Research

Selective accumulation of langerhans-type dendritic cells in small airways of patients with COPD

Geert R Van Pottelberge^1*, Ken R Bracke¹, Ingel K Demedts¹, Kim De Rijck¹, Susanne M Reinartz², Cornelis M van Drunen², Geert M Verleden³, Frank E Vermassen⁴, Guy F Joos¹ and Guy G Brusselle¹

• * Corresponding author: Geert R Van Pottelberge geert.vanpottelberge@ugent.be

Author Affiliations

¹ Laboratory for Translational Research in Obstructive Pulmonary Diseases, Department of Respiratory Medicine, Ghent University Hospital, Ghent, Belgium

² Department of Otorhinolaryngology, Academic Medical Center, Amsterdam, Netherlands

³ Department of Respiratory Medicine, University Hospital Gasthuisberg, Catholic University of Leuven, Belgium

⁴ Department of Thoracic and Vascular Surgery, Ghent University Hospital, Ghent, Belgium

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Respiratory Research 2010, 11:35 doi:10.1186/1465-9921-11-35

Published: 22 March 2010

Abstract

Background

Dendritic cells (DC) linking innate and adaptive immune responses are present in human lungs, but the characterization of different subsets and their role in COPD pathogenesis remain to be elucidated. The aim of this study is to characterize and quantify pulmonary myeloid DC subsets in small airways of current and ex-smokers with or without COPD.

Methods

Myeloid DC were characterized using flowcytometry on single cell suspensions of digested human lung tissue. Immunohistochemical staining for langerin, BDCA-1, CD1a and DC-SIGN was performed on surgical resection specimens from 85 patients. Expression of factors inducing Langerhans-type DC (LDC) differentiation was evaluated by RT-PCR on total lung RNA.

Results

Two segregated subsets of tissue resident pulmonary myeloid DC were identified in single cell suspensions by flowcytometry: the langerin+ LDC and the DC-SIGN+ interstitial-type DC (intDC). LDC partially expressed the markers CD1a and BDCA-1, which are also present on their known blood precursors. In contrast, intDC did not express langerin, CD1a or BDCA-1, but were more closely related to monocytes.

Quantification of DC in the small airways by immunohistochemistry revealed a higher number of LDC in current smokers without COPD and in COPD patients compared to never smokers and ex-smokers without COPD. Importantly, there was no difference in the number of LDC between current and ex-smoking COPD patients.

In contrast, the number of intDC did not differ between study groups. Interestingly, the number of BDCA-1+ DC was significantly lower in COPD patients compared to never smokers and further decreased with the severity of the disease. In addition, the accumulation of LDC in the small airways significantly correlated with the expression of the LDC inducing differentiation factor activin-A.

Conclusions

Myeloid DC differentiation is altered in small airways of current smokers and COPD patients resulting in a selective accumulation of the LDC subset which correlates with the pulmonary expression of the LDC-inducing differentiation factor activin-A. This study identified the LDC subset as an interesting focus for future research in COPD pathogenesis.