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RIG-I 介导的抗病毒信号在 HIV-1 感染中被一种蛋白酶介导的 RIG-I 隔离所抑制。

RIG-I-mediated antiviral signaling is inhibited in HIV-1 infection by a protease-mediated sequestration of RIG-I.

机构信息

Terry Fox Molecular Oncology Group, Lady Davis Institute, Jewish General Hospital, Montreal, Quebec, Canada.

出版信息

J Virol. 2011 Feb;85(3):1224-36. doi: 10.1128/JVI.01635-10. Epub 2010 Nov 17.

Abstract

The rapid induction of type I interferon (IFN) is essential for establishing innate antiviral responses. During infection, cytoplasmic viral RNA is sensed by two DExD/H box RNA helicases, RIG-I and MDA5, ultimately driving IFN production. Here, we demonstrate that purified genomic RNA from HIV-1 induces a RIG-I-dependent type I IFN response. Both the dimeric and monomeric forms of HIV-1 were sensed by RIG-I, but not MDA5, with monomeric RNA, usually found in defective HIV-1 particles, acting as a better inducer of IFN than dimeric RNA. However, despite the presence of HIV-1 RNA in the de novo infection of monocyte-derived macrophages, HIV-1 replication did not lead to a substantial induction of IFN signaling. We demonstrate the existence of an evasion mechanism based on the inhibition of the RIG-I sensor through the action of the HIV-1 protease (PR). Indeed, the ectopic expression of PR resulted in the inhibition of IFN regulatory factor 3 (IRF-3) phosphorylation and decreased expression of IFN and interferon-stimulated genes. A downregulation of cytoplasmic RIG-I levels occurred in cells undergoing a single-cycle infection with wild-type provirus BH10 but not in cells transfected with a protease-deficient provirus, BH10-PR(-). Cellular fractionation and confocal microscopy studies revealed that RIG-I translocated from the cytosol to an insoluble fraction during the de novo HIV-1 infection of monocyte-derived macrophages, in the presence of PR. The loss of cytoplasmic RIG-I was prevented by the lysosomal inhibitor E64, suggesting that PR targets RIG-I to the lysosomes. This study reveals a novel PR-dependent mechanism employed by HIV-1 to counteract the early IFN response to viral RNA in infected cells.

摘要

I 型干扰素(IFN)的快速诱导对于建立先天抗病毒反应至关重要。在感染过程中,细胞质中的病毒 RNA 被两种 DEAD/DEAH box RNA 解旋酶 RIG-I 和 MDA5 识别,最终驱动 IFN 的产生。在这里,我们证明来自 HIV-1 的纯化基因组 RNA 诱导 RIG-I 依赖性 I 型 IFN 反应。RIG-I 识别 HIV-1 的二聚体和单体形式,但 MDA5 不识别,单体 RNA,通常存在于缺陷型 HIV-1 颗粒中,作为 IFN 的更好诱导物比二聚体 RNA。然而,尽管单核细胞衍生的巨噬细胞中的新感染存在 HIV-1 RNA,但 HIV-1 复制并没有导致 IFN 信号的大量诱导。我们证明了一种逃避机制的存在,该机制基于 HIV-1 蛋白酶(PR)的作用抑制 RIG-I 传感器。事实上,PR 的异位表达导致 IFN 调节因子 3(IRF-3)磷酸化的抑制和 IFN 和干扰素刺激基因的表达减少。在野生型前病毒 BH10 进行单轮感染的细胞中,细胞质 RIG-I 水平下调,但在转染缺乏蛋白酶的前病毒 BH10-PR(-)的细胞中则没有。细胞分离和共聚焦显微镜研究表明,在单核细胞衍生的巨噬细胞中发生新感染 HIV-1 时,RIG-I 从细胞质易位到不可溶部分,同时存在 PR。溶酶体抑制剂 E64 可防止细胞质 RIG-I 的丢失,表明 PR 将 RIG-I 靶向溶酶体。这项研究揭示了 HIV-1 用于抵抗感染细胞中病毒 RNA 早期 IFN 反应的一种新的 PR 依赖性机制。

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