, St. Louis, MO, USA; Department of Medicine, Washington University in St. Louis, St. Louis, MO, USA. Electronic address: gjpattij@wustl.edu.

Abstract

When using liquid chromatography/mass spectrometry (LC/MS) to perform untargeted metabolomics, it is common to detect thousands of features from a biological extract. Although it is impractical to collect non-chimeric MS/MS data for each in a single chromatographic run, this is generally unnecessary because most features do not correspond to unique metabolites of biological relevance. Here we show that relatively simple data-processing strategies that can be applied on the fly during acquisition of data with an Orbitrap ID-X, such as blank subtraction and well-established adduct or isotope calculations, decrease the number of features to target for MS/MS analysis by up to an order of magnitude for various types of biological matrices. We demonstrate that annotating these non-biological contaminants and redundancies in real time during data acquisition enables comprehensive MS/MS data to be acquired on each remaining feature at a single collision energy. To ensure that an appropriate collision energy is applied, we introduce a method using a series of hidden ion-trap scans in an Orbitrap ID-X to find an optimal value for each feature that can then be applied in a subsequent high-resolution Orbitrap scan. Data from 100 metabolite standards indicate that this real-time optimization of collision energies leads to more informative MS/MS patterns compared to using a single fixed collision energy alone. As a benchmark to evaluate the overall workflow, we manually annotated unique biological features by independently subjecting E. coli samples to a credentialing analysis. While credentialing led to a more rigorous reduction in feature number, on-the-fly annotation with blank subtraction on an Orbitrap ID-X did not inappropriately discard unique biological metabolites. Taken together, our results reveal that optimal fragmentation data can be obtained in a single LC/MS/MS run for >90% of the unique biological metabolites in a sample when features are annotated during acquisition and collision energies are selected by using parallel mass spectrometry detection.

Keywords: Credentialing; Liquid chromatography; Mass spectrometry; Metabolite identification; Untargeted metabolomics.

MeSH terms

Chromatography, Liquid
Escherichia coli*
Metabolomics
Tandem Mass Spectrometry*
Workflow

Abstract

MeSH terms

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