Cytokine production by leukocytes of Papillon-Lefèvre syndrome patients in whole blood cultures.

[papillon-lefèvre syndrome]

Papillon-Lefèvre syndrome (PLS ) is characterised by aggressively progressive periodontitis combined with palmo-plantar hyperkeratosis . It is caused by "loss of function " mutations in the cathepsin C gene . The hypothesis behind this study is that PLS patients ' polymorphonuclear leukocytes (PMNs ) produce more proinflammatory cytokines to compensate for their reduced capacity to neutralize leukotoxin and to eliminate Aggregatibacter actinomycetemcomitans . Production of more interleukin (IL )-8 would result in the attraction of more PMNs . The aim of this study was to evaluate the cytokine profile in PLS patients ' blood cultures . Blood was sampled from eight PLS patients (one female ) from six families (antiinfective therapy completed : six ; edentulous : two ) with confirmed cathepsin C mutations and deficient enzyme activity . Nine healthy males served as controls . Whole blood cultures were stimulated with highly pure lipopolysaccharide (LPS ) from Escherichia coli R 515 and IL -1 β plus tumor necrosis factor (TNF )-α . Thereafter , release of IL -1 β (stimulation : LPS and LPS plus adenosine triphosphate ), IL -6 , IL -8 , interferon-inducible protein (IP )-10 , and interferon (IFN )-γ (stimulation : LPS , IL -1 β /TNF α ) were detected by ELISA . Medians of cytokine release were , with the exception of IP-10 , slightly higher for PLS than for controls ' cultures . None of these differences reached statistical significance . Increased production of IL -1 β , IL -6 , IL -8 , IP-10 , or IFN γ as a significant means to compensate for diminished activity and stability of polymorphonuclear leukocyte-derived proteases could not be confirmed in this study . Cytokine profiles in blood cultures may not be used to identify PLS patients .