Identifying biomarkers for asthma diagnosis using targeted metabolomics approaches

William Checkley; Maria P Deza; Jost Klawitter; Karina M Romero; Jelena Klawitter; Suzanne L Pollard; Robert A Wise; Uwe Christians; Nadia N Hansel

doi:10.1016/j.rmed.2016.10.011

Identifying biomarkers for asthma diagnosis using targeted metabolomics approaches

Respir Med. 2016 Dec:121:59-66. doi: 10.1016/j.rmed.2016.10.011. Epub 2016 Oct 21.

Authors

William Checkley¹, Maria P Deza², Jost Klawitter³, Karina M Romero⁴, Jelena Klawitter³, Suzanne L Pollard², Robert A Wise², Uwe Christians³, Nadia N Hansel²

Affiliations

¹ Division of Pulmonary and Critical Care, School of Medicine, Johns Hopkins University, Baltimore, USA. Electronic address: wcheckl1@jhmi.edu.
² Division of Pulmonary and Critical Care, School of Medicine, Johns Hopkins University, Baltimore, USA.
³ iC42 Clinical Research and Development, University of Colorado, Aurora, CO, USA.
⁴ Division of Pulmonary and Critical Care, School of Medicine, Johns Hopkins University, Baltimore, USA; Biomedical Research Unit, A.B. PRISMA, Lima, Peru.

Abstract

Background: The diagnosis of asthma in children is challenging and relies on a combination of clinical factors and biomarkers including methacholine challenge, lung function, bronchodilator responsiveness, and presence of airway inflammation. No single test is diagnostic. We sought to identify a pattern of inflammatory biomarkers that was unique to asthma using a targeted metabolomics approach combined with data science methods.

Methods: We conducted a nested case-control study of 100 children living in a peri-urban community in Lima, Peru. We defined cases as children with current asthma, and controls as children with no prior history of asthma and normal lung function. We further categorized enrollment following a factorial design to enroll equal numbers of children as either overweight or not. We obtained a fasting venous blood sample to characterize a comprehensive panel of targeted markers using a metabolomics approach based on high performance liquid chromatography-mass spectrometry.

Results: A statistical comparison of targeted metabolites between children with asthma (n = 50) and healthy controls (n = 49) revealed distinct patterns in relative concentrations of several metabolites: children with asthma had approximately 40-50% lower relative concentrations of ascorbic acid, 2-isopropylmalic acid, shikimate-3-phosphate, and 6-phospho-d-gluconate when compared to children without asthma, and 70% lower relative concentrations of reduced glutathione (all p < 0.001 after Bonferroni correction). Moreover, a combination of 2-isopropylmalic acid and betaine strongly discriminated between children with asthma (2-isopropylmalic acid ≤ 13 077 normalized counts/second) and controls (2-isopropylmalic acid > 13 077 normalized counts/second and betaine ≤ 16 47 121 normalized counts/second).

Conclusions: By using a metabolomics approach applied to serum, we were able to discriminate between children with and without asthma by revealing different metabolic patterns. These results suggest that serum metabolomics may represent a diagnostic tool for asthma and may be helpful for distinguishing asthma phenotypes.

Publication types

Research Support, N.I.H., Extramural

MeSH terms

Adolescent
Asthma / complications
Asthma / diagnosis*
Asthma / physiopathology
Betaine / blood
Biomarkers / blood*
Body Composition
Case-Control Studies
Child
Female
Humans
Malates / blood
Male
Metabolomics / methods*
Overweight / blood
Overweight / complications
Oxidative Stress / physiology
Young Adult

Substances

2-isopropylmalic acid
Biomarkers
Malates
Betaine

Grants and funding

R01 ES018845/ES/NIEHS NIH HHS/United States