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建立猪繁殖与呼吸综合征病毒(Porcine reproductive and respiratory syndrome virus,PRRSV)环介导间接PCR检测方法,用于该病毒的感染检测和高致病性毒株与低致病性毒株的鉴别诊断。根据GenBank数据库中PRRSV中国流行株ORF7和ORF1a基因序列的保守性,设计2对特异性探针,分别标记于大豆Lectin基因两端,作为报告基因,经过一步链置换反应后,采用反向PCR扩增报告基因,建立PRRSV环介导间接PCR检测方法,该方法扩增HP-PRRSV可得大小为193bp和355bp的特异片段,扩增LP-PRRSV可得大小为193bp和442bp的特异片段。试验结果表明,该方法能成功鉴别HP/LP-PRRSV,可检测出5.6TCID50/mL LP-PRRSV和18TCID50/mL HP-PRRSV的病毒RNA,HP/LP-PRRSV混合感染不影响检测灵敏度,与CSFV、PPV、PRV、PCV2、ETEC和Haemophilus parasui等常见猪源性病原的检测无明显交叉反应;对20份临床样本进行比较检测,环介导间接PCR检测出14份PRRSV阳性样本,其中4份LP-PRRSV、9份HP-PRRSV和1份LP/HP-PRRSV,与常规PCR检测结果一致。环介导间接PCR是一种简便快速、灵敏、特异的病原学诊断工具,适合PRRSV感染的快速检测和HP/LP-PRRSV鉴别诊断,尤其适合HP/LP-PRRSV混合感染的鉴别。
Abstract:The aim of this study is to establish the method of loop-mediated indirect PCR assay for detection of Reproductive and Respiratory Syndrome Virus(PRRSV) infection and differentiation of highly pathogenic PRRSV(HP-PRRSV) and lowly pathogenic PRRSV(LP-PRRSV).Based on the alignments of ORF2 gene sequences and ORF1a gene sequences of PRRSV Chinese isolates deposited in GenBank,two pairs of specific probes were designed and labeled to both ends of the soybean Lectin gene fragment by PCR,respectively.The probe-labeled soybean Lectin genes were used to be reporter genes for detection and differentiation of PRRSV.After one round strand displacement reaction,the reporter genes were amplified by reverse PCR.The specific PCR products were 193bp,355bp for HP-PRRSV and 193bp,442bp for LP-PRRSV,respectively.The method could detect 5.6 TCID50/mL LP-PRRSV RNA and 18 TCID50/mL HP-PRRSV RNA,and co-infection did not affect detection sensitivity.No amplification was observed with other porcine originated pathogens including CSFV,PPV,PRV,PCV2,ETEC and Haemophilus parasui.Twenty clinical samples were used for comparative testing with conventional PCR.Fourteen samples were found positive for PRRSV by the loop-mediated indirect PCR,of which 4 were LP-PRRSV,9 HP-PRRSV and 1 LP/HP-PRRSV co-infection,consistent with the conventional PCR test results.In conclusion,the loop-mediated indirect PCR is a simple,rapid,sensitive and specific etiologic diagnosis tool,and suitable for the differential diagnosis of HP/LP-PRRSV,especially for identification of mixed infection of HP/LP-PRRSV.
[1]Dwivedi V,Manickam C,Binjawadagi B,et al.Evalua-tion of immune responses to porcine reproductive and re-spiratory syndrome virus in pigs during early stage of in-fection under farm conditions[J].Virol J,2012,9:45-53.
[2]Lopez O J,Oliveira M F,Garcia E A,et al.Protectionagainst porcine reproductive and respiratory syndromevirus(PRRSV)infection through passive transfer ofPRRSV-neutralizing antibodies is dose dependent[J].Clin Vaccine Immunol,2007,14(3):269-275.
[3]An T Q,Tian Z J,Leng C L,et al.Highly PathogenicPorcine Reproductive and Respiratory Syndrome Virus,Asia[J].Emerg Infect Dis,2011,17(9):1782-1784.
[4]Guo A,Wu G,Gong W,et al.Outbreaks of highlypathogenic porcine reproductive and respiratory syn-drome in Jiangxi province,China[J].Ir Vet J,2012,65(1):14-22.
[5]Wu J,Li J,Tian F,et al.Genetic variation and patho-genicity of highly virulent porcine reproductive and re-spiratory syndrome virus emerging in China[J].ArchVirol,2009,154(10):1589-1597.
