Periyasamy Palsamy, Singh Seema, Oladapo Abiola, Kannan Muthukumar, Buch Shilpa
Deparment of Pharmacology and Experimental Neuroscience, University of Nebraska Medical Center, Omaha, NE, United States.
Front Immunol. 2025 May 8;16:1558842. doi: 10.3389/fimmu.2025.1558842. eCollection 2025.
HIV proteins, such as the Transactivator of transcription (Tat), mediate neuroinflammation in the central nervous system by promoting the release of pro-inflammatory cytokines and chemokines. Long noncoding RNAs (lncRNAs) regulate gene expression by sponging microRNAs (miRs), but their role in HIV Tat-mediated microglial activation remains poorly understood. This study aimed to investigate the involvement of the lncRNA Xist-miR-124-CCL2 axis in HIV Tat-exposed microglial cells.
Mouse primary microglial cells were exposed to HIV Tat, and the expression of lncRNA Xist, miR-124, and CCL2 was evaluated using qPCR, Western blotting, and ELISA. Dual-luciferase reporter and Argonaute immunoprecipitation assays were used to confirm molecular interactions. Functional experiments involved lncRNA Xist silencing and miR-124 overexpression. validation was performed using doxycycline-inducible HIV Tat transgenic mice.
HIV Tat significantly upregulated lncRNA Xist and downregulated miR-124 expression in mouse primary microglial cells. miR-124 was identified as a direct target of lncRNA Xist and the 3'-UTR of CCL2. Silencing lncRNA Xist or overexpressing miR-124 reduced HIV Tat-induced CCL2 expression and microglial activation. studies corroborated these findings, with doxycycline-fed iTat mice showing elevated lncRNA Xist and CCL2 levels and reduced miR-124 expression in the frontal cortex.
Our findings identify a novel regulatory axis whereby HIV Tat-induced upregulation of lncRNA Xist sponges miR-124, leading to CCL2 overexpression and microglial activation. Targeting the lncRNA Xist-miR-124-CCL2 pathway may represent a promising therapeutic strategy to mitigate neuroinflammation associated with NeuroHIV.
HIV蛋白,如转录反式激活因子(Tat),通过促进促炎细胞因子和趋化因子的释放介导中枢神经系统的神经炎症。长链非编码RNA(lncRNA)通过吸附微小RNA(miR)来调节基因表达,但其在HIV Tat介导的小胶质细胞激活中的作用仍知之甚少。本研究旨在探讨lncRNA Xist-miR-124-CCL2轴在暴露于HIV Tat的小胶质细胞中的作用。
将小鼠原代小胶质细胞暴露于HIV Tat,使用qPCR、蛋白质免疫印迹法和酶联免疫吸附测定法评估lncRNA Xist、miR-124和CCL2的表达。采用双荧光素酶报告基因和AGO免疫沉淀试验来确认分子相互作用。功能实验包括lncRNA Xist沉默和miR-124过表达。使用强力霉素诱导的HIV Tat转基因小鼠进行验证。
HIV Tat显著上调小鼠原代小胶质细胞中lncRNA Xist的表达并下调miR-124的表达。miR-124被鉴定为lncRNA Xist和CCL2的3'-UTR的直接靶点。沉默lncRNA Xist或过表达miR-124可降低HIV Tat诱导的CCL2表达和小胶质细胞激活。体内研究证实了这些发现,喂食强力霉素的iTat小鼠额叶皮质中lncRNA Xist和CCL2水平升高,miR-124表达降低。
我们的研究结果确定了一种新的调节轴,即HIV Tat诱导的lncRNA Xist上调吸附miR-124,导致CCL2过表达和小胶质细胞激活。靶向lncRNA Xist-miR-124-CCL2途径可能是减轻与神经HIV相关的神经炎症的一种有前景的治疗策略。
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