乳胶凝集试验检测鸡传染性法氏囊病毒血清抗体的研究

以鸡传染性法氏囊病病毒(IBDV)VP2基因工程抗原致敏乳胶微粒,用IBDV阳性血清进行方阵滴定,以最佳致敏系件制成乳胶抗源,建立乳胶凝集试验(LAT),用来检测血清中IBD抗体。对467份待测血清分别、同时作LAT和双向琼琼脂免疫扩散试验(DATA)。结果,LAT阳性419份,阴性48份;DAGT阳性425份,阴性42份.试验表明乳胶凝集试验操作简便、快速、敏感性高、特异性强,可用于现场检测,适合基层单位检测IBDV血清抗体。     

检测猪伪狂犬病病毒gE抗体红细胞凝集试验的建立及应用

以纯化的抗人红细胞单链抗体(ScFv)—猪伪狂犬病病毒(PRV)gE蛋白双功能融合蛋白为抗原,建立了检测猪伪狂犬病毒gE抗体的红细胞凝集试验。利用方阵滴定试验筛选出最佳抗原工作浓度为55μg/mL,血清最佳稀释度为1∶20,作用时间15 min,与猪瘟(CSF)、猪细小病毒(PPV)、猪繁殖与呼吸综合征(PRRS)、猪乙型脑炎(JE)、猪布氏杆菌病(Brucellosis)阳性血清和PRV gE缺失疫苗接种的猪免疫血清均不出现红细胞凝集现象,与PRV标准阳性血清反应出现肉眼可见的凝集圈。与美国进口的PRV抗体检测gE-ELISA诊断试剂盒检测结果比较,50份猪血清的阴、阳性检出符合率均为100%。红细胞凝集试验检测方法具有操作简便、敏感性和特异性较高的特点,可用于PRV野毒感染的快速筛查。     

检测猪乙型脑炎病毒抗体间接ELISA方法的建立与应用

以乙型脑炎病毒(JEV)弱毒疫苗株作为诊断抗原,对ELISA反应条件进行优化,初步建立了检测猪乙型脑炎病毒血清抗体的间接ELISA方法。应用该法检测从江苏、安徽、山东、浙江4省部分地区收集到的1089份血样,对华东地区猪乙型脑炎血清流行病学进行初步调查。结果JEV抗体阳性率为68.2%,其中,种猪JEV抗体阳性率为82.1%,商品猪JEV抗体阳性率为62.6%。从中随机抽取135份血样与国产商品化试剂盒进行比较,间接ELISA方法的特异性和敏感性分别为92%和96.4%,2种方法的符合率为95.6%;与NS1蛋白包被建立的ELISA比较,两者的符合率为97.7%;同时,本法的阳性检出率显著高于临床普遍使用的乳胶凝集试验结果。由此表明,本试验建立的间接ELISA方法具有较高的敏感性和特异性,适于大规模猪乙型脑炎血清流行病学调查。     

猪细小病毒病血清抗体VP2-ELISA检测方法的建立

利用纯化的猪细小病毒VP2蛋白为抗原,建立检测猪细小病毒血清抗体的间接VP2-ELISA。最佳反应条件为:抗原包被浓度300 ng/孔,4℃过夜,待检测血清1:50稀释。与猪细小病毒病阳性血清呈阳性反应,与猪瘟、猪伪狂犬病、猪繁殖与呼吸综合征、猪日本脑炎和猪圆环病毒病等5种疾病的阳性血清均无交叉反应。批间、批内试验变异系数均小于10%。用该方法与Ceditest PPV猪细小病毒抗体检测试剂盒对102份血清进行平行检测和比较,间接VP2-ELISA的敏感性为93.8%,特异性为81.1%,符合率为89.2%。结果表明,猪细小病毒血清抗体间接VP2-ELISA检测方法具有较高的敏感性和特异性,且重复性好,可用于猪细小病毒感染的血清抗体检测。     

乳胶凝集试验检测鸡新城疫病毒血清抗体的研究

用硫酸铵沉淀、透析浓缩的鸡新城疫病毒（ＮＤＶ）抗原致敏乳胶,然后所鸡新城疫阳性血清进行方阵滴定,选择出最佳致敏条件并制成新城疫病毒乳胶抗原,由此建立超乳胶凝集试验（ＬＡＴ）,用来检测新城疫血清抗体;用所建立的乳胶凝集试验（ＬＡＴ）和血凝抑制试验（ＨＩ）同步检测６９份鸡血清,结果乳胶凝集试验阳性６２份,阴性７份;血凝抑制试验阳性６６份,阴性３份,两者的总符合率为９４．２％（６５／６９）,且两者的检出率基本一致。结果表明,乳胶凝集试验具有操作简便、快速、敏感性高、特异性强且可用于现场检测等优点,是一种适合基层单位用来检测鸡新城疫病毒血清抗体的新方法。     

