基于转录组测序的金银花提取物抗鸽源新城疫病毒感染的作用机制研究

doi:10.12160/j.issn.1672-5190.2024.04.002

摘要/Abstract

摘要： [目的]探究金银花提取物抗鸽源新城疫病毒（Newcastle disease virus,NDV）感染的作用机制。[方法]选取未接种NDV疫苗的健康28日龄美国王鸽40只,适应性饲养7 d,于35日龄随机分为金银花预防（KO）组和攻毒对照（OE）组,每组20只。KO组试验鸽于35日龄开始在饮水中添加1.2%的金银花提取物,持续饮用7 d,42日龄时肌肉注射HA效价为5log2的鸽源NDV Pi/NJ/CH/4416/2016株0.5 mL/只;OE组试验鸽于35日龄进入正式试验,正常饮水,42日龄时肌肉注射HA效价为5log2的鸽源NDV Pi/NJ/CH/4416/2016株0.5 mL/只。攻毒7 d后,每组选取3只试验鸽采集脾脏组织样本制备组织切片,同时提取总RNA构建转录组文库,利用转录组测序（RNA-sequencing,RNA-Seq）技术进行差异表达基因（differentially expressed genes,DEGs）鉴定、GO功能富集分析和KEGG通路富集分析。随机选取4个显著差异表达基因,利用qRT-PCR验证测序结果。[结果]OE组鸽子脾细胞核异常增大且出现白色空泡,并伴有大量粒细胞浸润,而KO组脾脏组织仅见较多白色空泡和少量粒细胞浸润,未见脾细胞核异常增大。利用RNA-Seq技术从KO组鸽脾脏中共鉴定出374个DEGs,其中,112个基因表达显著上调,262个基因表达显著下调。GO功能富集分析显示,共有875个DEGs富集到312个GO条目,其中,生物学过程富集到149个条目,细胞组成过程富集到33个条目,分子功能过程富集到130个条目。KEGG通路富集分析显示,共有226个DEGs主要被富集在信息传递通路、代谢通路、天然免疫相关通路、细胞凋亡通路等93条KEGG信号通路。qRT-PCR验证结果显示,从DEGs中随机选取的4个显著差异表达基因（LOC110360702、LOC110360688、SFRP5、CHAD）的相对mRNA丰度变化趋势与RNA-Seq结果显示的4个基因变化趋势一致。[结论]金银花提取物通过激活宿主的信息传递、代谢调节及免疫应答等重要生理过程发挥抗鸽源NDV感染作用。研究结果为进一步探究鸽源NDV感染中免疫应答的分子机制提供了科学依据。

关键词: 鸽, 新城疫病毒, 金银花, 转录组测序, 差异表达基因, 天然免疫

Abstract: [Objective] This study was conducted to assess the mechanisms underlying the protective role of honeysuckle extract against Newcastle disease virus （NDV） infection in pigeon. [Method] A total of 40 healthy 28-day-old American king pigeons without NDV vaccination were selected and subjected to a 7-day adaptive rearing. At the age of 35 days, the experimental pigeons were randomly assigned into a honeysuckle extract protective （KO） group （n=10） or a virus challenge control （OE） group （n=10）. The pigeons in KO group drank the water containing 1.2% honeysuckle extract for 7 consecutive days, and at the age of 42 days, they were intramuscularly injected with 0.5 mL NDV Pi/NJ/CH/4416/2016 strain of pigeon origin with HA potency of 5log2 . The pigeons in OE group drank the normal water and were challenged with the same NDV strain at the same dosage at the age of 42 days. Seven days after challenge, 3 pigeons were chosen from both KO and OE groups. The spleen samples were collected for paraffin-embedded tissue section preparation and for total RNA extraction to construct the transcriptome libraries. RNA-Seq was used to identify differentially expressed genes （DEGs） and to perform GO functional enrichment analysis as well as KEGG pathway enrichment analysis. Four randomly selected significant DEGs identified by RNA-Seq were verified by using qRT-PCR. [Result] The splenocytes of the pigeons in OE group had abnormally enlarged nuclei and white vacuoles, accompanied by a large number of granulocyte infiltration in splenic tissues, while those of the pigeons in KO group had many white vacuoles and minor granulocyte infiltration alone, and no abnormally enlarged splenocyte nuclei in splenic tissues were observed. A total of 374 DEGs were identified in the spleens of the pigeons in KO group by RNA-Seq, of which 112 were significantly up-regulated and 262 were significantly down-regulated. GO functional enrichment analysis demonstrated that 875 DEGs were enriched in 312 GO entries, of which 149 belonged to biological process, 33 belonged to cellular component, and 130 belonged to molecular function. KEGG pathway enrichment analysis revealed that 226 DEGs were enriched in 93 KEGG signaling pathways, including information transmission pathway, metabolic pathway, natural immunity related pathway, and apoptosis pathway. The qRT-PCR validation test showed that the relative mRNA abundance of the 4 randomly selected significant DEGs （LOC110360702, LOC110360688, SFRP5 and CHAD） had the same change trend as the RNA-Seq results. [Conclusion] Honeysuckle extract exerts protective role against NDV infection in pigeon by activating important physiological processes of host such as information transmission, metabolic regulation and immune response. The results obtained in this study provide a scientific basis for further investigation on the molecular mechanism of immune response to NDV infection in pigeon.

