LncRNA MALAT1通过上调CHCHD2和下调IFN-I表达促进HIV-1复制。

IF 5.5 2区生物学 Q1 BIOCHEMICAL RESEARCH METHODS

Molecular & Cellular Proteomics Pub Date : 2025-07-01 Epub Date: 2025-05-23 DOI:10.1016/j.mcpro.2025.100997

Mei-Rong Wang, Cheng-Si Bai, Jian-Wei Dai, Lan Yang, Fang-Yi Quan, Jian-Chun Ma, Xing-Yuan Chen, Shao-Wei Zhu, Ying-Qi Xu, Zhou-Fu Xiang, Ya-le Jiang, Qi Cheng, Wei-Hao Zhang, Ke-Han Chen, Jian-Hua Wang, Yong Feng, Xiao-Ping Chen, Yong Xiong, Shu-Liang Chen, Wei Hou, Hai-Rong Xiong

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引用次数: 0

摘要

长链非编码RNA （lncRNAs）是细胞生物学中包括病毒复制在内的RNA和蛋白质功能的有效调节剂。新兴研究表明，lncrna通过调节不同的细胞机制激活或抑制HIV-1的复制和潜伏期。转移相关肺腺癌转录本1 （MALAT1）是副斑完整性所需的致癌lncRNA，已被证明与病毒感染有关。然而，其影响巨噬细胞中HIV-1感染的机制尚不清楚。在这项研究中，我们进行了rna深度测序，比较了感染HIV-1或不感染HIV-1的巨噬细胞中lncrna的谱，发现MALAT1在感染HIV-1的巨噬细胞中显著上调。MALAT1敲低抑制HIV-1感染，而MALAT1过表达增强病毒复制，表明MALAT1促进HIV-1复制。我们进一步进行了蛋白质组学分析，发现coiled-coil-helix-coil -coil-helix- helix- domain-containing 2 （CHCHD2）是受rnai介导的MALAT1敲低影响最下调的蛋白。接下来，我们证明MALAT1以CHCHD2依赖的方式促进HIV-1复制，并通过海绵化miR-145-5p作为竞争内源RNA调节CHCHD2表达，miR-145-5p可以相互结合MALAT1和CHCHD2 mRNA的3'UTR。此外，用特异性小干扰rna （sirna）敲低内源性MALAT1或CHCHD2可促进IRF7的表达，并增强干扰素-α和-β启动子的活性，增加干扰素刺激基因（ISG）和黏液病毒抗性蛋白B （MxB）的产生。此外，MALAT1或CHCHD2敲低可促进STAT2的表达，从而增强下游MxB的产生，从而扩大了CHCHD2作为先天免疫应答负调节因子的作用。这些发现提高了我们对巨噬细胞中MALAT1/miR-145-5p/CHCHD2通路调控HIV-1复制的理解，为潜在的靶向治疗干预提供了新的见解。

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LncRNA MALAT1 Facilitates HIV-1 Replication by Upregulation of CHCHD2 and Downregulation of IFN-I Expression.

Long noncoding RNAs (lncRNAs) are effective regulators of both RNA and protein functions throughout cell biology, including viral replication. Emerging studies have shown that lncRNAs activate or inhibit the replication and latency of HIV-1 by regulating different cellular mechanisms. Metastasis-associated lung adenocarcinoma transcript 1 (MALAT1) is an oncogenic lncRNA required for paraspeckle integrity and has been proven to be linked to viral infection. However, the mechanisms by which it influences HIV-1 infection in macrophages remain unclear. In this study, we performed RNA-deep sequencing to compare the profiles of lncRNAs in macrophages with or without HIV-1 and found that MALAT1 was dramatically upregulated in HIV-1-infected macrophages. MALAT1 knockdown inhibited HIV-1 infection, whereas MALAT1 overexpression enhanced viral replication, indicating that MALAT1 promotes HIV-1 replication. We further performed proteomics analysis and found that coiled-coil-helix-coiled-coil-helix domain-containing 2 (CHCHD2) was the most downregulated protein affected by RNAi-mediated knockdown of MALAT1. We next demonstrated that MALAT1 favored HIV-1 replication in a CHCHD2-dependent manner and functioned as a competing endogenous RNA to regulate CHCHD2 expression by sponging miR-145-5p, which could mutually bind the MALAT1 and 3'UTR of chchd2 mRNA. Furthermore, knockdown of endogenous MALAT1 or CHCHD2 with specific small interfering RNAs (siRNAs) promoted the expression of IRF7, and enhanced the promoter activities of interferons-α and -β, increasing their production as well as that of a critical interferon-stimulated gene (ISG), myxovirus resistance protein B (MxB). Moreover, MALAT1 or CHCHD2 knockdown promoted the expression of STAT2 to enhance the production of downstream MxB, which expanded the role of CHCHD2 as a negative regulator of the innate immune response. These findings improve our understanding of MALAT1/miR-145-5p/CHCHD2 pathway regulation of HIV-1 replication in macrophages, providing new insights into potential targeted therapeutic interventions.

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来源期刊

Molecular & Cellular Proteomics 生物-生化研究方法

CiteScore

11.50

自引率

4.30%

发文量

131

审稿时长

84 days

期刊介绍： The mission of MCP is to foster the development and applications of proteomics in both basic and translational research. MCP will publish manuscripts that report significant new biological or clinical discoveries underpinned by proteomic observations across all kingdoms of life. Manuscripts must define the biological roles played by the proteins investigated or their mechanisms of action. The journal also emphasizes articles that describe innovative new computational methods and technological advancements that will enable future discoveries. Manuscripts describing such approaches do not have to include a solution to a biological problem, but must demonstrate that the technology works as described, is reproducible and is appropriate to uncover yet unknown protein/proteome function or properties using relevant model systems or publicly available data. Scope: -Fundamental studies in biology, including integrative "omics" studies, that provide mechanistic insights -Novel experimental and computational technologies -Proteogenomic data integration and analysis that enable greater understanding of physiology and disease processes -Pathway and network analyses of signaling that focus on the roles of post-translational modifications -Studies of proteome dynamics and quality controls, and their roles in disease -Studies of evolutionary processes effecting proteome dynamics, quality and regulation -Chemical proteomics, including mechanisms of drug action -Proteomics of the immune system and antigen presentation/recognition -Microbiome proteomics, host-microbe and host-pathogen interactions, and their roles in health and disease -Clinical and translational studies of human diseases -Metabolomics to understand functional connections between genes, proteins and phenotypes