ELISA法检测疫苗中牛血清残留量的适用性研究

为了验证ELISA法对病毒性疫苗中残余牛血清蛋白检测的适用性,用牛血清蛋白ELISA测定法与牛血清白蛋白ELISA测定法、牛血清IgG-ELISA测定法对麻疹疫苗、风疹疫苗、腮腺炎疫苗洗涤前病毒培养液、洗涤后病毒收获液以及多种成品疫苗中的残余牛血清蛋白含量进行了测定。结果显示,麻疹疫苗、风疹疫苗、腮腺炎疫苗洗涤前病毒培养液中牛血清白蛋白含量依次为IgG含量的70.5倍、65倍、84.3倍,洗涤后病毒收获液中两者比值分别为4.2、1.8和8.1;牛血清白蛋白ELISA法和牛血清蛋白ELISA法均能检测出疫苗中牛血清白蛋白,但前者测不出牛血清IgG,而后者可准确检测牛血清IgG。牛血清蛋白ELISA测定法可同时检测牛血清白蛋白和牛血清IgG,更适用于疫苗残余牛血清蛋白含量的测定。     

A comparison of an enzyme-linked immunosorbent assay and counter current electrophoresis for the detection of bovine serum albumin in virus vaccines

A monoclonal antibody directed against bovine serum albumin (BSA) has been developed and used in an enzyme-linked immunosorbent assay (ELISA) system for the detection of BSA in virus vaccines. The results correlated well with those obtained with a counter current electrophoresis system which has been employed routinely for this purpose. The ELISA was slightly more sensitive and more readily applicable to the screening of large numbers of samples but could not be used in the presence of certain stabilizers.     

牛血清蛋白酶联免疫检测试剂盒的研制及验证

为研制酶联免疫试剂盒以检测病毒性疫苗中残余牛血清蛋白(BSP)含量,制备高效价高纯度的兔抗BSP多克隆抗体作为包被抗体和酶标抗体,建立了ELISA双抗体夹心法并组建试剂盒,通过标准剂量曲线可对样品中所含BSP、BSA及B-IgG进行定量,经验证该方法标准曲线线性范围内r≥0.98,对BSP的检测限量为3ng/ml;分别检测5、10、20ng/ml含量的BSP时,试验内(n=12)和试验间(n=3)测定的变异系数在3.71%到7.29%之间,回收率在93.4%~106.3%,未见该方法与人血清白蛋白、卵清蛋白以及疫苗复合保护剂之间有交叉反应。该法敏感度高,准确性、重复性和稳定性好,可用于疫苗牛血清残余蛋白的质量控制。     

Collective experiences of adventitious viruses of animal-derived raw materials and what can be done about them

Contamination of animal-derived raw materials with viruses, mycoplasmas, bacteria and fungi is common. These contaminants can interfere with the diagnosis of viral infection, and vaccines produced using infected cell cultures could lead to seroconversion or disease in the vaccinated animal. The purity, safety and efficacy of viral vaccines requires testing of the ingredients, cell substrates and final product. Methods for detection of viruses, especially bovine viral diarrhea virus, in nutrient serum, cell cultures, seed viruses and viral vaccines, and the frequency of their detection at the Center for Veterinary Biologics are discussed. This revised version was published online in August 2006 with corrections to the Cover Date.     

The development and standardization of an ELISA for ovalbumin determination in influenza vaccines

A double antibody sandwich enzyme-linked immunosorbent assay (ELISA) for the detection of ovalbumin in influenza vaccines has been developed and standardized. Commercially available reagents were used. ELISA was compared to single radial immunodiffusion (SRD) and immunoelectro-osmophoresis (IEOP) techniques. The detection limit by ELISA was 0.5 ng/ml. This method was found to be at least 1000 times more sensitive than SRD and at least 200 times more sensitive than IEOP. It was concluded that ELISA is a specific, sensitive and reproducible method for the determination of the small amounts of ovalbumin found as an impurity in unconcentrated influenza vaccines.     

牛血清蛋白酶联免疫试剂盒性能的验证

为了全面验证研制的牛血清蛋白(BSP)酶联免疫试剂盒的性能,由3个部门6人协作进行了验证。结果表明,,6人进行的18次试验全部满足BSP-ELISA试剂盒的质控标准,达标率100%;6名实验人员对3、4、5、10、20ng/ml浓度的BSP标准品进行测定,结果变异系数在1.96%~6.24%之间,精密度较好;回收率在94.8%~98.7%之间,准确度理想,测量限量为3ng/ml。该试剂盒与人血白蛋白、卵清蛋白等均无交叉反应,对BSA、B-IgG特异性蛋白的检测回收率为101.2%和94.7%;与牛血清白蛋白试剂盒对比测定11种疫苗总计108批,符合率为96.3%,针对不同疫苗,BSP残余量约为BSA的1.12~3.13倍,验证结果表明,该试剂盒可检测疫苗中BSP而不仅是BSA,能更全面客观地反映疫苗中牛血清的真实情况,有利于疫苗生产的严格质量监控。     

