单克隆抗体捕捉猪瘟病毒抗原ELISA方法的建立

分别用原核表达的猪瘟病毒（CSFV）主要抗原E2蛋白和猪瘟基因疫苗免疫BALB/c小鼠,通过细胞融合与克隆筛选出5株稳定分泌CSFV抗体的杂交瘤细胞株1E2、1G7、3A2、3B7和4B6.间接免疫荧光和Western-blotting试验结果表明,5株单抗均与CSFV E2蛋白和全病毒抗原反应.将筛选的CSFV特异性单抗1E2、3B7和4B6纯化后等量混合后包被酶标板（捕捉抗体）,与兔抗CSFV IgG（检测抗体）联合应用,建立起CSFV抗原捕捉ELISA（AC-ELISA）方法.随后采用方阵滴定法确定了单抗与多抗的最适工作浓度及判定检测结果的OD450临界值.最后以建立的AC-ELISA检测CSFV细胞培养物、CSFV攻毒死亡猪的病料和临床猪瘟组织样品,结果表明,该方法敏感、特异、重复性好,与病毒分离和RT-PCR方法符合率分别为86.2%和90.3%.     

某规模化猪场伪狂犬病的诊断

河南平顶山某猪场母猪出现较严重的流产和产死胎现象,且50日龄~70日龄仔猪出现神经症状,根据临床表现初步诊断为伪狂犬病。为排除猪繁殖与呼吸综合征和猪瘟,进行了实验室诊断。应用ELISA方法检测发病保育猪及母猪血清的伪狂犬病病毒野毒株gE抗体,并对发病仔猪病料进行了伪狂犬病病毒(PRV)、猪繁殖与呼吸综合征病毒(PRRSV)和猪瘟病毒(CSFV)的实时荧光定量PCR检测。结果显示,伪狂犬病病毒野毒抗体阳性,实时荧光定量PCR检测确定仔猪病料中PRV核酸阳性,PRRSV和CSFV核酸阴性。结合临床症状及实验室检测,确诊该猪场发生的是猪伪狂犬病。     

猪瘟病毒RT-PCR核酸检测与ELISA抗原检测试验应用研究

本试验根据NCBI公布的猪瘟病毒石门毒株E2基因序列,设计、合成了1对检测猪瘟病毒E2基因的PCR引物。以120份疑似猪瘟病料为试验材料,使用RT-PCR核酸检测与ELISA抗原检测2种方法,分别用这2种方法检测疑似病料,并且比较这2种方法在猪瘟病料检测中的实际差别。通过猪瘟病毒RT-PCR核酸检测结果及ELISA抗原检测结果相互印证,为云南猪瘟的诊断及防制提供了技术支持。     

Evaluation of a multiplex real-time RT-PCR for quantitative and differential detection of wild-type viruses and C-strain vaccine of Classical swine fever virus

Classical swine fever virus (CSFV) is the causative agent of classical swine fever (CSF), one of OIE listed diseases. Most of the currently available detection methods do not allow discrimination between wild-type CSF viruses and the vaccine strains. This study was designed to develop a multiplex real-time RT-PCR for the quantitative and differential detection of wild-type viruses and C-strain vaccine widely used in China. CSFV specific primers and two differently labeled TaqMan probes for the differentiation of wild-type viruses from C-strain vaccine were designed in the 5'-untranslated region of the viral genome of CSFV. The two TaqMan probes specifically hybridize wild-type viruses of different subgroups and C-strain vaccine, respectively, in the multiplex real-time RT-PCR, with no cross-reaction to a number of non-CSFV porcine viruses. The sensitivity of the assay for detecting wild-type and C-strain-type vaccine viruses was determined to be 41.8 and 81.5copies/microL viral RNA, respectively. Completely correct differentiation of wild-type viruses from C-strain vaccine was achieved when testing reference strains and characterized field isolates of CSFV in China. The multiplex real-time RT-PCR was able to detect the viral RNA in the whole blood samples of experimentally infected pigs as early as 2 days post-infection, 3 to 4 days prior to the onset of clinical signs in co-housed pigs. The agreements between the multiplex real-time RT-PCR and a multiplex RT-nested PCR for detection of wild-type and C-strain-type viruses were 96.9% and 100%, respectively, when detecting 106 different field samples. There is a positive correlation between the titers of C-strain vaccines titrated in rabbits and RNA copies quantitated by the multiplex real-time RT-PCR. The novel assay described here is rapid and sensitive, and is useful for differentiating field strains and C-strain of CSFV in China.     

