4.4 Article

The plasma metabolome of Atlantic salmon as studied by 1H NMR spectroscopy using standard operating procedures: effect of aquaculture location and growth stage

Journal

METABOLOMICS
Volume 17, Issue 6, Pages -

Publisher

SPRINGER
DOI: 10.1007/s11306-021-01797-0

Keywords

Metabolomics; H-1 NMR spectroscopy; NMR metabolomics; Atlantic salmon; Aquaculture; Standard operating procedures; SOP

Funding

  1. Norwegian Seafood Research Foundation, FHF Project [901435]
  2. Danish Innovation Foundation [IFD: 4105-00015B]

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This study applied H-1 NMR to analyze plasma metabolome in Atlantic salmon from Norway. Results showed significant metabolic differences between adult salmon and smolts, with different levels of lipoproteins, cholesterol, and propylene glycol. Growth stage accounted for 24% of metabolite variation, while aquaculture site and practice contributed 12%.
Introduction Metabolomics applications to the aquaculture research are increasing steadily. The use of standardized proton nuclear magnetic resonance (H-1 NMR) spectroscopy can provide the aquaculture industry with an unbiased, reproducible, and high-throughput screening tool, which can help to diagnose nutritional and disease-related metabolic disorders in farmed fish. Objective Standard operating procedures developed for analysing (human) plasma by H-1 NMR were applied to fingerprint the metabolome in plasma samples collected from Atlantic salmon. The aim was to explore the metabolome of salmon plasma in relation to growth stage and sampling site. Methods A total of 72 salmon were collected from three aquaculture sites in Norway (Lat. 65, 67, and 70 degrees N) and over two sampling events (December 2017 and November 2018). Plasma drawn from each salmon was measured by H-1 NMR and metabolites were quantified using the SigMa software. The NMR data was analysed by principal component analysis (PCA) and ANOVA-simultaneous component analysis (ASCA). Results Important metabolic differences were evidenced, with adult salmon having a much higher content of very low-density lipoproteins and cholesterol in their plasma, while smolts displayed significantly higher levels of propylene glycol. Overall, 24% of the metabolite variation was due to the growth stage, whereas 12% of the metabolite variation was related to the aquaculture site and practice (p < 0.001). Conclusion This study provides a baseline investigation of the plasma metabolome of the Atlantic salmon and demonstrates how H-1 NMR metabolomics can be used in future investigations for comparing aquaculture practices and their influence on the fish metabolome.

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