Key words: pigeon, Newcastle disease virus, honeysuckle, RNA-Seq, differentially expressed genes, natural immunity

中图分类号:

莫红芳, 石宗承, 杨燕燕, 俸云, 虞霖田, 石德顺, 熊晓妍. 基于转录组测序的金银花提取物抗鸽源新城疫病毒感染的作用机制研究[J]. 畜牧与饲料科学, 2024, 45(4): 10-19.

MO Hongfang, SHI Zongcheng, YANG Yanyan, FENG Yun, YU Lintian, SHI Deshun, XIONG Xiaoyan. Transcriptome Sequencing Analysis Reveals the Potential Molecular Mechanisms of Honeysuckle Extract in Protecting Newcastle Disease Virus Infection in Pigeon[J]. Animal Husbandry and Feed Science, 2024, 45(4): 10-19.

参考文献

[1] MAYO M A.Virus taxonomy - Houston 2002[J].Archives of Virology,2002,147(5):1071-1076.
[2] 何颖. 鸽Ⅰ型副黏病毒的全基因组测序及病原学特性分析[D].南宁:广西大学,2020.
[3] HAMAGUCHI M,YOSHIDA T,NISHIKAWA K,et al.Transcriptive complex of Newcastle disease virus. Ⅰ. Both L and P proteins are required to constitute an active complex[J].Virology,1983,128(1):105-117.
[4] UJVARI D.Phylogenetic analysis reveals extensive evolution of avian paramyxovirus type 1 strains of pigeons (Columba livia) and suggests multiple species transmission[J].Virus Research,2003,96(1/2):63-73.
[5] 撒薇. PPMV-1的分离鉴定、代表性毒株的全基因组序列分析及细胞凋亡通路相关因子RT-qPCR方法的建立[D].南宁:广西大学,2021.
[6] GANAR K,DAS M,RAUT A A,et al.Emergence of a deviating genotype Ⅵ pigeon paramyxovirus type-1 isolated from India[J].Archives of Virology,2017,162(7):2169-2174.
[7] NOORUZZAMAN M,BARMAN L R,MUMU T T,et al.A pigeon-derived sub-genotype ⅩⅪ.1.2 Newcastle disease virus from Bangladesh induces high mortality in chickens[J].Viruses,2021,13(8):1520.
[8] 原宇. 鸽Ⅰ型副黏病毒分离鉴定及其灭活疫苗和卵黄抗体制备[D].杨凌:西北农林科技大学,2022.
[9] 莫红芳,石宗承,何东贤,等.金银花对鸽新城疫病毒感染肉鸽器官组织、血清免疫指标及抗氧化能力的影响[J].畜禽业,2024,35(1):1-8.
[10] 张仁群,李仪晴,刘子怡,等.金银花多糖的提取、分离纯化、结构特征和生物活性研究进展[J].中华中医药学刊,2023,41(5):155-159.
[11] 莫红芳,石宗承,何东贤,等.金银花的生物学功能及其在动物生产中的应用研究进展[J].中国畜牧杂志,2024,60(2):7-11.
[12] 王苡瑄,李菲,王洁,等.基于网络药理学的金花葵抗心肌缺血的作用机制研究[J].中国药师,2020,23(9):1700-1709.
[13] 林乐丰,刁云飞,范冰峰,等.基于高通量测序的梅花鹿卵巢衰老的转录组分析[J].中国畜牧兽医,2023,50(8):3157-3170.
[14] 张驰,陈嘉婷,辛紫萱,等.弓形虫慢性感染小鼠脑转录组分析及与抑郁相关的犬尿氨酸通路的验证[J].中国寄生虫学与寄生虫病杂志,2023,41(3):270-278.
[15] 张一帆. 基因Ⅵk亚型PPMV-1分离鉴定及致病性分析[D].广州:华南农业大学,2019.
