Estimation of Chicken Intake by Adults Using Metabolomics-Derived Markers

Xiaofei Yin; Helena Gibbons; Milena Rundle; Gary Frost; Breige A McNulty; Anne P Nugent; Janette Walton; Albert Flynn; Michael J Gibney; Lorraine Brennan

doi:10.3945/jn.117.252197

Estimation of Chicken Intake by Adults Using Metabolomics-Derived Markers

J Nutr. 2017 Oct 1;147(10):1850-1857. doi: 10.3945/jn.117.252197.

Authors

Affiliations

¹ School of Agriculture and Food Science, Institute of Food and Health, University College Dublin, Dublin, Ireland.
² Faculty of Medicine, Department of Medicine, Imperial College London, London, United Kingdom.
³ School of Food and Nutritional Sciences, University College Cork, Cork, Ireland.

PMID: 28794208
DOI: 10.3945/jn.117.252197

Abstract

Background: Improved assessment of meat intake with the use of metabolomics-derived markers can provide objective data and could be helpful in clarifying proposed associations between meat intake and health.

Objective: The objective of this study was to identify novel markers of chicken intake using a metabolomics approach and use markers to determine intake in an independent cohort.

Methods: Ten participants [age: 62 y; body mass index (in kg/m2): 28.25] in the NutriTech food intake study consumed increasing amounts of chicken, from 88 to 290 g/d, in a 3-wk span. Urine and blood samples were analyzed by nuclear magnetic resonance and mass spectrometry, respectively. A multivariate data analysis was performed to identify markers associated with chicken intake. A calibration curve was built based on dose-response association using NutriTech data. A Bland-Altman analysis evaluated the agreement between reported and calculated chicken intake in a National Adult Nutrition Survey cohort.

Results: Multivariate data analysis of postprandial and fasting urine samples collected in participants in the NutriTech study revealed good discrimination between high (290 g/d) and low (88 g/d) chicken intakes. Urinary metabolite profiles showed differences in metabolite levels between low and high chicken intakes. Examining metabolite profiles revealed that guanidoacetate increased from 1.47 to 3.66 mmol/L following increasing chicken intakes from 88 to 290 g/d (P < 0.01). Using a calibration curve developed from the NutriTech study, chicken intake was calculated through the use of data from the National Adult Nutrition Survey, in which consumers of chicken had a higher guanidoacetate excretion (0.70 mmol/L) than did nonconsumers (0.47 mmol/L; P < 0.01). A Bland-Altman analysis revealed good agreement between reported and calculated intakes, with a bias of -30.2 g/d. Plasma metabolite analysis demonstrated that 3-methylhistidine was a more suitable indicator of chicken intake than 1-methylhistidine.

Conclusions: Guanidoacetate was successfully identified and confirmed as a marker of chicken intake, and its measurement in fasting urine samples could be used to determine chicken intake in a free-living population. This trial was registered at clinicaltrials.gov as NCT01684917.

Keywords: 3-methylhistidine; dietary markers; estimated chicken intake; guanidoacetate; metabolomics.

MeSH terms

Animals
Biomarkers / analysis
Chickens
Fasting / urine
Female
Glycine / analogs & derivatives*
Glycine / urine
Humans
Male
Meat*
Metabolomics*
Methylhistidines / blood*
Middle Aged
Red Meat

Substances

Biomarkers
Methylhistidines
glycocyamine
3-methylhistidine
Glycine

Associated data

ClinicalTrials.gov/NCT01684917