Tristetraprolin expression by keratinocytes controls local and systemic inflammation
Mathieu Andrianne, Assiya Assabban, Caroline La, Denis Mogilenko, Delphine Staumont Salle, Sébastien Fleury, Gilles Doumont, Gaëtan Van Simaeys, Sergei A. Nedospasov, Perry J. Blackshear, David Dombrowicz, Stanislas Goriely, Laurye Van Maele
Mathieu Andrianne, Assiya Assabban, Caroline La, Denis Mogilenko, Delphine Staumont Salle, Sébastien Fleury, Gilles Doumont, Gaëtan Van Simaeys, Sergei A. Nedospasov, Perry J. Blackshear, David Dombrowicz, Stanislas Goriely, Laurye Van Maele
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Research Article Dermatology Inflammation

Tristetraprolin expression by keratinocytes controls local and systemic inflammation

Abstract

Tristetraprolin (TTP, encoded by the Zfp36 gene) regulates the mRNA stability of several important cytokines. Due to the critical role of this RNA-binding protein in the control of inflammation, TTP deficiency leads to the spontaneous development of a complex inflammatory syndrome. So far, this phenotype has been largely attributed to dysregulated production of TNF and IL‑23 by myeloid cells, such as macrophages or DCs. Here, we generated mice with conditional deletion of TTP in keratinocytes (Zfp36fl/flK14-Cre mice, referred to herein as Zfp36ΔEP mice). Unlike DC-restricted (CD11c-Cre) or myeloid cell–restricted (LysM-Cre) TTP ablation, these mice developed exacerbated inflammation in the imiquimod-induced psoriasis model. Furthermore, Zfp36ΔEP mice progressively developed a spontaneous pathology with systemic inflammation, psoriatic-like skin lesions, and dactylitis. Finally, we provide evidence that keratinocyte-derived TNF production drives these different pathological features. In summary, these findings expand current views on the initiation of psoriasis and related arthritis by revealing the keratinocyte-intrinsic role of TTP.

Authors

Mathieu Andrianne, Assiya Assabban, Caroline La, Denis Mogilenko, Delphine Staumont Salle, Sébastien Fleury, Gilles Doumont, Gaëtan Van Simaeys, Sergei A. Nedospasov, Perry J. Blackshear, David Dombrowicz, Stanislas Goriely, Laurye Van Maele

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Figure 5

TTP controls the mRNA stability of many proinflammatory mediators in TPA-stimulated primary mouse keratinocytes.

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TTP controls the mRNA stability of many proinflammatory mediators in TPA...
Primary keratinocytes isolated from Zfp36ΔEP and Zfp36fl/fl newborns were stimulated for 2 hours with TPA (100 ng/ml), rIL-17A (50 ng/ml), or rIL-22 (50 ng/ml). (A) Expression of Zfp36 was assessed by RTqPCR and Western blot (mock condition). (B) Gene expression in response to TPA stimulation. (C and D) Expression of Tnf (C) and Cxcl2 (D) after rIL-17A or rIL-22 stimulation. Results are given as mean ± SEM of at least 3 independent experiments performed in triplicate. Normalized mRNA levels were expressed relative to the Zfp36fl/fl untreated condition arbitrarily set to 1. (E) mRNA half-life analysis. Two hours after TPA stimulation, actinomycin D (10 μg/ml) and SB203580 (1 μM) were added for the indicated times. SB203580 was used to abolish the inhibitory effect of p38 MAPK on TTP activation. Total RNA was extracted and analyzed by RTqPCR. Results are given as mean ± SEM of 2 experiments performed in triplicate (a total of 6 wells from each genotype). Statistical significance (*P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001) was assessed by 1-way ANOVA test with Bonferroni correction (A) or by 2-tailed Mann-Whitney test compared with the Zfp36fl/fl group (BE).