Efficacy of E2-sub-unit marker and C-strain vaccines in reducing horizontal transmission of classical swine fever virus in weaner pigs

At present, two types of vaccines against classical swine fever (CSF) virus are commercially available: E2 sub-unit marker vaccines and the conventional attenuated live C-strain vaccines. To evaluate the reduction of the horizontal virus transmission, three comparable experiments were carried out in which groups of weaner pigs (vaccinated with a marker vaccine or a C-strain vaccine) were challenged with CSF virus at 0, 7, and 14 days post-vaccination (dpv). Virus transmission was prevented totally when the challenge occurred at 14 dpv with an E2-marker vaccine (0/12 contact pigs positive in virus isolation (VI); R = 0 (0; 1.5)). At 7 dpv, transmission was reduced slightly (5/12 contact pigs positive in VI; R = 1.0 (0.3; 3.0)), whereas at 0 dpv, vaccination had no effect on transmission (10/12 contact pigs positive in VI; R = 2.9 (1.5; 10.8)). In the C-strain-vaccinated pigs, no virus transmission was detected even when the challenge was performed at the same day as the vaccination (0/12 contact pigs positive in VI; R = 0 (0; 1.5)).     

Comparison of two real-time RT-PCR assays for differentiation of C-strain vaccinated from classical swine fever infected pigs and wild boars

Classical swine fever is one of the most important infectious diseases for the pig industry worldwide due to its economic impact. Vaccination is an effective means to control disease, however within the EU its regular use is banned owing to the inability to differentiate infected and vaccinated animals, the so called DIVA principle. This inability complicates monitoring of disease and stops international trade thereby limiting use of the vaccine in many regions. The C-strain vaccine is safe to use and gives good protection. It is licensed for emergency vaccination in the EU in event of an outbreak. Two genetic assays that can distinguish between wild type virus and C-strain vaccines have recently been developed. Here the results from a comparison of these two real-time RT-PCR assays in an interlaboratory exercise are presented. Both assays showed similar performance.     

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。     

猪瘟兔化弱毒疫苗株基因组的遗传变异分析

参照已发表的猪瘟病毒基因组序列设计了9对引物，用RT-PCR从猪瘟兔化弱毒疫苗株细胞培养物中扩增得到了覆盖猪瘟病毒基因组全长的9个cDNA片段，将所得cDNA片段分别克隆至pMD18-T载体中，经测序和拼接后，获得了猪瘟兔化弱毒疫苗株基因组全序列。序列分析表明，猪瘟兔化弱毒疫苗株基因组全长12310个碱基，其5’非编码区（5＇-NCR）和3＇-NCR分别由373和239个碱基组成，在3’末端有富含T的碱基插入，其间为1个大的开放阅读框架，编码3898个氨基酸残基的多聚蛋白，与国内外已发表的另外7个猪瘟兔化弱毒疫苗株基因组全序列相比，核苷酸同源性为98．7％～99．9％，氨基酸同源性为98．6％～99．9％。基因组全序列比较显示，猪瘟兔化弱毒疫苗株基因组在遗传上相当稳定。     

A promising multiple-epitope recombinant vaccine against classical swine fever virus

Classical swine fever (CSF) is a highly contagious and often fatal disease of swine. It is caused by classical swine fever virus (CSFV), one of the members of the genus Pestivirus of the Flaviviridae family. The development of a safe and effective vaccine against the CSF is critical to pandemic control, this article shows a tandem-repeat multiple-epitope recombinant vaccine can protect pigs from CSFV challenge. That was composed as following: two copies each of glycoprotein E2 residues 693–707, 241–276 and 770–781, and two copies amino acid residues 1446–1460 of the non-structural protein NS2-3. In the challenge test, all of the swine vaccinated with Chinese vaccine strain (C-strain) were fully protected from a challenge with CSFV. However, after three successive vaccinations with the multiple-epitope recombinant vaccine, three out of five pigs were protected from challenge with CSFV (in terms of both clinical signs and viremia). These results demonstrate that multiple-epitope recombinant vaccine which carrying the major CSFV epitopes can induce a high level of epitope-specific antibodies and exhibit a protective capability that parallels induced by C-strain to a certain extent.     

猪瘟病毒荧光定量RT—PCR检测方法的建立及其初步应用

针对CSFV基因组5＇端非编码区序列设计并合成了高度特异的一对引物和一条探针,用于猪瘟病毒实时荧光定量PCR检测方法的建立。将提取的病毒的总RNA做为模板进行反转录和PCR,将PCR产物克隆到pMDl8-T载体后进行大肠杆菌转化,提取阳性质粒做为标准品绘制标准曲线,成功地建立了特异性检测CSFV的荧光定量RT-PCR方...     

