| Literature DB >> 28318807 |
Siobhán Smith1, Thilini Fernando2, Pei Wen Wu2, Jane Seo2, Joan Ní Gabhann1, Olga Piskareva1, Eoghan McCarthy3, Donough Howard3, Paul O'Connell4, Richard Conway4, Phil Gallagher4, Eamonn Molloy4, Raymond L Stallings1, Grainne Kearns5, Lindsy Forbess6, Mariko Ishimori6, Swamy Venuturupalli6, Daniel Wallace6, Michael Weisman6, Caroline A Jefferies7.
Abstract
Systemic lupus erythematosus (SLE) is a complex disease targeting multiple organs as a result of overactivation of the type I interferon (IFN) system, a feature currently being targeted by multiple biologic therapies against IFN-α. We have identified an estrogen-regulated microRNA, miR-302d, whose expression is decreased in SLE patient monocytes and identify its target as interferon regulatory factor (IRF)-9, a critical component of the transcriptional complex that regulates expression of interferon-stimulated genes (ISGs). In keeping with the reduced expression of miR-302d in SLE patient monocytes, IRF9 levels were increased, as was expression of a number of ISGs including MX1 and OAS1. In vivo evaluation revealed that miR-302d protects against pristane-induced inflammation in mice by targeting IRF9 and hence ISG expression. Importantly, patients with enhanced disease activity have markedly reduced expression of miR-302d and enhanced IRF9 and ISG expression, with miR-302d negatively correlating with IFN score. Together these findings identify miR-302d as a key regulator of type I IFN driven gene expression via its ability to target IRF9 and regulate ISG expression, underscoring the importance of non-coding RNA in regulating the IFN pathway in SLE.Entities:
Keywords: IFN signalling; IFN-stimulated genes; MicroRNA; SLE
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Year: 2017 PMID: 28318807 DOI: 10.1016/j.jaut.2017.03.003
Source DB: PubMed Journal: J Autoimmun ISSN: 0896-8411 Impact factor: 7.094