猪伪狂犬病血清抗体gB-ELISA检测方法的建立

用纯化的猪伪狂犬病病毒gB重组蛋白为抗原,建立了检测猪伪狂犬病血清抗体的gB-ELISA方法。最佳反应条件为：抗原包被浓度为3.15μg/mL,待检血清稀释度为1∶40。该方法对猪圆环病毒病、猪瘟、猪细小病毒病、猪繁殖与呼吸综合征（猪蓝耳病）、猪乙型脑炎、猪布氏杆菌病5种疾病阳性血清和SPF猪阴性血清检测呈阴性反应。批间、批内试验变异系数均不超过8%。用该方法与HerdChek ELISA试剂盒同时对119份血清进行了平行检测,其相对敏感性、特异性和符合率分别为：75%、80.7%和79%。试验结果表明：猪伪狂犬病血清抗体gB-ELISA检测方法具有较高的敏感性和特异性,且重复性好,可用于猪伪狂犬病毒血清抗体检测。     

应用乳胶凝集试验对猪粪便中轮状病毒的检出

我们改进了一种对腹泻猪粪中轮状病毒的简便凝集试验检出方法。法是用抗猪轮状病毒OSU毒株抗体被了的乳胶颗粒(抗OSU—LA)在玻片上进行凝集试验,此法对检出猪轮病毒具有高的敏感性和特异性。抗 OSU—LA和OSU抗原在载玻片上进行时,2分钟之内呈现出明显可见的凝集现象。此种乳胶凝集(LA)试验的敏感性比电子显微镜(EM)检出法高4倍。LA试验法可用于快速诊断猪轮状病毒感染症。     

PEDV流行株重组截短N蛋白间接ELISA检测方法的建立

为了建立猪流行性腹泻病毒(porcine epidemic diarrhea virus,PEDV)抗体检测的间接ELISA方法,本研究以纯化的原核表达的PEDV截短N蛋白作为包被抗原,建立了PEDV抗体检测的间接ELISA方法,将该方法命名为rnPED-ELISA。该抗原不与其他常见的7种猪病的阳性血清发生交叉反应,批内和批间重复性试验的变异系数均小于13%;rnPED-ELISA相对于血清中和试验(SN)试验的敏感性为93.33%,特异性为90.00%;rnPED-ELISA与TSZ全病毒抗体检测试剂盒的符合率达91.67%。采用rnPED-ELISA方法检测200份临床样品,PEDV抗体阳性检出率为69.5%。本试验建立的rnPED-ELISA方法具有良好的敏感性和特异性,可为免疫猪群抗体监测和猪流行性腹泻流行病学调查提供一种快速、简便的血清学诊断方法。     

检测猪细小病毒血清抗体乳胶凝集试验方法的建立及初步应用

将猪细小病毒在IBRS-2细胞上同步培养增殖,待出现细胞病变后,反复冻融,收获病毒液,用甲醛灭活。随后用经硫酸胺沉淀、透析后浓缩的细小病毒液进行方阵滴定,选择致敏乳胶的最佳条件,制成细小病毒乳胶凝集试验（LAT）抗原。抗原与细小病毒阳性血清反应出现肉眼可见的凝集颗粒,而与生理盐水、PBS、犊牛血清、猪瘟、衣原体、口蹄疫、伪狂犬病、弓形体及萎缩性鼻炎等阳性血清不出现凝集现象。用所建立的细小病毒乳胶凝集试验（LAT）与血凝抑制试验检测了203份猪血清,其中血凝抑制抗体阳性为161份,阴性为42份,阳性率为79.31％;乳胶凝集抗体阳性为150份,阴性为53份,阳性率为73.89％,两种方法阳性符合率为93.16％,经统计学检验P＞0.05,两者差异不显著。结果表明,乳胶凝集试验可以作为临床上大量血样进行血凝抑制试验前的初筛,具有简便、准确的优点,在检测细小病毒（PPV）抗体上具有较好的应用前景。     

猪繁殖与呼吸综合征病毒抗体NSP7-ELISA检测方法的建立

为了建立区分猪繁殖与呼吸综合征病毒(PRRSV)感染抗体和灭活疫苗免疫抗体的诊断方法,试验以重组表达蛋白NSP7为抗原,建立检测PRRSV抗体的NSP7-ELISA方法,并对最适反应条件进行确定,然后对猪瘟病毒、猪口蹄疫病毒、猪圆环病毒、猪伪狂犬病病毒、猪细小病毒阳性血清和采自长春市的150份血样样品进行检测。结果表明:NSP7-ELISA最佳工作条件为NSP7抗原的最适包被浓度2.0μg/m L,血清稀释度1∶40,酶标抗体的工作浓度1∶5 000,以5%脱脂奶粉封闭过夜;猪瘟病毒等5种猪常见病毒感染阳性血清的检测结果均为阴性;在150份血清样本检测中,敏感性、特异性和符合率分别为88.1%(37/42)、90.7%(98/108)、90.0%(135/150)。说明建立的方法具有良好的特异性和敏感性,可用于区分PRRSV感染抗体和灭活疫苗免疫抗体。     

