Department of Pathology, University of Texas Medical Branch, Galveston, TX, United States.
Institute for Human Infections and Immunity, University of Texas Medical Branch, University Boulevard, Galveston, TX, United States.
Front Immunol. 2019 Jan 9;9:3014. doi: 10.3389/fimmu.2018.03014. eCollection 2018.
Recent discovery that much of the mammalian genome does not encode protein-coding genes (PCGs) has brought widespread attention to long noncoding RNAs (lncRNAs) as a novel layer of biological regulation. Enhancer lnc (elnc) RNAs from the enhancer regions of the genome carry the capacity to regulate PCGs in or in . Spotted fever rickettsioses represent the consequence of host infection with Gram-negative, obligate intracellular bacteria in the Genus . Despite being implicated in the pathways of infection and inflammation, the roles of lncRNAs in host response to species have remained a mystery. We have profiled the expression of host lncRNAs during infection of susceptible mice with as a model closely mimicking the pathogenesis of human spotted fever rickettsioses. RNA sequencing on the lungs of infected hosts yielded reads mapping to 74,964 non-coding RNAs, 206 and 277 of which were determined to be significantly up- and down-regulated, respectively, in comparison to uninfected controls. Following removal of short non-coding RNAs and ambiguous transcripts, remaining transcripts underwent in-depth analysis of mouse lung epigenetic signatures H3K4Me1 and H3K4Me3, active transcript markers (POLR2A, p300, CTCF), and DNaseI hypersensitivity sites to identify two potentially active and highly up-regulated elncRNAs NONMMUT013718 and NONMMUT024103. Using Hi-3C sequencing resource, we further determined that genomic loci of NONMMUT013718 and NONMMUT024103 might interact with and regulate the expression of nearby PCGs, namely Id2 (inhibitor of DNA binding 2) and Apol10b (apolipoprotein 10b), respectively. Heterologous reporter assays confirmed the activity of elncRNAs as the inducers of their predicted PCGs. In the lungs of infected mice, expression of both elncRNAs and their targets was significantly higher than mock-infected controls. Induced expression of NONMMUT013718/Id2 in murine macrophages and NONMMUT024103/Apol10b in endothelial cells was also clearly evident during infection . Finally, shRNA mediated knock-down of NONMMUT013718 and NONMMUT024103 elncRNAs resulted in reduced expression of endogenous Id2 and Apl10b, demonstrating the regulatory roles of these elncRNAs on their target PCGs. Our results provide very first experimental evidence suggesting altered expression of pulmonary lncRNAs and elncRNA-mediated regulation of PCGs involved in immunity and during host interactions with pathogenic rickettsiae.
最近的发现表明,哺乳动物基因组的大部分并不编码蛋白质编码基因(PCGs),这使得长非编码 RNA(lncRNA)作为一种新的生物调控层受到广泛关注。基因组增强子区域的增强子 lnc(elnc)RNA 具有在或调节 PCGs 的能力。斑点热立克次体代表了宿主感染革兰氏阴性、专性细胞内细菌属的后果。尽管在感染和炎症途径中被牵连,但 lncRNA 在宿主对物种的反应中的作用仍然是一个谜。我们已经对易感小鼠感染作为一种模型进行了宿主 lncRNA 的表达谱分析,该模型非常类似于人类斑点热立克次体病的发病机制。对感染宿主肺部进行 RNA 测序,产生了映射到 74964 个非编码 RNA 的读数,其中 206 个和 277 个分别被确定为与未感染对照相比显著上调和下调。在去除短非编码 RNA 和模糊转录本后,剩余的转录本进行了小鼠肺表观遗传特征 H3K4Me1 和 H3K4Me3、活性转录本标记物(POLR2A、p300、CTCF)和 DNaseI 超敏位点的深入分析,以鉴定两个潜在的活性和高度上调的 elncRNA NONMMUT013718 和 NONMMUT024103。使用 Hi-3C 测序资源,我们进一步确定 NONMMUT013718 和 NONMMUT024103 的基因组位点可能相互作用并调节附近 PCGs 的表达,即 Id2(DNA 结合抑制因子 2)和 Apol10b(载脂蛋白 10b)。异源报告基因检测证实了 elncRNA 作为其预测 PCGs 的诱导物的活性。在感染小鼠的肺部,elncRNA 及其靶基因的表达均明显高于模拟感染对照。在感染过程中,在感染的小鼠巨噬细胞中诱导表达 NONMMUT013718/Id2 和内皮细胞中的 NONMMUT024103/Apol10b 也非常明显。最后,shRNA 介导的 NONMMUT013718 和 NONMMUT024103 elncRNA 的敲低导致内源性 Id2 和 Apl10b 的表达减少,证明了这些 elncRNA 对其靶 PCGs 的调节作用。我们的研究结果提供了第一个实验证据,表明肺 lncRNA 的表达改变和 elncRNA 介导的参与免疫和宿主与致病性立克次体相互作用的 PCGs 的调节。
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