检测牛冠状病毒抗体间接ELISA方法的建立与应用

[背景]牛冠状病毒(Bovine coronavirus,BCoV)是引起新生犊牛死亡的主要病原之一,有效的检测手段是防治该病的前提。目前BCoV ELISA检测方法存在敏感性低、不稳定等缺陷。[目的]对原有BCoV ELISA方法进行改进,建立间接ELISA检测方法。[方法]应用我国BCoV流行毒株CD株n基因为模板,预测N蛋白抗原表位,通过原核表达制备可溶性的重组N蛋白作为抗原,建立间接ELISA方法,应用该方法对黑龙江省2010-2017年的BCoV感染进行血清流行病学调查。[结果]该ELISA方法最佳工作条件为:用50 mmol/LpH 9.6碳酸盐作为包被液,抗原包被浓度2.5μg/mL;用PBST作为样本稀释液,稀释浓度1:50,37℃孵育1.5 h;HRP-羊抗牛IgG稀释浓度1:7 500,37℃孵育1.0 h;用1%明胶37℃封闭30 min。阴阳性临界值为0.225。该方法与BRV、BRSV、BVDV、IBRV、BPIV3和E.coli阳性血清均无交叉反应。批内和批间变异系数均小于10%,与病毒中和试验的符合率高达93.5%。对黑龙江省部分地区共603份奶牛血清样品检测结果显示,BCoV抗体阳性率为98.84%。[结论]建立的ELISA方法特异性强、敏感性高、稳定性好,为进一步研发ELISA试剂盒提供了技术基础。     

Enzyme-linked immunosorbent assay for the detection of Fusobacterium necrophorum antibody in bovine sera.

An enzyme-linked immunosorbent assay (ELISA) with HCl heat extracted antigen of Fusobacterium necrophorum was developed for the detection of antibody in bovine sera. Optimal conditions for antigen concentration and dilution of bovine serum were established. Pretreatment of positive reference serum with the antigens of different bacteria demonstrated no decrease, whereas the serum pretreated with F. necrophorum antigens revealed a decrease in the ELISA values. The apparent difference in ELISA values was observed between the sera derived from cattle infected and not infected with Fusobacterium necrophorum. These findings indicate that the ELISA detects the antibody to F. necrophorum in bovine sera.     

Advances in the development of molecular tools for the control of bovine babesiosis in Mexico

The severe negative impact that bovine babesiosis has in the Mexican cattle industry has not been ameliorated basically due to the lack of safe and effective commercially available vaccines and sensitive and reliable diagnostic tests. In recent years, the Bovine Babesiosis Laboratory at the National Center for Disciplinary Research in Veterinary Parasitology-INIFAP in Morelos State, Mexico has been directing efforts towards three main research areas: (1) The development of in vitro culture-derived, improved and safer live vaccines. This has been done in two ways: using gamma-irradiated bovine serum and erythrocytes for the in vitro culture of vaccine strains, which reduces the risk of contaminating pathogens, and improving the immune response, by the addition of L. casei, a strong stimulant of the innate immune system. (2) The study of antigens considered as vaccine candidates with the goal of developing a recombinant vaccine that suits the country's needs. Knowing their degree of conservation or variation in Mexican isolates, their phylogenetic relationship and their protective, immuno-stimulatory properties, are first steps towards that goal. (3) The development of new tools for diagnosis, detection and discrimination of bovine babesiosis is the third area. Developing variants of ELISA, which are more reliable than the currently used IFAT, are a priority, and finally, taking advantage of the genomes of Babesia bigemina, and B. bovis, we are identifying genes than allow us to discriminate isolates using molecular tools.     

小鼠仙台病毒标准化血清的制备及鉴定

目的制备标准化抗小鼠仙台病毒（Sendai Virus,SV）免疫血清,为清洁级及SPF级实验小鼠质量检测提供批量、稳定、敏感的质控血清。方法使用动物来源的仙台病毒（sv）感染BALB／c小鼠,获得高效价免疫血清,经IFA、IEA、ELISA等方法检测血清效价。结果制备多量抗SV血清,经多种方法检定,IFA效价达1：640,IEA效价达1：320,ELISA效价达1：102400～1：204800。结论本研究中制备的sV抗血清达到同批次大量高滴度的水平,可作为检测实验小鼠中sv病原的标准化质控血清。     

Quantitation of poliovirus antigens in inactivated viral vaccines by enzyme-linked immunosorbent assay using animal sera and monoclonal antibodies

Recent advances in methods for the manufacture of inactivated poliovirus vaccines have resulted in increased vaccine immunogenicity. In conjunction with this capability it is important to have available highly sensitive and quantitative potency assays. The potential suitability of enzyme-linked immunoassay (ELISA) was evaluated using animal sera with neutralizing antibodies or neutralizing monoclonal antibodies for antigen detection in potency tests. The monoclonal antibodies developed, which bound D antigen but not C antigen, were neutralizing unless relatively weakly reactive. Those that bound C antigen only were non-neutralizing. Those that bound both C and D antigens were sometimes neutralizing. D-specific and D/C-specific neutralizing monoclonal antibodies against type-2 poliovirus protected mice on passive immunization against paralytic disease and death from the MEF strain virus. Potency measurements by ELISA using either D-specific neutralizing monoclonal antibodies or type-specific goat sera for antigen detection were sensitive and precise. Tests using C-specific monoclonal antibodies for antigen detection indicated that increased C antigen content may result in falsely elevated reactivities of animal sera with some vaccines. Monoclonal antibodies may be useful ELISA reagents for IPV potency testing.     