猪细小病毒VP2蛋白单克隆抗体的制备及抗原捕捉ELISA方法的建立

为制备猪细小病毒VP2蛋白单克隆抗体(McAb),建立检测猪细小病毒的抗原捕捉ELISA方法 (AC-ELISA),本研究以原核表达的重组VP2蛋白作为免疫原,免疫6周龄BALB/c雌鼠,取其脾细胞与骨髓瘤细胞SP2/0进行融合,经间接ELISA方法筛选,成功获得了2株能稳定分泌抗猪细小病毒VP2蛋白的McAb,命名为3C4、5F8。以多克隆抗体作为捕获抗体、单克隆抗体5F8作为检测抗体,通过双抗夹心ELISA各个反应条件的优化,建立检测猪细小病毒抗原捕捉ELISA方法。该方法与日本乙脑病毒(JEV)、猪流行性腹泻病毒(PEDV)、伪狂犬病毒(PRV)、猪繁殖与呼吸综合征病毒(PRRSV)、猪瘟病毒(CSFV)均不发生交叉反应;与RT-PCR相比较,符合率、敏感性和特异性分别为93.6%、90.9%、94.4%。本研究建立的猪细小病毒AC-ELISA有良好的重复性、敏感性和特异性,可应用于猪细小病毒感染的早期诊断。     

Evaluation of a recombinant MIC3 based latex agglutination test for the rapid serodiagnosis of Toxoplasma gondii infection in swines

The entire gene encoding microneme protein 3 (MIC3) from Toxoplasma gondii was cloned into the plasmid pGEX-KG and subsequently expressed in Escherichia coli as a glutathione-S-transferase (GST) fusion protein. The recombinant MIC3 (rMIC3) was purified and evaluated in a latex agglutination test (LAT) as the diagnostic antigen for the detection of antibodies to T. gondii in pig sera. The specificity, stability, and reproducibility of the test were examined. No agglutination was found when the sensitized latex beads were mixed with phosphate-buffered saline (PBS), borate-buffered saline (BBS), normal saline, and negative serum samples. There was no cross-reactivity with the standard positive sera of other pathogens. But intense agglutination occurred with T. gondii antibody positive serum samples. In our study, the coincidence rate of tested positive-sera of the LAT with rMIC3-sensitized latex particles and the ELISA with rSAG1 was up to 92.8%, T. gondii specific antibodies were detected by the LAT in all piglets that were experimentally infected with T. gondii tachyzoites from 8 to 42 days after infection. Our results indicated that the rMIC3 based latex agglutination test appears to be suitable for the detection of T. gondii antibodies at the early stage of infection.     

Development of a specific latex agglutination test based on a recombinant hemagglutinin protein to detect antibodies to H5 avian influenza viruses

A latex agglutination test (LAT) was developed for rapid detection of antibodies to H5 avian influenza viruses (AIVs). The hemagglutinin protein of H5 AIV was covalently linked to carboxylated latex by ethyl-dimethyl-amino-propyl carbodiimide to prepare the sensitized latex beads. The LAT was evaluated with the hemagglutination inhibition (HI) assay as the reference test. The H5-LAT showed a sensitivity of 87.0% and specificity of 88.9% in detecting 126 serum samples from experimentally infected chickens and a sensitivity of 82.5% and specificity of 86% in detecting 587 field chicken serum samples from mostly vaccinated chickens. The agreement ratio between H5-LAT and HI was found to be 87.3% and 83.1% for the two groups of samples, respectively. Difficulty with background agglutination in stored chicken sera was overcome by serum pretreatment with either dried chicken liver powder or dilution buffer containing detergent Tween-20. The H5-LAT has advantages over a previously reported whole-virus LAT in terms of biosafety in preparation, chemical stability, and higher specificity. It is a rapid and simple test suitable for field monitoring of antibodies to H5-type AIV.     

The Development and Application of the Latex Agglutination Test to Detect Serum Antibodies against Japanese Encephalitis Virus

The attenuated SA14-14-2 strain of Japanese encephalitis virus (JEV) was cultured in BHK-21 cells. The viral supernatant was purified and concentrated with PEG (MW 20 000). A suitable concentration of JEV antigen was used to sensitize latex to prepare the latex antigen. The specificity, sensitivity and stability of the antigen were assessed. A latex agglutination test (LAT) was developed for rapidly detecting antibody against JEV infection. The LAT and haemagglutination inhibition (HI) assay were compared by simultaneously testing 35 porcine serum samples from five farms. Ninety per cent (20/23) of the samples were seropositive by both assays. No significant difference was found between the two methods (p > 0.05). Furthermore, when 1613 porcine sera from 120 farms were tested by LAT, the number of positive sera was 652, while that of negative sera was 961, ranging from 20% to 50% positive throughout the year. These results indicate that LAT is an appropriate candidate method for epidemiological surveys for and diagnosis of Japanese encephalitis.     