[16] 刘世谋. 珠三角地区鸽新城疫流行病学调查及综合免疫程序优化[D].广州:华南农业大学,2018.
[17] BARBEZANGE C,JESTIN V.Molecular study of the quasispecies evolution of a typical pigeon paramyxovirus type 1 after serial passages in pigeons by contact[J].Avian Pathology,2005,34(2):111-122.
[18] LUO B B,XU Y F,WU S X,et al.A novel immunosensor based on excessively tilted fiber grating coated with gold nanospheres improves the detection limit of Newcastle disease virus[J].Biosensors and Bioelectronics,2018,100:169-175.
[19] ELMARDI N A,BAKHEIT M A,KHALAFALLA A I.Phylogenetic analysis of some Newcastle disease virus isolates from the Sudan[J].Open Veterinary Journal,2016,6(2):89-97.
[20] CHEN F,CHAN K H,JIANG Y,et al.In vitro susceptibility of 10 clinical isolates of SARS coronavirus to selected antiviral compounds[J].Journal of Clinical Virology,2004,31(1):69-75.
[21] SHINADA M,AZUMA M,KAWAI H,et al.Enhancement of interferon-gamma production in glycyrrhizin-treated human peripheral lymphocytes in response to concanavalin A and to surface antigen of hepatitis B virus[J].Proceedings of the Society for Experimental Biology and Medicine,1986,181(2):205-210.
[22] 邰佳,马海英.金银花制剂的抗病毒作用研究进展[J].中国中医药现代远程教育,2022,20(14):200-203.
[23] 刘占悝,李智杰,刘泽余,等.中药金银花体外抗牛病毒性腹泻病毒的作用研究[J].黑龙江畜牧兽医,2020(14):116-120,154-155.
[24] 石俊英,郭承军.金银花体外抗流感病毒有效部位研究[J].山东中医药大学学报,2010,34(2):178-180.
[25] 张黔东,毕文文,张芸,等.金银花对鸭瘟病毒感染鸭免疫器官功能影响的研究[J].中国预防兽医学报,2022,44(11):1216-1223.
[26] 谢骏辉,陈潇飞,王国贵,等.转录组测序技术的发展及其在畜禽养殖中的应用[J].中国畜牧杂志,2023,59(10):103-110.
[27] 敬云鸿,朱康平,王红梅,等.公猪胚胎期和成年期睾丸组织转录组差异分析[J].中国畜牧杂志,2023,59(8):283-292.
[28] 贾燕青,仇薪鑫,张蓉,等.IFI35介导细胞凋亡抑制新城疫病毒增殖的分子机制研究[J].西北农业学报,2022,31(10):1250-1257.
[29] 郭良兴,聂芙蓉,黄安群,等.基于转录组测序的新城疫疫苗免疫鸡胸腺差异表达基因分析[J].中国家禽,2021,43(12):14-20.
[30] 陈曦,刘通,白潜,等.新城疫疫苗免疫武定鸡和霞烟鸡的外周血淋巴细胞转录组分析[J].中国家禽,2022,44(7):43-49.
[31] 陈卿. 基因Ⅶ型新城疫病毒感染鸡脾脏的免疫应答特征与细胞嗜性研究[D].扬州:扬州大学,2022.
[32] 薄一丹. NDV感染CEF细胞后转录组学分析以及La Sota株感染性克隆的构建[D].保定:河北农业大学,2022.
[33] 曾德平,陆颖,余科辰,等.猪流行性腹泻病毒感染仔猪空肠组织的转录组学分析[J/OL].中国动物传染病学报:1-9[2024-04-15].https://doi.org/10.19958/j.cnki.cn31-2031/s.20230206.003.