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肌苷介导 Toll 样受体 7(TLR7)和 TLR8 对 RNA 的感应调节。

Inosine-mediated modulation of RNA sensing by Toll-like receptor 7 (TLR7) and TLR8.

机构信息

Centre for Cancer Research, Monash Institute of Medical Research, Monash University, Clayton, Victoria, Australia.

出版信息

J Virol. 2014 Jan;88(2):799-810. doi: 10.1128/JVI.01571-13. Epub 2013 Nov 13.

Abstract

RNA-specific adenosine deaminase (ADAR)-mediated adenosine-to-inosine (A-to-I) editing is a critical arm of the antiviral response. However, mechanistic insights into how A-to-I RNA editing affects viral infection are lacking. We posited that inosine incorporation into RNA facilitates sensing of nonself RNA by innate immune sensors and accordingly investigated the impact of inosine-modified RNA on Toll-like receptor 7 and 8 (TLR7/8) sensing. Inosine incorporation into synthetic single-stranded RNA (ssRNA) potentiated tumor necrosis factor alpha (TNF-α) or alpha interferon (IFN-α) production in human peripheral blood mononuclear cells (PBMCs) in a sequence-dependent manner, indicative of TLR7/8 recruitment. The effect of inosine incorporation on TLR7/8 sensing was restricted to immunostimulatory ssRNAs and was not seen with inosine-containing short double-stranded RNAs or with a deoxy-inosine-modified ssRNA. Inosine-mediated increase of self-secondary structure of an ssRNA resulted in potentiated IFN-α production in human PBMCs through TLR7 recruitment, as established through the use of a TLR7 antagonist and Tlr7-deficient cells. There was a correlation between hyperediting of influenza A viral ssRNA and its ability to stimulate TNF-α, independent of 5'-triphosphate residues, and involving Adar-1. Furthermore, A-to-I editing of viral ssRNA directly enhanced mouse Tlr7 sensing, when present in proportions reproducing biologically relevant levels of RNA editing. Thus, we demonstrate for the first time that inosine incorporation into immunostimulatory ssRNA can potentiate TLR7/8 activation. Our results suggest a novel function of A-to-I RNA editing, which is to facilitate TLR7/8 sensing of phagocytosed viral RNA.

摘要

RNA 特异性腺苷脱氨酶 (ADAR)-介导的腺苷到肌苷 (A-to-I) 编辑是抗病毒反应的关键途径。然而,人们对 A-to-I RNA 编辑如何影响病毒感染的机制知之甚少。我们假设肌苷掺入 RNA 有助于先天免疫传感器识别非自身 RNA,并因此研究了肌苷修饰 RNA 对 Toll 样受体 7 和 8 (TLR7/8) 感应的影响。肌苷掺入合成的单链 RNA (ssRNA) 以序列依赖性方式增强了人外周血单核细胞 (PBMC) 中肿瘤坏死因子 α (TNF-α) 或α干扰素 (IFN-α) 的产生,表明 TLR7/8 的募集。肌苷掺入对 TLR7/8 感应的影响仅限于免疫刺激 ssRNA,而与含有肌苷的短双链 RNA 或脱氧肌苷修饰的 ssRNA 无关。肌苷介导的 ssRNA 自身二级结构增加导致通过 TLR7 募集增强 IFN-α 的产生,这是通过使用 TLR7 拮抗剂和 Tlr7 缺陷细胞建立的。流感 A 病毒 ssRNA 的超编辑与其刺激 TNF-α 的能力之间存在相关性,这与 5'-三磷酸残基无关,并且涉及 Adar-1。此外,当以复制生物学相关水平的 RNA 编辑的比例存在时,病毒 ssRNA 的 A-to-I 编辑直接增强了小鼠 Tlr7 的感应。因此,我们首次证明肌苷掺入免疫刺激 ssRNA 可以增强 TLR7/8 的激活。我们的研究结果表明 A-to-I RNA 编辑具有促进 TLR7/8 识别吞噬的病毒 RNA 的新功能。

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