猪瘟病毒及其致病机制研究进展

猪瘟(CSF)是猪的一种高度接触性传染病,该传染病可分为急性、亚急性、慢性、非典型性和不明显型.急性CSF由强毒株引发,一般导致高发病率和死亡率,而弱毒病毒感染则表现不明显.由于疫苗的广泛应用,有效地控制了猪瘟的大流行,减少了急性死亡.但从20世纪80年代以后,临床症状不典型且病程变长的非典型性猪瘟(或慢性猪瘟)成为该病的主要发生形式,持续感染普遍存在,疫苗的预防效果明显下降,使猪瘟防制遇到了新的困难.以目前人类对猪瘟的认识水平,尚难以从分子水平解释这一新变化的成因,这是因为对猪瘟病毒致病机理及其分子基础的认识深度不够.就此,文章综述了猪瘟及猪瘟病毒研究进展,主要涉及CSFV生物学特性、致病机制及其防控,希望能为猪瘟防控提供新的思路和对策.     

猪瘟疫苗中牛病毒性腹泻病毒2型的检测

为对上海某猪场送检的一份猪瘟疫苗进行牛病毒性腹泻病毒(BVDV)检测,本研究将猪瘟疫苗样品接种于MDBK细胞,盲传15代后仍无致细胞病变效应,但间接免疫荧光试验表明接种该疫苗后的MDBK细胞能够被单克隆抗体BZ-53(BVDV-2)识别。采用BVDV-1和BVDV-2的5’-UTR的通用检测引物和针对BVDV E2的引物,对样品RNA进行RT-PCR检测,结果显示,样品能够扩增出约288 bp的BVDV特异性片段;此外,5’-UTR和E2基因片段的测序分析结果表明分离株属于BVDV-2,并且其E2基因与牛源XJ-04株(BVDV-2)的E2基因同源性最高(92.3%),而与猪源ZM-95株(BVDV-1)的E2基因同源性较低(64.5%)。由此证明,该猪瘟疫苗中的确污染有一株BVDV-2株。     

Comparison of antibody values in sera of pigs vaccinated with a subunit or an attenuated vaccine against classical swine fever

Ten pigs, aged 85 days, were vaccinated with a subunit vaccine containing 32 g of classical swine fever virus glycoprotein E2 (gp E2) (group 1), and a further 10 pigs were vaccinated with a C strain vaccine (10^4±0.15 TCID₅₀/ml), produced by amplification in minipig kidney (MPK) cell culture (group 2). Nine non-vaccinated pigs served as a control group (group 3). Serum samples were collected before (day 0) and at 4, 10, 21 and 28 days after vaccination and were analysed by two commercially available enzyme immunoassays and by a neutralizing peroxidase-linked assay (NPLA). At the same times, peripheral blood was taken for determining the total leukocyte count and the body temperature was taken daily. Antibodies were not detected in serum samples collected before vaccination (day 0), and no side-effects that could be connected with vaccination were observed during the trial. Ten days after vaccination 6/10 pigs vaccinated with the subunit vaccine were seropositive. On days 21 and 28, the ratios of serologically positive to vaccinated pigs were 9/10 and 10/10, respectively. Four of the ten pigs that were vaccinated with the C strain vaccine were positive on day 21 and 9/10 on day 28. However, the results of the NPLA showed that only 4/10 pigs had an antibody titre >1:32 at the end of the trial in both the vaccinated groups, even though the subunit vaccine initiated an earlier and higher level of neutralizing antibodies than the vaccine produced from the C strain. Challenge was performed 28 days after vaccination on four randomly selected pigs from both vaccinated groups. The pigs survived the challenge without showing any clinical signs of classical swine fever (CSF), while two nonvaccinated control pigs died on the 10th and 12th days after infection.     

泉州市洛江区猪瘟抗体水平检测效果分析

结合实验室每年的检测工作,2013-2014年对洛江区辖区内20个生猪规模养殖场和89个散养户的856份猪血清进行猪瘟疫苗免疫抗体检测。结果表明:洛江区猪瘟疫苗免疫抗体合格率呈现上升趋势,规模场猪瘟疫苗免疫抗体合格率明显高于散养户,免疫2次的抗体合格率明显高于1次。抗体检测工作的开展,对制定科学合理的免疫程序,有效防控猪瘟疫情的发生发挥了积极的作用。     

Factors critical for successful vaccination against classical swine fever in endemic areas

Classical swine fever (CSF) or hog cholera, caused by the classical swine fever virus (CSFV), is one of the most important viral diseases that cause serious economic loss to the swine industry worldwide. During the past 5 years, several techniques for measuring porcine cell-mediated immunity (CMI) were applied, in conjunction with other conventional techniques, to study factors that influence the induction of CSFV-specific immunity. Information, obtained from a series of experiments, demonstrated cell-mediated immune responses in providing protective immunity against CSF infection. Although it has been confirmed that commercially available modified live CSF vaccines are able to induce complete protection in vaccinated pigs, several factors including maternal immunity, the age of primary vaccination, vaccination protocol and complications caused by other pathogens, can greatly affect the effectiveness of CSF vaccines in the field.     

