税收诱导 NF-κB 招募到未整合的 HIV-1 DNA 以挽救病毒基因表达和复制。
Tax Induces the Recruitment of NF-κB to Unintegrated HIV-1 DNA To Rescue Viral Gene Expression and Replication.
机构信息
Department of Molecular Genetics and Microbiology, Duke University Medical Center, Durham, North Carolina, USA.
出版信息
J Virol. 2021 Jun 10;95(13):e0028521. doi: 10.1128/JVI.00285-21.
We previously reported that the normally essential step of integration of the HIV-1 proviral DNA intermediate into the host cell genome becomes dispensable in T cells that express the human T cell leukemia virus 1 (HTLV-1) Tax protein, a known activator of cellular NF-κB. The rescue of integrase (IN)-deficient HIV-1 replication by Tax results from the strong activation of transcription from the long terminal repeat (LTR) promoter on episomal HIV-1 DNA, an effect that is closely correlated with the recruitment of activating epigenetic marks, such as H3Ac, and depletion of repressive epigenetic marks, such as H3K9me3, from chromatinized unintegrated proviruses. In addition, activation of transcription from unintegrated HIV-1 DNA coincides with the recruitment of NF-κB to the two NF-κB binding sites found in the HIV-1 LTR enhancer. Here, we report that the recruitment of NF-κB to unintegrated viral DNA precedes, and is a prerequisite for, Tax-induced changes in epigenetic marks, so that an IN HIV-1 mutant lacking both LTR NF-κB sites is entirely nonresponsive to Tax and fails to undergo the epigenetic changes listed above. Interestingly, we found that induction of Tax expression at 24 h postinfection, when unintegrated HIV-1 DNA is already fully repressed by inhibitory chromatin modifications, is able to effectively reverse the epigenetic silencing of that DNA and rescue viral gene expression. Finally, we report that heterologous promoters introduced into IN-deficient HIV-1-based vectors are transcriptionally active even in the absence of Tax and do not increase their activity when the HIV-1 promoter and enhancer, located in the LTR U3 region, are deleted, as has been recently proposed. Integrase-deficient expression vectors based on HIV-1 are becoming increasingly popular as tools for gene therapy due to their inability to cause insertional mutagenesis. However, many IN lentiviral vectors are able to achieve only low levels of gene expression, and methods to increase this low level have not been extensively explored. Here, we analyzed how the HTLV-1 Tax protein is able to rescue the replication of IN HIV-1 in T cells, and we describe IN lentiviral vectors, lacking any inserted origin of replication, that are able to express a heterologous gene effectively.
我们之前报道过,在表达人类 T 细胞白血病病毒 1 (HTLV-1) Tax 蛋白的 T 细胞中,HIV-1 前病毒 DNA 中间体整合到宿主细胞基因组的正常必需步骤变得可有可无,Tax 是一种已知的细胞 NF-κB 激活剂。Tax 拯救整合酶 (IN) 缺陷型 HIV-1 复制是由于来自于染色体外 HIV-1 DNA 的长末端重复 (LTR) 启动子的转录被强烈激活,这种效应与激活的表观遗传标记(如 H3Ac)的募集以及抑制性表观遗传标记(如 H3K9me3)从染色质化未整合前病毒的耗竭密切相关。此外,未整合的 HIV-1 DNA 的转录激活与 NF-κB 募集到 HIV-1 LTR 增强子中的两个 NF-κB 结合位点相一致。在这里,我们报告说,NF-κB 募集到未整合的病毒 DNA 先于 Tax 诱导的表观遗传标记变化,并作为 Tax 诱导的表观遗传标记变化的先决条件,因此缺乏两个 LTR NF-κB 位点的 IN HIV-1 突变体完全对 Tax 无反应,并且不能经历上述表观遗传变化。有趣的是,我们发现,在感染后 24 小时诱导 Tax 表达,此时未整合的 HIV-1 DNA 已经被抑制性染色质修饰完全抑制,能够有效地逆转该 DNA 的表观遗传沉默并拯救病毒基因表达。最后,我们报告说,即使在没有 Tax 的情况下,引入 IN 缺陷型 HIV-1 为基础的载体中的异源启动子也具有转录活性,并且当位于 LTR U3 区域的 HIV-1 启动子和增强子被删除时,它们的活性不会增加,最近已经提出了这种情况。由于不能引起插入突变,基于 HIV-1 的 IN 缺陷型表达载体越来越多地被用作基因治疗工具。然而,许多 IN 慢病毒载体只能实现低水平的基因表达,并且尚未广泛探索增加这种低水平的方法。在这里,我们分析了 HTLV-1 Tax 蛋白如何拯救 T 细胞中 IN HIV-1 的复制,并且我们描述了缺乏任何插入复制起点的 IN 慢病毒载体,该载体能够有效地表达异源基因。
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