Dominant components of the Thoroughbred metabolome characterised by (1) H-nuclear magnetic resonance spectroscopy: A metabolite atlas of common biofluids

E E Escalona; J Leng; A C Dona; C A Merrifield; E Holmes; C J Proudman; J R Swann

doi:10.1111/evj.12333

Dominant components of the Thoroughbred metabolome characterised by (1) H-nuclear magnetic resonance spectroscopy: A metabolite atlas of common biofluids

Equine Vet J. 2015 Nov;47(6):721-30. doi: 10.1111/evj.12333. Epub 2015 Jan 28.

Authors

E E Escalona¹, J Leng², A C Dona¹, C A Merrifield¹, E Holmes¹, C J Proudman³, J R Swann²

Affiliations

¹ Section of Biomolecular Medicine, Division of Computational and Systems Medicine, Faculty of Medicine, Imperial College London, UK.
² Department of Food and Nutritional Sciences, University of Reading, Berkshire, UK.
³ Department of Gastroenterology, School of Veterinary Medicine, University of Liverpool, Neston, UK.

PMID: 25130591
DOI: 10.1111/evj.12333

Abstract

Reasons for performing study: Metabonomics is emerging as a powerful tool for disease screening and investigating mammalian metabolism. This study aims to create a metabolic framework by producing a preliminary reference guide for the normal equine metabolic milieu.

Objectives: To metabolically profile plasma, urine and faecal water from healthy racehorses using high resolution (1) H-nuclear magnetic resonance (NMR) spectroscopy and to provide a list of dominant metabolites present in each biofluid for the benefit of future research in this area.

Study design: This study was performed using 7 Thoroughbreds in race training at a single time point. Urine and faecal samples were collected noninvasively and plasma was obtained from samples taken for routine clinical chemistry purposes.

Methods: Biofluids were analysed using (1) H-NMR spectroscopy. Metabolite assignment was achieved via a range of one- and 2-dimensional experiments.

Results: A total of 102 metabolites were assigned across the 3 biological matrices. A core metabonome of 14 metabolites was ubiquitous across all biofluids. All biological matrices provided a unique window on different aspects of systematic metabolism. Urine was the most populated metabolite matrix with 65 identified metabolites, 39 of which were unique to this biological compartment. A number of these were related to gut microbial host cometabolism. Faecal samples were the most metabolically variable between animals; acetate was responsible for the majority (28%) of this variation. Short-chain fatty acids were the predominant features identified within this biofluid by (1) H-NMR spectroscopy.

Conclusions: Metabonomics provides a platform for investigating complex and dynamic interactions between the host and its consortium of gut microbes and has the potential to uncover markers for health and disease in a variety of biofluids. Inherent variation in faecal extracts along with the relative abundance of microbial-mammalian metabolites in urine and invasive nature of plasma sampling, infers that urine is the most appropriate biofluid for the purposes of metabonomic analysis.

Keywords: biofluids; horse; metabolites; metabolomics; metabonomics; nuclear magnetic resonance.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Body Fluids / chemistry*
Feces / chemistry*
Horses / blood
Horses / metabolism*
Magnetic Resonance Spectroscopy / methods*
Metabolome*
Metabolomics / methods
Urine / chemistry*