摘要
背景:弓形虫是一种单细胞寄生虫,能够感染人类和多种动物物种。虽然已知弓形虫感染会对肝脏和肠道微生物群产生不利影响,但受感染小鼠的肠道微生物群与肝脏转录组之间的确切相互作用在很大程度上仍是未知的。在本研究中,我们通过口服低剂量(n = 10)PRU(II型)裂头蚴,人工诱导BALB/c小鼠急性和慢性淋病感染。然后,我们进行了粪便 16S rRNA 基因扩增子测序和 RNA 转录组测序,以研究肠道微生物群的组成,以及在不同感染阶段小鼠肝脏中长非编码 RNA(lncRNA)、环状 RNA(circRNA)、microRNA(miRNA)和信使 RNA(mRNA)的表达谱:结果:分析显示,小鼠感染淋球菌后,肠道微生物群在感染周期内发生了动态变化。值得注意的是,我们观察到在感染的急性期肠杆菌科动物的丰度显著增加,而在慢性期乳杆菌科动物的丰度升高。肝脏转录组分析发现了许多差异表达(DE)的非编码RNA和mRNA,这些RNA和mRNA可能参与介导淋病双球菌诱导的肝脏免疫反应和炎症。在感染的急性期,包括Lpin1、Usp2、Pim3和Il6ra在内的几个促炎症基因在肝脏中显著上调。其中,Lpin1 可能与肠杆菌过度生长密切相关。相反,一些抗炎基因,如 Dmbt1 和 Ddit4,则只在慢性感染阶段上调。基因本体(GO)富集分析进一步揭示了肝脏功能的阶段性特征。具体来说,在感染的急性期,与炎症相关的通路被显著富集。有趣的是,在慢性感染阶段,与微生物群调节相关的通路,如 "对革兰氏阴性菌的防御反应"、"由抗菌肽介导的抗微生物体液免疫反应 "和 "抗微生物体液反应 "被富集。此外,竞争性内源 RNA(CeRNA)网络显示,许多 DElncRNA 和 DEcircRNA 竞争性地调控 DEmiRNA mmu-miR-690,后者靶向 Nr1d1 基因。这些发现让我们深入了解了在淋球菌感染的不同阶段肝脏与肠道微生物群之间复杂的相互作用:总之,我们的研究结果突显了小鼠感染淋球菌期间肝脏与肠道微生物群之间错综复杂的相互作用,在感染周期内,肠道微生物群的组成和肝脏中关键基因的表达谱都发生了动态变化。Background: Toxoplasma gondii is a single-cell parasite capable of infecting both humans and a variety of animal species. Although T. gondii infection is known to adversely affect the liver and gut microbiota, the precise interplay between the gut microbiome and the liver transcriptome in infected mice remains largely unknown. In this study, we artificially induced acute and chronic stages of T. gondii infection in BALB/c mice via the oral of low doses (n = 10) of PRU (Type II) bradyzoites. Then, we performed fecal 16S rRNA gene amplicon sequencing and RNA transcriptome sequencing to investigate the composition of the gut microbiota and the expression profiles of long non-coding RNAs (lncRNAs), circular RNAs (circRNAs), microRNAs (miRNAs), and messenger RNAs (mRNAs) in the livers of mice infected with T. gondii at different stages of infection.
Results: Analysis revealed dynamic alterations in the gut microbiota of mice following infection with T. gondii over the course of the infection cycle. Notably, we observed a significant increase in the abundance of Enterobacteriaceae during the acute stage of infection, while the abundance of Lactobacteriaceae was elevated during the chronic stage. Liver transcriptome analysis identified numerous differentially expressed (DE) non-coding RNAs and mRNAs potentially potentially involved in mediating liver immune responses and inflammation induced by T. gondii. During the acute stage of infection, several pro-inflammatory genes, including Lpin1, Usp2, Pim3, and Il6ra were significantly up-regulated in the liver. Among these, Lpin1 may be closely associated with the development of Enterobacteriaceae overgrowth. Conversely, some anti-inflammatory genes, such as Dmbt1, and Ddit4, were exclusively up-regulated during the chronic stage of infection. Gene ontology (GO) enrichment analysis further revealed the stage-specific features of liver functionality. Specifically, during the acute stage of infection, pathways associated with inflammation were significantly enriched. Interestingly, during the chronic stage of infection, pathways related to microbiota regulation, such as 'defense response to Gram-negative bacterium', 'antimicrobial humoral immune response mediated by antimicrobial peptide', and 'antimicrobial humoral response' were enriched. Additionally, competing endogenous RNAs (CeRNAs) networks revealed that numerous DElncRNAs and DEcircRNAs competitively regulated DEmiRNA mmu-miR-690, which targets the Nr1d1 gene. These findings provide insights into the complex interplay between the liver and gut microbiota during different stages of T. gondii infection.
Conclusions: In summary, our results highlight the intricate interaction between the liver and gut microbiota in mice during T. gondii infection, with dynamic alterations observed in both the gut microbiota composition and the expression profiles of key genes in the liver over the course of the infection cycle.
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