The development and standardization of an enzyme-linked immunosorbent assay for the detection of antibodies to bovine herpesvirus 2

A single dilution enzyme-linked immunosorbent assay (ELISA) for the detection of antibodies to bovine herpesvirus 2 has been developed, standardized and compared with the virus neutralization test. The results of the two tests correlated well. A positive/negative threshold was established for the ELISA. The ELISA was reproducible, sensitive, rapid and specific.     

猪和牛轮状病毒抗原和抗体的检测

应用ELISA直接双抗体夹心法检查轮状病毒抗原,24份仔猪和29份犊牛的腹泻粪样,分别有12和16份阳性。用病毒RNA电泳分析检查阳性粪样,各出现两种病毒RNA电泳型,用中和试验检查17份成年牛和16份成年猪血清,分别有16和15份病毒抗体阳性。将其与ELISA间接法和结合法进行了比较。     

实验兔出血症病毒检测方法的建立与免疫效果调查

目的检测全省六个实验兔场的兔子所携带的兔出血症病毒（RHDV）情况,调查实验兔RHDV抗体水平,评价不同疫苗的免疫效果,比较HAI与ELISA两种方法的符合率。方法采用HAI、ELISA方法对1168份实验兔RHDV抗体进行了检测,并与RT-PCR方法的检测结果进行对比分析。结果我省实验兔免疫情况较好,不同饲养场的实验兔免疫合格率虽有不同,但未发生疫情。通过比较发现ELISA法检测的抗体合格率明显高于HAI法。结论LISA、HAI和RT-PCR方法均适合实验兔RHDV的检测。     

Isolation, purification and characterization of surface antigens of the bovine filarial parasite Setaria digitata for the immunodiagnosis of bancroftian filariasis

The surface antigens of the bovine filarial parasite Setaria digitata were isolated by EDTA extraction and purified by affinity chromatography using sepharose bound human filarial (Wuchereria bancrofti) antibodies obtained from chronic human filarial sera. The purified and crude antigens were used in enzyme-linked immunosorbent assay (ELISA) for the detection of serum antibodies in bancroftian filariasis. The purified antigen showed sensitive and specific reactions in ELISA for the detection of antibodies in filarial sera and showed least cross reactivity with other parasitic infections. The crude and purified antigens showed about 18 and 6 peptide bands respectively in SDS-PAGE and about 11 and 6 antigenic bands respectively in enzyme-linked immunoelectrotransfer blot (EITB). The purified antigen was observed to be glycoprotein in nature. It was possible to identify the stage-specific infection in human filariasis by using the crude and purified antigens in EITB.     

Possibilities of vaccine manufacture in human diploid cell strains with a serum replacement factor.

Cell lines MDCK (canine kidney), BGM (Buffalo green monkey kidney) and human embryonic lung fibroblast will support viral growth efficiently in medium without serum. Both MRC-5 and WI-38 cell strains have been approved by the Food and Drug Administration for manufacturing viral vaccines against cytomegalovirus and varicella-zoster virus. In this study we examine these two cell lines and viruses for their ability to grow in medium containing a serum replacement. The serum substitute used is LPSR-1 (low protein serum replacement). Using LPSR-1 in defined medium, we demonstrate multipassage cell growth and viral cultivation and replication equivalent to those obtained in medium containing fetal bovine serum (FBS). Viral growth after complete elimination of FBS varies and depends on cell line and virus. Serum substitutes can eliminate FBS in the viral growth phase of vaccine production and reduce costs.     

An immunosensor with potential for the detection of viral antigens in body fluids, based on surface second harmonic generation

Field methods of assessing the immune status of animals are required to optimise vaccination programmes to control bovine viral diarrhoea (BVD) virus. An optoelectronic immunosensor was evaluated for the detection of viral antigens in a crude cell lysate in a pilot study. Binding of (BVD) virus antigen by two monoclonal antibodies immobilised on two different media (ELISA plate wells, and glass coverslips) was detected and quantified using the laser induced surface second harmonic generation (SSHG) technique. The results for both assays were correlated with an enzyme-linked immunoassay (ELISA) used for the diagnosis of BVD virus infection in cattle (ELISA plate; R(2)=0.86, coverslips; Exp. 1; R(2)=0.75, Exp. 2; R(2)=0.67). The method will allow rapid detection of antigens in the body fluids of farm animals.