利用 CRISPR/Cas9 基因编辑方法研究巨噬细胞中 Trem2 依赖性基因表达的机制

Mohnish Alishala
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摘要

髓系细胞上表达的触发受体 2(TREM2)是一种在组织损伤时在巨噬细胞中表达的表面受体。这种受体在驱动吞噬和抑制炎症方面发挥作用。因此,它在阿尔茨海默病、肝纤维化和代谢综合征等疾病中发挥着重要作用。这些疾病都有一群表达 TREM2 的巨噬细胞,而健康组织中并不存在这种巨噬细胞。然而,TREM2 参与这些疾病的确切途径尚不清楚。巨噬细胞基因表达受多种转录因子(如 ATF3 和 TFEB)调控。RNA-seq或ChIP-seq实验表明,这些转录因子参与了上述一些疾病过程。我们要解决的研究问题是,这两种转录因子如何直接影响巨噬细胞中的转录,特别是TREM2通路中的转录。我们利用 CRISPR/Cas9 基因编辑技术为每种转录因子生成功能缺失等位基因。结果显示,与Trem2基因敲除相比,Atf3基因敲除在RNA序列中上调或下调的基因很少。另一方面,Tfeb与Trem2基因敲除有13个基因的表达量低于对照组,有10个基因的表达量高于对照组。Tfeb 基因敲除组与对照组的 Trem2 表达量没有差异,这进一步证明了 Tfeb 位于 Trem2 的下游。由于在 Tfeb KO 中 Trem2 水平保持一致,因此 Trem2 对巨噬细胞疾病群体基因的一些影响很可能是通过 Tfeb 直接介导的。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Use of CRISPR/Cas9 Gene Editing Methods to Investigate the Mechanism of Trem2-Dependent Gene Expression in Macrophages
Triggering Receptor Expressed on Myeloid Cells 2 (TREM2) is a surface receptor expressed in macrophages during tissue injury. This receptor plays a role in driving phagocytosis and dampening inflammation. Because of this, it plays a large part in diseases such as Alzheimer’s disease, liver fibrosis, and metabolic syndrome. Each of these diseases all have a population of TREM2-expressing macrophages that does not exist in healthy tissue. However, the exact pathway in which TREM2 is involved in these diseases is rather unknown. Macrophage gene expression is regulated by a variety of transcription factors such as ATF3 and TFEB. These transcription factors have been suggested to be involved in some of the disease processes mentioned above by RNA-seq or ChIP-seq experiments.The research question we addressed was how these two transcription factors directly affectvtranscription in macrophages, specifically in the TREM2 pathway. CRISPR/Cas9 gene editing was used to generate loss of function alleles for each transcription factor. RNA-seq was then used to compare gene expression to define thegene-specific transcriptional roles of each factor and determine whether they play roles downstream of TREM2 signaling.Results showed that Atf3 knockout had very few genes upregulated or downregulated in the RNA seq compared to Trem2 knockout. Tfeb, on the other hand, had 13 genes in common with Trem2 knockout that were expressed lower than the control and 10 genes in common expressed higher than the control. The Tfeb knockout hadno difference in Trem2 expression between the knockout population and control, further providing evidence that Tfeb is located downstream of Trem2. Because Trem2 levels stayed consistent in the Tfeb KO, it is likely thatsome of the effects of Trem2 on the macrophage disease population genes are directly mediated through Tfeb.
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