Abstract

Respiratory health of children is a health priority. Club cell protein (CC16) is an interesting biomarker of lung diseases and adverse effects towards the airway epithelium integrity. Osteopontin (OPN) and nuclear factor-kappa B (NF-κB) also play a role in respiratory health. The use of urine as biomarker source is useful in studies involving children but necessitates proper adjustment for physiological confounders influencing the urinary excretion, potentially characterized with beta-2-microglobulin (β2M), retinol binding protein 4 (RBP4) or myoglobin (MYO), as well as adjustment for possible renal dysfunction, characterized by human serum albumin (HSA). The simultaneous quantification of all these proteins in urine could facilitate children’s health monitoring. A multiple reaction monitoring method (MRM) was developed and validated for the relative quantification of the seven mentioned urinary proteins. A total of nine proteotypic peptides were selected and used for the relative quantification of the seven proteins. The MRM method was completely validated for all proteins and partially for OPN. LOQ’s ranged from 0.3 to 42.8 ng/ml, a good reproducibility and a good linearity were obtained across the analytical measurement range (r2 > 0.98). The method yielded varying correlations (r2 of 0.78, 0.71, 0.34 and 0.15 for CC16, β2M, RBP4 and HSA respectively) with available immunoassay data. It also allowed the identification and successful quantification of β2M and RBP4 as a protein candidate for adjustment of renal handling and dysfunction. All proteins were detected in the urine samples except for MYO and NF-κB. Our validated MRM-method is able to simultaneously quantify in urine biomarkers of airway epithelium integrity and biomarkers of variation in renal function and urinary dilution. This will allow to investigate further in future studies if urine can be used as a good surrogate source for biomarkers of airway epithelium integrity, and to understand the complex relationship between cause and effect in children’s respiratory health monitoring.

Highlights

  • Respiratory health of children is a health priority

  • Abbreviations ACN Acetonitrile β2M Beta-2-microglobulin bovine serum albumin (BSA) Bovine serum albumin CC16 Club cell protein CE Collision energy DTT d l-Dithiothreitol formic acid (FA) Formic acid human serum albumin (HSA) Human serum albumin IAA Iodoacetamide LC–MS/MS Liquid chromatography coupled with tandem mass spectrometry latex immunoassay (LIA) Latex immunoassay

  • We aimed to develop and validate a monitoring method (MRM) method targeting simultaneously the potential protein biomarkers for respiratory health (CC16, NF-κB and OPN) or for renal dysfunction (HSA) as well as potential adjusters of renal handling (RBP4, MYO and β2M) and to allow relative quantification in urine from a study cohort of young children

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Summary

Introduction

Respiratory health of children is a health priority. Club cell protein (CC16) is an interesting biomarker of lung diseases and adverse effects towards the airway epithelium integrity. Our validated MRM-method is able to simultaneously quantify in urine biomarkers of airway epithelium integrity and biomarkers of variation in renal function and urinary dilution This will allow to investigate further in future studies if urine can be used as a good surrogate source for biomarkers of airway epithelium integrity, and to understand the complex relationship between cause and effect in children’s respiratory health monitoring. LMW Low-molecular-weight LOD Limit of detection LOQ Limit of quantification m/z Mass-to-charge ratio MRM Multiple reaction monitoring MS Mass spectrometry MYO Myoglobin NALF Nasal lavage fluid NF-κB Nuclear factor-kappa B NH4HCO3 Ammonium bicarbonate OPN Osteopontin RBP4 Retinol binding protein 4 resp. Its relation to lower airway inflammation has not been fully studied in childhood asthma

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