猪瘟疫苗在猪圆环病毒2型阳性猪场的免疫效果观察

为了研究猪圆环病毒2型(PCV-2)感染对猪瘟疫苗免疫效力的影响,对PCR证实为PCV-2阳性的试验猪进行猪瘟疫苗的免疫,分别在免疫后第1、3、7、14、21、28和63天对试验猪进行猪瘟病毒(CSFV)和PCV-2的抗体检测。检测结果表明PCV-2阳性猪在猪瘟疫苗免疫后均未能产生有效的CSFV抗体,从免疫猪的血液和内脏组织中也未能检测到CSFV核酸。虽然只能从1头PCV-2阳性猪的血清中检测到PCV-2抗体,但是却能从全部实验猪的淋巴结中检测到PCV-2的核酸。试验猪的病理组织学观察和白细胞计数也表明PCV-2阳性猪的淋巴结呈典型的PCV-2感染的病理变化,且白细胞数量显著低于健康猪。表明PCV-2的感染会对猪的免疫系统造成损害从而抑制猪瘟疫苗的免疫效果。     

猪捷申病毒TaqMan实时定量RT-PCR方法的建立

为建立猪捷申病毒(PTV)的早期检测及定量分析方法,本研究基于PTV 11个血清型基因组5′端非编码区保守序列,设计引物和TaqMan探针,建立了检测PTV的TaqMan实时定量RT-PCR方法.应用该方法对PTV、猪细小病毒、猪繁殖与呼吸综合症病毒、猪圆环病毒2型、猪伪狂犬病毒以及猪瘟病毒进行特异性试验,结果除PTV为阳性外其它均为阴性;针对PTV最低可检测到10个拷贝;批内、批间重复试验的变异系数均小于3％.应用建立的方法与病毒分离方法分别对91份临床样品进行检测,检出率分别为79.12％和57.14％,两者的符合率是78.02％.经临床应用表明,该实时定量RT-PCR方法可为PTV的早期诊断及定量分析提供技术手段.     

用RT-PCR技术检测盐渍猪肠衣中猪瘟病毒的研究

参考GenBank中发表的猪瘟病毒（CSFV）序列，设计一对CSFV特异性PCR引物；从CSFV感染猪盐渍小肠中提取总RNA，经逆转录后进行PCR扩增，在盐渍小肠中成功扩增出与预期大小（168bp）一致的特异性条带，而正常猪和感染猪伪狂犬病病毒的猪小肠扩增结果均为阴性。用本方法对20例不同稀释浓度的盐渍猪肠衣样本进行检测，结果显示比经典抗原检测方法（抗原捕获ELISA法）具有更高的敏感性。实验表明，本RT—PCR技术能应用于盐渍猪肠衣的CSFV检测，为快速、准确检测盐渍猪肠衣中CSFV提供了一条新途径。     

猪瘟诊断方法的研究进展

猪瘟是由猪瘟病毒引起的一种急性、发热性、接触性传染病,可引起各种年龄猪发病。随着对猪瘟病毒研究的深入,猪瘟在一定程度上得到了有效控制。但是近年来,世界各国流行的猪瘟在流行病学、临床症状和病理变化等方面出现了一些新的变化,猪瘟的防控出现了许多新的情况。我国猪瘟的发病率亦呈上升趋势,严重威胁着我国养猪业的发展,给养猪业造成了极大的经济损失。因此,建立准确的实验室诊断方法,对于预防和控制猪瘟有重要意义。本文综述了猪瘟诊断技术方面的研究进展,为猪瘟的及时诊断提供参考。     

Laboratory decision-making during the classical swine fever epidemic of 1997-1998 in The Netherlands

The National Reference Laboratory for classical swine fever (CSF) virus in the Netherlands examined more than two million samples for CSF virus or serum antibody during the CSF epizootic of 1997–1998. The immense amount of samples and the prevalence of border disease (BD) virus and bovine viral diarrhoea (BVD) virus infections in Dutch pig herds necessitated the diagnostic efforts of the laboratory to be focused on generating CSF specific test results throughout the eradication campaign.

Detection of 82% of the 429 outbreaks was achieved through the combined use of a direct immunofluorescence and peroxidase assay (FAT/IPA) with samples (tonsils) collected from clinically-suspected pigs. This suggests that in the majority of the outbreaks, the pigs had clinical signs that were recognised by the farmer and/or veterinarians, indicating the presence of CSF virus in a pig herd. A positive diagnosis of 74% of all the tissue samples (tonsils) collected at infected pig holdings was established by FAT. More than 140,000 heparinised blood samples were examined by virus isolation, resulting in the detection of 4.5% of the infected herds. CSF virus was isolated in approximately 29% of all the blood samples collected from pigs at infected or suspected farms.

Several serological surveys — each done within a different framework — led to the detection of 13.5% of the total number of outbreaks. The detection of CSF virus antibody in serum was carried out by semi-automated blocking ELISA. Approximately 28.5% of the sera which reacted in the ELISA were classified as CSF virus-neutralising antibody positive and 26.5% as positive for other pestiviruses following the virus neutralisation test (VNT).