A multiplex RT-PCR assay for the rapid and differential diagnosis of classical swine fever and other pestivirus infections

Classical swine fever is a highly contagious viral disease causing severe economic losses in pig production almost worldwide. All pestivirus species can infect pigs, therefore accurate and rapid pestivirus detection and differentiation is of great importance to assure control measures in swine farming. Here we describe the development and evaluation of a novel multiplex, highly sensitive and specific RT-PCR for the simultaneous detection and rapid differentiation between CSFV and other pestivirus infections in swine. The universal and differential detection was based on primers designed to amplify a fragment of the 5′ non-coding genome region for the detection of pestiviruses and a fragment of the NS5B gene for the detection of classical swine fever virus. The assay proved to be specific when different pestivirus strains from swine and ruminants were evaluated. The analytical sensitivity was estimated to be as little as 0.89 TCID₅₀. The assay analysis of 30 tissue homogenate samples from naturally infected and non-CSF infected animals and 40 standard serum samples evaluated as part of two European Inter-laboratory Comparison Tests conducted by the European Community Reference Laboratory, Hanover, Germany proved that the multiplex RT-PCR method provides a rapid, highly sensitive, and cost-effective laboratory diagnosis for classical swine fever and other pestivirus infections in swine.     

CSFV的RT-PCR检测在控制与净化猪瘟中的应用

应用反转录-聚合酶链反应(RT-PCR)检测健康猪扁桃体猪瘟病毒以监控与净化猪瘟.2006年用RT-PCR对广西某存栏250头种猪场的母猪扁桃体连续进行3次猪瘟病毒检测,检出并清除带毒猪,猪群中猪瘟病毒的带毒猪明显下降.结果表明,RT-PCR检测猪扁桃体可应用于猪场猪瘟的控制与净化.     

应用套式RT—PCR检测猪瘟制品中牛病毒性腹泻病毒污染的研究

为建立猪瘟制品中牛病毒性腹泻病毒（BVDV）污染的诊断方法,本研究根据GenBank公布的BVDV全基因组序列,选择BVDV保守性比较高的5′非编码区,利用Olig06．0软件设计了2对特异性引物,建立了检测BVDV的套式RT-PCR方法。该方法极大提高了常规RT-PCR检测方法的特异性和敏感性,重复性好、特异性强、敏感性高,可以准确快速检测出极低含量的BVDV,为动物与疫苗生物制品原辅料中BVDV的快速低含量检测提供了一种简单、特异、敏感、快速的检测方法。     

一种猪瘟兔化弱毒活疫苗效力检验方法的研究

现有猪瘟活疫苗的效力检验多采用兔体定型热反应法(RID),但该方法存在重复性差、检验周期长、数据不精确等缺点,为克服兔体定型热反应法存在的缺陷,本研究建立了一种快速、准确、稳定的检测猪瘟病毒含量及疫苗效力的间接免疫荧光方法(IFA),该方法以出现特异性荧光作为检测标准,通过添加促细胞感染剂PB增加特异性荧光数量,可以在4d内检测出猪瘟活疫苗成品或半成品病毒含量,该方法检验周期短、数据精确、重复性好,为猪瘟活疫苗效力检验方法的完善提供了有力支持。     

猪瘟病毒的分离鉴定及其E2基因序列分析

2004~2005年上海和江苏3家猪场发生仔猪急性死亡,用ELISA鉴别试剂盒证明为猪瘟感染。用PK15细胞分离病毒,传代至第3代无细胞病变,RT-PCR扩增E2基因为阳性,扩增片段经纯化后克隆入T载体并进行序列测定。通过DNAStar软件对3株病毒的基因序列进行了比较,同时构建了系统进化树,结果表明,三株病毒分离株均扩增出269bp片段并且核苷酸序列100%同源,这3株与Alfort、Shimen株、兔化弱毒株(HCLV)和Brescia4个标准毒株核苷酸序列同源性均在90%以上,说明在江苏、上海地区分离得到的3株猪瘟病毒与流行毒株在基因序列上没有发生大的变异。     

猪全血溶血对猪瘟抗体检测的影响

为研究猪全血溶血是否对猪瘟抗体效价产生影响,在明溪县某规模养殖场选择注射过2次猪瘟疫苗的肉猪20头,抽取全血各2份,共40份,相同条件保存,使其中1份溶血。将进行溶血处理和未处理的全血离心出的血清进行物理性状观察和ELISA检测,并对检测的OD值进行比较分析。结果发现,是否溶血对ELISA检测的OD值无统计学差异,表明短期内只要保存得当,是否溶血不会造成猪瘟抗体效价的显著降低。     

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.