[6]Hu H,Li X,Zhang Z,et al.Porcine reproductive andrespiratory syndrome viruses predominant in southeast-ern China from 2004to 2007were from a common sourceand underwent further divergence[J].Arch Virol,2009,154(3):391-398.
[7]王仕荣,向晖,吴健敏,等.广西“猪高热综合征”主要病原调查及PRRSV Nsp2基因变异分析[J].中国兽医学报,2009,29(03):249-253.
[8]郭杨,林华,郭宇飞,等.高致病性PRRSV SC-JX01株Nsp2基因的序列分析和抗原表位预测[J].中国兽医杂志,2010,46(04):10-13.
[9]Benson J E,Yaeger M J,Christopher-Hennings J,etal.A comparison of virus isolation,immunohistochem-istry,fetal serology,and reverse-transcription polymer-ase chain reaction assay for the identification of porcinereproductive and respiratory syndrome virus transplacen-tal infection in the fetus[J].J Vet Diagn Invest,2002,14(1):8-14.
[10]肖跃强,管宇,唐娜,等.PRRSV经典与高致病性毒株RT-PCR鉴别检测方法的建立[J].中国兽医学报,2010,30(07):873-877.
[11]Chen Y,Tian H,He J H,et al.Indirect ELISA withrecombinant GP5for detecting antibodies to porcine re-productive and respiratory syndrome virus[J].VirolSin,2011,26(1):61-66.
[12]Giammarioli M,Pellegrini C,Casciari C,et al.Devel-opment of a novel hot-start multiplex PCR for simulta-neous detection of classical swine fever virus,Africanswine fever virus,porcine circovirus type 2,porcinereproductive and respiratory syndrome virus and por-cine parvovirus[J].Vet Res Commun,2008,32(3):255-262.
[13]Risatti G,Holinka L,Lu Z,et al.Diagnostic evalua-tion of a real-time reverse transcriptase PCR assay fordetection of classical swine fever virus[J].J Clin Mi-crobiol,2005,43(1):468-471.
[14]Zhao K,Han F,Zou Y,et al.Rapid detection of por-cine circovirus type 2using a TaqMan-based real-timePCR[J].Virol J,2010,7(1):374-378.
[15]刘忠华,余兴龙,李润成,等.高致病性猪繁殖与呼吸综合征病RT-PCR快速鉴别诊断方法的建立与临床应用[J].微生物学通报,2008,35(8):1268-1272.
[16]柴政,李曦,王小武,等.PRRSV高致病性毒株和经典毒株SYBR GreenⅠ实时荧光PCR鉴别方法的建立[J].中国兽医科学,2009,39(02):140-144.
[17]Wernike K,Hoffmann B,Dauber M,et al.Detectionand typing of highly pathogenic porcine reproductiveand respiratory syndrome virus by multiplex real-timeRT-PCR[J].PLoS One,2012,7(6):e38251.
[18]王永芬,郑鸣,边传周.环介导间接PCR检测方法的建立[J].生物技术通报.2012,8:130-134.
[19]郑鸣,边传周,王老七.建立环介导间接PCR同时检测3种主要猪源性病毒[J].中国农业科学,2011,44(21):4499-4507.
[20]郑鸣,边传周,刘仲敏.Chelex法结合环介导间接聚合酶链式反应检测肉制品单增李斯特菌[J].食品科学,2012,33(10):190-194.
[21]李玉峰,王先炜,陈闻,等.猪繁殖与呼吸综合征病毒nsp2基因缺失株RT-PCR检测方法的建立[J].南京农业大学学报,2009,32(3):169-171.
[22]郝晓芳,周艳君,田志军,等.高致病性猪繁殖与呼吸综合征病毒RT-PCR鉴别诊断方法的建立[J].中国预防兽医学报,2007,29(9):704-709.
基本信息:
DOI:10.13242/j.cnki.bingduxuebao.002402
中图分类号:S858.28
引用信息:
[1]郑鸣,李华玮,边传周,等.环介导间接PCR鉴别高、低致病性猪繁殖与呼吸综合征病毒方法的建立[J].病毒学报,2013,29(04):364-370.DOI:10.13242/j.cnki.bingduxuebao.002402.
基金信息:
河南省重点科技攻关项目(092102110073)
2013-06-20
2013-06-20
2013-06-20