We concluded that two of the CSF laboratory diagnostic methods described were determinative in the eradication campaign: first, the FAT for the screening of diseased pigs; and second, the ELISA and VNT when millions of predominantly healthy pigs needed to be screened for the presence of CSF serum antibody. Decision-making on the basis of results generated by either method can, however, be seriously hindered when samples are examined from pig herds with a high prevalence of non-CSF pestiviruses.     

上海地区规模化猪场牛病毒性腹泻病毒感染状况的血清学调查

为调查猪瘟疫苗是否会引起牛病毒性腹泻的发生及上海地区规模化猪场该病的流行情况,本试验采用酶联免疫吸附试验方法,对分别免疫接种3种猪瘟疫苗的57头试验猪以及上海地区2005年-2009年10个区(县)共740份血清进行了牛病毒性腹泻病毒(BVDV)抗原和抗体的检测.经检测,所有样品抗原和抗体均为阴性.结果表明,免疫猪瘟脾...     

某猪场猪瘟免疫程序的调整及免疫效果评价

为了更好地预防和控制猪瘟,找出适合四川某猪场的猪瘟免疫程序,笔者根据实际情况对免疫程序进行了调整。然后用ELISA和IHA法对免疫程序调整前后的不同日龄猪血清进行了抗体检测,结果显示:调整前用ELISA法检测到3日龄、25日龄、50日龄、90日龄和120日龄猪只的猪瘟抗体阳性率分别为80%、54.54%、77.78%、80%和95%,用IHA法测得的阳性率分别为100%、63.64%、77.78%、90%和95%;调整后用ELISA法测得的猪瘟抗体阳性率分别为100%、80%、77.27%、77.78%和95%,用正向IHA法测得的抗体阳性率分别为97.73%、94.44%、96.15%、100%和100%。调整前用ELISA和IHA测得的平均阳性率为77.46%、85.28%,调整后则变为86.01%、97.66%,虽然均符合农业部颁布的猪群猪瘟抗体阳性率应不低于70%的标准,但免疫程序调整后的抗体阳性率明显高于调整前,可见调整后的免疫程序更适合于该猪场。     

Development and evaluation of a novel antigen capture assay for the detection of classical swine fever virus antigens

An antigen-capture enzyme immunoassay (EIA) was developed to detect classical swine fever virus (CSFV) antigen directly from 10% w/v tissue suspension. The assay, based on the sandwich principle, uses a biotinylated monoclonal antibody bound to streptavidin-coated microplates as the capture system and a swine anti-CSFV antibody and rabbit anti-swine HRPO-conjugate as the detector system. The antigen-capture EIA was compared with conventional virus isolation and polymerase chain reaction (PCR) for detection of CSFV in tissues. The ability of the antigen-capture EIA to discriminate classical swine fever (CSF) from bovine viral diarrhea and African swine fever viruses was also tested. The assay was shown to detect 21 different strains of CSFV and was unreactive with tissues from uninfected animals. Signal to noise (S/N) ratios were calculated from the EIA absorbance values. Readings from samples positive by virus isolation (n=47) averaged a S/N ratio of 5.34. In contrast, samples negative by virus isolation (n=96) demonstrated a mean S/N ratio of 0.16. At S/N cut-off value of 1.0, all samples that yield virus isolation and PCR negative result were negative in the antigen-capture EIA. Compared with virus propagation in tissue culture using PK15 cells (followed by indirect peroxidase assay detection) and PCR, the EIA had a specificity of 98.7% and a sensitivity of 91.4%. The EIA is simple, can be performed in 4 h and lends itself to automation for screening of tissues sample from pigs suspected of CSFV infection.     

用荧光定量RT-PCR方法检测猪瘟病毒

为了建立能特异检测不同基因型猪瘟病毒(Classical swine fever virus,CSFV),同时又能区分其他瘟病毒的基因检测方法,本实验针对CSFV基因组5′端非编码区设计并合成了简并引物和TaqMan探针,在优化反应条件的基础上,成功地建立了特异检测CSFV的荧光定量RT-PCR检测方法。再以已知滴度的CSFV石门株血毒总RNA反转录产物建立标准品,该标准品可以用于定量临床样品中的CSFV滴度,所建立的荧光定量PCR方法可以灵敏地检测出10~(-0.82)个TCID_(50)病毒含量。最后用建立的方法对108份临床样品进行检测并同时进行病毒分离,荧光定量PCR方法检测出73份阳性样品且与病毒分离的符合率为100%,而常规RT-PCR只检测出54份阳性样品,表明本荧光定量RT-PCR法在检测猪瘟病料上具有潜在的应用价值。