重组N蛋白抗原检测PRRSV抗体ELISA的研究Ⅱ.试剂盒阴阳性临界值的测定及其与IDEXX公司试剂盒的比较

对临床上采集的899份猪血清样本。用以纯化的重组N蛋白为包被抗原建立的检测猪繁殖与呼吸综合征病毒（PRRSV）抗体的间接ELISA进行检测．运用统计学方法摸清了检测结果的分布规律。并扣国外IDEXX公司PRRSV抗体检测试剂盒同时对460份血清样本进行检测。结果表明。2种方法的符合率为91．73％。利用TG—ROC软件确定了自制的ELISA酶标板（NP—ELISA）的临界值。并标定试剂盒的特异性扣敏感性均为92．6％。ELISA的结果判定标准是：当以血清样本L为标准参考阳性血清时，样品与阳性血清的比值（S／P）小于或等于0．4为阴性；S／P在0．4与0．5之间为可疑；S／P大于或等于0．5为阳性。与IDEXX公司PRRSV抗体检测试剂盒对临床样品的检测结果进行比较后，初步判定所建立的ELISA之所以出现较多的假阴性。可能是目前临床上出现了PRRSV欧洲型所致。     

猪传染性胸膜肺炎研究进展

猪传染性胸膜肺炎(PCP)已成为危害各国养猪业的主要传染病之一,其病原体胸膜肺炎放线杆菌主要定居在猪的呼吸道,有较高的宿主特异性。国内外已建立起补体结合试验、酶联免疫吸附试验、乳胶凝集试验、间接荧光抗体技术等用于PCP的检测和流行病学研究。该文就其疫苗的研制、分类、应用等进行概述。     

猪繁殖与呼吸综合征病毒重组M蛋白间接ELISA抗体检测方法的建立及应用

为建立一种敏感、特异、快速、高通量的猪繁殖与呼吸综合征病毒(PRRSV)抗体血清学检测方法,本研究利用原核表达技术表达了PRRSV M蛋白,将纯化后的重组M蛋白作为包被抗原建立了检测PRRSV抗体的间接ELISA方法。参照已发表的PRRSV基因组M基因序列,设计合成1对特异性引物,RT-PCR扩增了长约435 bp的M基因片段,将目的片段亚克隆至pET32a(+)表达载体中,经IPTG诱导获得了以包涵体形式表达的重组M蛋白,重组蛋白纯化后,免疫印迹检测结果表明具有良好的抗原性和特异性。以重组M纯化蛋白为包被抗原,经间接ELISA反应条件的优化,建立了检测PRRSV抗体的间接ELISA方法,该方法检测猪瘟病毒(CSFV)、猪细小病毒(PPV)、猪乙型脑炎病毒(JEV)、猪伪狂犬病病毒(PRV)、猪传染性胃肠炎病毒(TGEV)、猪圆环病毒2型(PCV2)其他6种常见猪病病原的阳性血清均为阴性;该方法批内与批间重复性试验的变异系数分别小于5%和10%;该方法与商品化ELISA试剂盒的符合率为95.3%。本研究建立的M-ELISA检测方法将为猪群免疫PRRS疫苗后抗体水平监测及PRRSV野毒感染的快速诊断与流行病学调查等提供了一种简便易行、快速、高通量的血清学抗体检测方法。     

Serodiagnosis of bovine leptospirosis by IgG-Enzyme-Linked Immunosorbent Assay and Latex Agglutination Test

The efficacy of a recombinant leptospiral outer membrane protein LipL41 as an antigen for conducting IgG-Enzyme linked immunosorbent assay (ELISA) and latex agglutination test (LAT) for serodiagnosis of bovine leptospirosis was evaluated. The recombinant LipL41 antigen developed and used for detecting the antibodies was specific in detection of the pathogenic serovars of Leptospira, as the expression of the LipL41 antigen is restricted only to pathogenic leptospires. A total of 430 bovine serum samples were subjected to IgG-ELISA and LAT, and the sensitivity and specificity were assessed in comparison with microscopic agglutination test (MAT). The sensitivity and specificity of IgG-ELISA and LAT were 86.84% and 93.16%, and 95.42% and 98.33% respectively. Both the tests are found to be sensitive, specific and concurred with the standard MAT. The study concluded that the rLipL41 protein could be used as a potential diagnostic antigen in different assay formats for bovine leptospirosis.