Improved batch correction in untargeted MS-based metabolomics

Ron Wehrens; Jos A Hageman; Fred van Eeuwijk; Rik Kooke; Pádraic J Flood; Erik Wijnker; Joost J B Keurentjes; Arjen Lommen; Henriëtte D L M van Eekelen; Robert D Hall; Roland Mumm; Ric C H de Vos

doi:10.1007/s11306-016-1015-8

Improved batch correction in untargeted MS-based metabolomics

Metabolomics. 2016:12:88. doi: 10.1007/s11306-016-1015-8. Epub 2016 Mar 18.

Authors

Affiliations

¹ Biometris, Wageningen UR, Wageningen, The Netherlands ; Bioscience, Wageningen UR, Wageningen, The Netherlands.
² Biometris, Wageningen UR, Wageningen, The Netherlands.
³ Laboratory of Genetics, Wageningen UR, Wageningen, The Netherlands ; Laboratory of Plant Physiology, Wageningen UR, Wageningen, The Netherlands.
⁴ Laboratory of Genetics, Wageningen UR, Wageningen, The Netherlands ; Horticulture and Production Physiology, Wageningen UR, Wageningen, The Netherlands ; Max Planck Institute For Plant Breeding Research, Cologne, Germany.
⁵ Laboratory of Genetics, Wageningen UR, Wageningen, The Netherlands ; Developmental Biology, Hamburg University, Hamburg, Germany.
⁶ Laboratory of Genetics, Wageningen UR, Wageningen, The Netherlands.
⁷ RIKILT, Wageningen UR, Wageningen, The Netherlands.
⁸ Bioscience, Wageningen UR, Wageningen, The Netherlands.
⁹ Bioscience, Wageningen UR, Wageningen, The Netherlands ; Laboratory of Plant Physiology, Wageningen UR, Wageningen, The Netherlands.

Abstract

Introduction: Batch effects in large untargeted metabolomics experiments are almost unavoidable, especially when sensitive detection techniques like mass spectrometry (MS) are employed. In order to obtain peak intensities that are comparable across all batches, corrections need to be performed. Since non-detects, i.e., signals with an intensity too low to be detected with certainty, are common in metabolomics studies, the batch correction methods need to take these into account.

Objectives: This paper aims to compare several batch correction methods, and investigates the effect of different strategies for handling non-detects.

Methods: Batch correction methods usually consist of regression models, possibly also accounting for trends within batches. To fit these models quality control samples (QCs), injected at regular intervals, can be used. Also study samples can be used, provided that the injection order is properly randomized. Normalization methods, not using information on batch labels or injection order, can correct for batch effects as well. Introducing two easy-to-use quality criteria, we assess the merits of these batch correction strategies using three large LC-MS and GC-MS data sets of samples from Arabidopsis thaliana.

Results: The three data sets have very different characteristics, leading to clearly distinct behaviour of the batch correction strategies studied. Explicit inclusion of information on batch and injection order in general leads to very good corrections; when enough QCs are available, also general normalization approaches perform well. Several approaches are shown to be able to handle non-detects-replacing them with very small numbers such as zero seems the worst of the approaches considered.

Conclusion: The use of quality control samples for batch correction leads to good results when enough QCs are available. If an experiment is properly set up, batch correction using the study samples usually leads to a similar high-quality correction, but has the advantage that more metabolites are corrected. The strategy for handling non-detects is important: choosing small values like zero can lead to suboptimal batch corrections.

Keywords: Arabidopsis thaliana; Batch correction; Mass spectrometry; Non-detects; Untargeted metabolomics.