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鲫鱼咽部黏孢子虫病组织局部的 RNA-seq 分析:鱼类-寄生虫对话中咽部黏膜免疫应答的新见解。

RNA-seq analysis of local tissue of Carassius auratus gibelio with pharyngeal myxobolosis: Insights into the pharyngeal mucosal immune response in a fish-parasite dialogue.

机构信息

Key Laboratory of Aquaculture Diseases Control, Ministry of Agriculture and State Key Laboratory of Freshwater Ecology and Biotechnology, Institute of Hydrobiology, Chinese Academy of Sciences, Wuhan, China; University of Chinese Academy of Sciences, Beijing, China.

Guangdong Provincial Water Environment and Aquatic Products Security Engineering Technology Research Center, Guangzhou Key Laboratory of Aquatic Animal Diseases and Waterfowl Breeding, College of Animal Sciences and Technology, Zhongkai University of Agriculture and Engineering, Guangzhou, Guangdong, China.

出版信息

Fish Shellfish Immunol. 2019 Nov;94:99-112. doi: 10.1016/j.fsi.2019.08.076. Epub 2019 Aug 30.

DOI:10.1016/j.fsi.2019.08.076
PMID:31476388
Abstract

The lack of practical control measures for pharyngeal myxobolosis is becoming an important limiting factor for the sustainable development of the gibel carp (Carassius auratus gibelio) culture industry in China. Myxobolus honghuensis has been identified as the causative agent of this pandemic disease, which exclusively infects the pharynx of gibel carp, a potential important mucosal lymphoid-associated tissue (MLAT). Myxozoa generally initiate invasion through the mucosal tissues of fish, where some of them also complete their sporogonial stages. However, the pharynx-associated immune responses of teleost against myxosporeans infection remain unknown. Here, a de novo transcriptome assembly of the pharynx of gibel carp naturally infected with M. honghuensis was performed for the first time, using RNA-seq. Comparative analysis of severely infected and mildly infected pharyngeal tissues (SI group and MI group) from the same fish individuals and control pharyngeal tissues (C group) from the uninfected fish was carried out to investigate the potential mucosal immune function of the fish pharynx, and characterize the panoramic picture of pharynx local mucosal immune responses of gibel carp against the M. honghuensis infection. A total of 242,341 unigenes were obtained and pairwise comparison resulted in 13,009 differentially-expressed genes (DEGs) in the SI/C group comparison, 6014 DEGs in the MI/C group comparison, and 9031 DEGs in the SI/MI group comparison. Comprehensive analysis showed that M. honghuensis infection elicited a significant parasite load-dependent alteration of the expression of numerous innate and adaptive immune-related genes in the local lesion tissue. Innate immune molecules, including mucins, toll-like receptors, C-type lectin, serum amyloid A, cathepsins and complement components were significantly up-regulated in the SI group compared with the C group. Up-regulation of genes involved in apoptosis signaling pathway and the IFN-mediated immune system were found in the SI group, suggesting these two pathways played a crucial role in innate immune response to M. honghuensis infection. Up-regulation of chemokines and chemokine receptors and the induction of the leukocyte trans-endothelial migration pathways in the severely and mildly infected pharynx suggested that many leucocytes were recruited to the local infected sites to mount a strong mucosal immune responses against the myxosporean infection. Up-regulation of CD3D, CD22, CD276, IL4/13A, GATA3, arginase 2, IgM, IgT and pIgR transcripts provided strong evidences for the presence of T/B cells and specific mucosal immune responses at local sites with M. honghuensis infection. Our results firstly demonstrated the mucosal function of the teleost pharynx and provided evidences of intensive local immune defense responses against this mucosa-infecting myxosporean in the gibel carp pharynx. Pharyngeal myxobolosis was shaped by a prevailing anti-inflammatory response pattern during the advanced infection stages. Further understanding of the functional roles of fish immune molecules involved in the initial invasion and/or final sporogony site may facilitate future development of control strategies for this myxobolosis.

摘要

咽部粘孢子虫病缺乏实用的控制措施,这正在成为中国异育银鲫养殖产业可持续发展的一个重要制约因素。已鉴定出湖北粘体虫是这种大流行疾病的病原体,它专门感染异育银鲫的咽部,这是一个潜在的重要黏膜相关淋巴组织(MLAT)。粘孢子虫通常通过鱼类的黏膜组织开始入侵,其中一些也在那里完成它们的孢子生殖阶段。然而,硬骨鱼类对粘孢子虫感染的咽相关免疫反应仍然未知。在这里,首次使用 RNA-seq 对自然感染湖北粘体虫的异育银鲫咽部进行了从头转录组组装。对来自同一鱼个体的严重感染和轻度感染咽部组织(SI 组和 MI 组)与未感染鱼的对照咽部组织(C 组)进行了比较分析,以研究鱼类咽部的潜在黏膜免疫功能,并描绘异育银鲫咽部对湖北粘体虫感染的局部黏膜免疫反应全景图。共获得 242341 个基因,在 SI/C 组比较中发现 13009 个差异表达基因(DEGs),在 MI/C 组比较中发现 6014 个 DEGs,在 SI/MI 组比较中发现 9031 个 DEGs。综合分析表明,湖北粘体虫感染引起了局部病变组织中大量固有和适应性免疫相关基因表达的显著寄生虫负荷依赖性改变。与 C 组相比,SI 组中多种先天免疫分子,包括粘蛋白、Toll 样受体、C 型凝集素、血清淀粉样蛋白 A、组织蛋白酶和补体成分显著上调。在 SI 组中发现了参与细胞凋亡信号通路和 IFN 介导的免疫系统的基因上调,表明这两个通路在先天免疫对湖北粘体虫感染的反应中发挥了关键作用。在严重和轻度感染的咽部中,趋化因子和趋化因子受体的上调以及白细胞跨内皮迁移途径的诱导表明,许多白细胞被招募到局部感染部位,对粘孢子虫感染产生强烈的黏膜免疫反应。CD3D、CD22、CD276、IL4/13A、GATA3、精氨酸酶 2、IgM、IgT 和 pIgR 转录本的上调为 T/B 细胞的存在和局部感染部位的特异性黏膜免疫反应提供了强有力的证据。我们的研究结果首次证明了硬骨鱼类咽部的黏膜功能,并为在异育银鲫咽部存在针对这种黏膜感染的粘孢子虫的强烈局部免疫防御反应提供了证据。咽部粘孢子虫病在晚期感染阶段形成了一种占主导地位的抗炎反应模式。进一步了解参与初始入侵和/或最终孢子生殖部位的鱼类免疫分子的功能作用,可能有助于未来开发针对这种粘孢子虫病的控制策略。

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