Kinetics of TH2 biomarkers in sputum of asthmatics following inhaled allergen

Rob G J A Zuiker; Marcella K Ruddy; Nicoletta Morelli; Robin Mogg; Veronica M Rivas; Kristien van Dyck; Inge De Lepeleire; Michael R L Tanen; J Diderik Boot; Ingrid M C Kamerling; Zuzana Diamant

doi:10.3402/ecrj.v2.28319

Kinetics of TH2 biomarkers in sputum of asthmatics following inhaled allergen

Eur Clin Respir J. 2015 May 26:2. doi: 10.3402/ecrj.v2.28319. eCollection 2015.

Authors

Affiliations

¹ Centre for Human Drug Research, Leiden, The Netherlands.
² EMD Serono, Rockland, MA, USA.
³ VU Medical Center, Amsterdam, The Netherlands.
⁴ Janssen Pharmaceutical Companies of Johnson & Johnson, Spring House, PA, USA.
⁵ Merck Research Laboratories, Rahway, NJ, USA.
⁶ Merck Research Laboratories, Brussels, Belgium.
⁷ HAL Allergy B.V., Leiden, The Netherlands.
⁸ Skane University Hospital, Department of Respiratory Medicine and Allergology, Institute for Clinical Science, Skane University, Lund, Sweden ; Departments of Clinical Pharmacy & Pharmacology and General Practice, University Medical Center Groningen, Groningen, The Netherlands ; QPS Netherlands, Groningen, The Netherlands.

Abstract

Background: Allergen-induced late airway response offers important pharmacodynamic targets, including T helper 2 (TH2) biomarkers. However, detection of inflammatory markers has been limited in dithiothreitol-processed sputum.

Objectives: To test whether allergen-induced TH2 inflammatory markers can be reproducibly quantified by sensitive detection techniques in ultracentrifuged sputum and the effect of fluticasone (FP) on these endpoints.

Methods: Thirteen allergic asthmatics with dual allergen-induced airway responses, documented during a single-blind placebo run-in period, participated in a double-blind, two-period crossover study. Each period consisted of three consecutive days, separated by ≥3 weeks. Following randomization, subjects inhaled FP (500 µg bid, five doses total) or placebo. On Day 2 in each study period, allergen challenge was performed and airway response measured by forced expiratory volume in 1 sec (FEV1) until 7 h post-challenge. Sputum was induced 24 h pre-allergen and 7 and 24 h post-allergen. Sputum samples were split into two portions: TH2 biomarkers were quantified by Meso Scale multiplex platform following ultracentrifugation, and cell differentials were counted on Giemsa-May-Grünwald-stained cytospins. Allergen-induced changes in inflammatory endpoints were compared between FP and placebo using a mixed model ANCOVA.

Results: Inhaled allergen induced dual airway responses in all subjects during both placebo periods with reproducible late asthmatic response (LAR) and increased sputum inflammatory biomarkers (IL-2, IL-4, IL-13, and eotaxin-1) and eosinophil counts. FP effectively blunted both the LAR and the inflammatory biomarkers.

Conclusions: Combining novel, sensitive quantification methods with ultracentrifugation allows reproducible quantification of sputum biomarkers following allergen challenge, reversed by FP. This approach allows non-invasive identification of pharmacodynamic targets for anti-asthma therapies.

Keywords: TH2 inflammation; allergen bronchial provocation test; asthma; fluticasone; sputum.