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Plasma IL ‐33 in atopic patients correlates with pro‐inflammatory cytokines and changes cholesterol transport protein expression: a surprising neutral overall impact on atherogenicity
Author(s) -
Voloshyna I.,
Mucci T.,
Sher J.,
Fonacier L. S.,
Littlefield M. J.,
Carsons S.,
Reiss A. B.
Publication year - 2015
Publication title -
clinical and experimental allergy
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.462
H-Index - 154
eISSN - 1365-2222
pISSN - 0954-7894
DOI - 10.1111/cea.12516
Subject(s) - endocrinology , medicine , chemistry , scavenger receptor , pathogenesis , inflammation , receptor , cholesterol , tumor necrosis factor alpha , cytokine , interleukin 4 , immunology , lipoprotein
Summary Objective Interleukin ( IL )‐33 has been associated with atopic and inflammatory conditions. IL ‐33 may be atheroprotective inducing a Th1‐to‐Th2 immunologic switch. However, the role of IL ‐33 in cardiovascular disease remains unclear. This study examines the effect of physiological and elevated IL ‐33 levels in plasma from atopic patients ( AP ) on cholesterol metabolism in human macrophages as compared to plasma from healthy controls ( HC ). Methods Twenty‐five AP and 25 HC were enrolled in this study. Plasma samples were analysed for levels of IL ‐33, IFN ‐γ, TNF ‐α, IL ‐17α, IL ‐5 and soluble ST 2. THP ‐1 differentiated macrophages were exposed to HC and AP plasma. Expression of proteins involved in reverse cholesterol transport ( ABCA 1, ABCG 1 and 27‐hydroxylase) and scavenger receptors, responsible for uptake of modified lipids ( CD 36, ScR‐A1, CXCL 16 and LOX ‐1), was measured using QRT ‐ PCR and immunoblotting techniques. Results IL ‐33 was significantly higher in AP plasma: 106.7 ± 95 pg/mL versus HC plasma (53.4 ± 23 pg/mL). IL ‐33 concentration strongly correlated with levels of IFN ‐γ ( r  = 0.85), TNF α ( r  = 0.9) and IL ‐17α ( r  = 0.94). No significant difference was found in soluble ST 2 levels. An important contrast was observed for 27‐hydroxylase: normal IL ‐33 in AP plasma amplified 27‐hydroxylase while increased IL ‐33 suppressed it. Expression of CD 36 and SR ‐A1 was greater in macrophages exposed to plasma with high IL ‐33, while CXCL 16 was higher in cells grown in the presence of plasma with normal IL ‐33. Conclusions Here, we demonstrate that high levels of IL ‐33 and a high IL ‐33/soluble ST 2 ratio correlates with elevated levels of IFN ‐γ, TNF ‐α and IL ‐17α as well as IL ‐5, demonstrating that IL ‐33 has pleiotropic effects. However, elevated IL ‐33 did not significantly impact lipid accumulation in macrophages overall. Given the wide variety of cellular responses regulated by IL ‐33, further investigation with a larger sample size will allow us to clarify the threshold concentration of IL ‐33 that leads to optimal cholesterol balance.

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