四种常见猪肠道病毒多重RT-PCR检测方法的建立及临床应用  被引量：6

作　　者：辛忠昊 焦安琪 朱彤[1] 刘丽萍 黄兵[1] 于江[2] 郭效珍 吴家强[2] XIN Zhonghao;JIAO Anqi;ZHU Tong;LIU Liping;HUANG Bing;YU Jiang;GUO Xiaozhen;WU Jiaqiang(Key Laboratory of Poultry Disease Diagnosis and Immunity in Shandong Province,Poultry Research Institute,Shandong Academy of Agricultural Sciences,Jinan 250000,Shandong,China;Key Laboratory of Animal and Poultry Disease Control and Breeding,Institute of Animal Science and Veterinary Medicine,Shandong Academy of Agricultural Sciences,Jinan 250000,Shandong,China)

机构地区：[1]山东省农业科学院家禽研究所山东省家禽疫病诊断与免疫重点实验室,山东济南250000 [2]山东省农业科学院畜牧兽医研究所山东省畜禽疫病防治与繁育重点实验室,山东济南250000

出　　处：《微生物学通报》2022年第12期5126-5137,共12页Microbiology China

基　　金：山东省自然科学基金青年项目(ZR2021QC054);山东省重大科技创新工程(2020CXGC010801);山东省现代农业产业技术体系(SDAIT-08-01);山东省农业重大应用技术创新项目(SD2019XM007);高层次人才工程项目。

摘　　要：【背景】猪流行性腹泻病毒(porcine epidemic diarrhea virus,PEDV)、猪传染性胃肠炎病毒(transmissible gastroenteritis virus,TGEV)、猪δ冠状病毒(porcine deltacoronavirus,PDCoV)和猪轮状病毒(porcinerotavirus,PoRV)是当前导致猪群发生病毒性腹泻的4种主要病原,并且常发生混合感染。【目的】建立一种可鉴别诊断这4种腹泻病毒病的检测方法,对于临床诊断具有重要意义。【方法】针对PEDV的M蛋白基因、TGEV的N蛋白基因、PDCoV的N蛋白基因和PoRV的VP7蛋白基因分别设计特异性引物,进而构建相应的重组质粒标准品。通过对PCR反应条件优化,建立可同时检测PEDV、TGEV、PDCoV和PoRV的多重RT-PCR检测方法。随后通过敏感性、特异性和重复性试验对该方法的有效性进行验证。【结果】敏感性试验结果显示,对PEDV-M、TGEV-N、PDCoV-N和PoRV-VP7重组质粒标准品的最低检测下限分别为1.75×10^(2)、1.5×10^(3)、1.6×10^(2)和1.6×10^(2)copies/μL;特异性试验结果显示,仅可检出本研究中的4种靶病毒,而猪群常见病毒CSFV、PRRSV、PCV2和PRV未能检出。重复性试验结果显示,选取10^(8)、10^(6)和10^(4)copies/μL3个不同浓度的重组质粒作为模板,其他条件不变,分别进行5次重复试验,5次试验均扩增出清晰、均匀的条带。对山东各地区送检的52份临床腹泻样品通过建立的四重RT-PCR方法进行检测,发现PEDV、TGEV、PDCoV和PoRV的阳性率分别为37%(19份)、6%(3份)、10%(5份)和25%(13份)。其中PEDV和PoRV混合感染2份(4%),PEDV和TGEV混合感染2份(4%),PEDV和PDCoV混合感染1份(2%)。通过单重RT-PCR对该多重RT-PCR临床样品检测结果进行重复验证,结果显示多重RT-PCR与常规单重RT-PCR结果符合率为100%。最后随机挑选5个检测为阳性的临床样本进行测序验证,结果均为相应病毒的基因片段。【结论】本研究建立了可同时检测PEDV、TGEV、PDCoV和PoRV的四重RT-PCR检测方法,研究结果为临床4[Background]Porcine epidemic diarrhea virus(PEDV),porcine transmissible gastroenteritis virus(TGEV),porcine deltacoronavirus(PDCoV),and porcine rotavirus(PoRV)are the four main pathogens that cause viral diarrhea in pigs and often occur in mixed infections.[Objective]To establish a method for simultaneous detection of the four viruses in clinical practice.[Methods]The specific primers were designed for the M protein gene of PEDV,N protein gene of TGEV,N protein gene of PDCoV,and VP7 protein gene of RoRV,and the corresponding recombinant plasmids were constructed.By optimizing the PCR conditions,a multiplex RT-PCR assay for the simultaneous detection of PEDV,TGEV,PDCoV,and PoRV was successfully established.Further,the sensitivity,specificity,and reproducibility of the established method were evaluated.[Results]The sensitivity test showed that the multiplex RT-PCR assay had the lower limits of detection of 1.75×10^(2),1.5×103,1.6×10^(2)and 1.6×10^(2) copies/μL for PEDV-M,TGEV-N,PDCoV-N,and PoRV-VP7 recombinant plasmid standards,respectively.The results of specificity test showed that only the four target viruses in this study could be detected,while other common porcine viruses such as classical swine fever virus(CSFV),porcine reproductive and respiratory syndrome virus(PRRSV),porcine circovirus type 2(PCV2),and porcine pseudorabies virus(PRV)could not be detected.The five replicate tests with 108,106 and 104 copies/μL of recombinant plasmids as templates and other conditions unchanged all produced clear and uniform bands.The 52 clinical diarrhea samples from various regions in Shandong Province were tested by the established quadruple RT-PCR assay.The results showed that the positive rates of PEDV,TGEV,PDCoV,and PoRV were 37%(19 samples),6%(3 samples),10%(5 samples)and 25%(13 samples),respectively.2(4%),2(4%),and 1(2%)samples showed mixed infections of PEDV and PoRV,mixed infections of PEDV and TGEV,and mixed infections of PEDV and PDCoV,respectively.Further,the results of the multiplex RT-PCR assay were val

关 键 词：多重RT-PCR 猪流行性腹泻病毒 猪传染性胃肠炎病毒 猪δ冠状病毒 猪轮状病毒 

分 类 号：S858.28[农业科学—临床兽医学]