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东方蜜蜂微孢子虫侵染意大利蜜蜂工蜂过程中nce-miR-12220及其靶基因的表达谱
引用本文:吴鹰,叶亚萍,张佳欣,钱加珺,张文德,余岢骏,吉挺,蔺哲广,赵红霞,陈大福,郭睿.东方蜜蜂微孢子虫侵染意大利蜜蜂工蜂过程中nce-miR-12220及其靶基因的表达谱[J].菌物学报,2022,41(10):1546-1557.
作者姓名:吴鹰  叶亚萍  张佳欣  钱加珺  张文德  余岢骏  吉挺  蔺哲广  赵红霞  陈大福  郭睿
作者单位:1 福建农林大学动物科学学院(蜂学学院),福建 福州 3500022 福建农林大学蜂疗研究所,福建 福州 3500023 扬州大学动物科学与技术学院,江苏 扬州 2250004 广东省科学院动物研究所,广东 广州 510260
基金项目:国家自然科学基金(32172792);财政部和农业农村部国家现代农业产业技术体系(CARS-44-KXJ7);福建农林大学硕士生导师团队项目;福建农林大学杰出青年科研人才计划项目(xjq201814);国家级大学生创新创业训练计划项目;福建省大学生创新创业训练计划项目(202210389128);福建省大学生创新创业训练计划项目(202210389115)
摘    要:东方蜜蜂微孢子虫Nosema ceranae侵染成年蜜蜂导致蜜蜂微孢子虫病。本研究旨在验证东方蜜蜂微孢子虫nce-miR-12220的存在和表达,并检测nce-miR-12220及其靶基因在病原侵染意大利蜜蜂Apis mellifera ligustica (简称意蜂)工蜂过程的表达谱。Stem-loop RT-PCR和Sanger测序结果显示nce-miR-12220真实存在和表达。靶向预测结果显示nce-miR-12220共靶向KRAB-Aγ tubulin等15个基因。上述靶基因可注释到19个GO条目和3条KEGG通路。RT-qPCR结果显示,相较于接种后1 d (1 day post infection,1 dpi),nce-miR-12220在2 dpi上调表达,而在3-12 dpi阶段总体表现出显著下调表达的趋势。类似地,与1 dpi相比,靶基因KRAB-A在2 dpi上调表达,而在3-12 dpi阶段总体呈下调表达的趋势。另外,与1 dpi相比,靶基因γ tubulin在2-12 dpi阶段总体表现出显著下调表达的趋势。上述结果表明nce-miR-12220与KRAB-Aγ tubulin之间存在潜在的靶向结合和正向调控关系;东方蜜蜂微孢子虫通过下调表达nce-miR-12220抑制KRAB-A的表达进而促进增殖;意蜂工蜂可能通过抑制东方蜜蜂微孢子虫的γ tubulin表达抵御病原侵染。研究结果明确了nce-miR-12220及其靶基因KRAB-Aγ tubulin在东方蜜蜂微孢子虫侵染意蜂工蜂过程中的动态表达规律,为深入探究nce-miR-12220在病原侵染中的功能及调控机制提供了理论和实验依据。

关 键 词:意大利蜜蜂  东方蜜蜂微孢子虫  微小RNA  调控网络  表达谱  正调控  
收稿时间:2022-01-18

Expression profiles of nce-miR-12220 and its target genes during the Nosema ceranae infection process of Apis mellifera ligustica workers
Authors:WU Ying  YE Yaping  ZHANG Jiaxin  QIAN Jiajun  ZHANG Wende  YU Kejun  JI Ting  LIN Zheguang  ZHAO Hongxia  CHEN Dafu  GUO Rui
Institution:1 College of Animal Sciences (College of Bee Science), Fujian Agriculture and Forestry University, Fuzhou 350002, Fujian, China2 Apitherapy Institute, Fujian Agriculture and Forestry University, Fuzhou 350002, Fujian, China3 College of Animal Science and Technology, Yangzhou University, Yangzhou 225000, Jiangsu, China4 Institute of Zoology, Guangdong Academy of Sciences, Guangzhou 510260, Guangdong, China
Abstract:Nosema ceranae infects adult bee and results in nosemosis. This study aims at verifying the existence and expression of nce-miR-12220 and detecting the expression profiles of nce-miR-12220 and its target genes during the N. ceranae infection of Apis mellifera ligustica workers. Stem-loop RT-PCR and Sanger sequencing confirmed the true existence and expression of nce-miR-12220. Targeting prediction showed that nce-miR-12220 can target a total of 15 genes. These targets could be annotated to 19 GO terms and 3 KEGG pathways, respectively. RT-qPCR test indicated that compared with nce-miR-12220 at 1 day post infection (1 dpi ), nce-miR-12220 was up-regulated at 2 dpi and significantly down-regulated during the stage of 3-12 dpi. Similarly, in comparison with KRAB-A at 1 dpi, the target gene KRAB-A was up-regulated at 2 dpi and down-regulated during the stage of 3-12 dpi. The target gene γ tubulin presented an overall significantly down-regulated trend during the stage of 2-12 dpi as compared with that at 1 dpi. These results suggest that there is potential target binding and positive regulation relationship between nce-miR-12220 and KRAB-A and γ tubulin; N. ceranae likely suppressed the expression of KRAB-A by down-regulating nce-miR-12220, further promoting its own proliferation; A. m. ligustica workers probably resist N. ceranae invasion through inhibiting the γ tubulin expression. The findings not only reveal the dynamic expression rule of nce-miR-12220 and target genes KRAB-A and γ tubulin during the N. ceranae infection of A. m. ligustica workers, but also provide theoretical and experimental bases for further investigating the function and regulatory mechanism of nce-miR-12220 in the infection process.
Keywords:Apis mellifera ligustica   Nosema ceranae  microRNA  regulation network  expression profile  positive regulation  
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