共查询到19条相似文献,搜索用时 489 毫秒
1.
《中国预防兽医学报》2020,(9)
为评价A型口蹄疫疫苗免疫水平,本研究以本实验室前期制备的口蹄疫病毒(FMDV)的单克隆抗体(MAb)3D9为捕获抗体,以HRP标记的MAb 9A9作为检测抗体,建立了基于MAb的检测A型FMDV抗体的固相竞争ELISA(SPCE)方法,并对其条件进行优化。结果显示,MAb 3D9的包被浓度为1.16μg/mL,A型FMDV抗原的最佳稀释度为1:5,HRP标记的MAb 9A9的最佳稀释度为1:5 000,当血清132稀释时,检测的临界值确定为35%。利用该方法分别检测A型、O型口蹄疫抗体阳性标准血清以及牛冠状病毒、牛轮状病毒以及猪繁殖与呼吸障碍综合征病毒、猪圆环病毒、猪瘟病毒的标准阳性血清。结果显示,除A型口蹄疫阳性标准血清为阳性结果外其余均为阴性结果,未出现交叉反应,表明本研究建立的方法特异性强。该方法对经病毒中和试验(VNT)检测为阳性的3份血清进行敏感性试验,敏感性分别为1:1 024、1:256、1:128,均高于VNT,表明其敏感性较高;重复性试验结果显示,该方法批内和批间重复试验的变异系数均小于10%,表明其重复性较好。利用该方法与液相阻断ELISA方法(LPBE)和VNT对112份血清样品同时检测,分析三者相关性。结果显示,本实验建立的SPCE方法与二者的相关系数分别为0.901和0.916,表明该方法可靠性较好且与VNT的相关性更高。进一步利用本研究建立的SPCE方法和韩国Jeno A型FMDV ELISA抗体检测试剂盒同时检测470份临床血清样品(90份羊血清、170份牛血清和210份猪血清),结果显示该方法检测羊血清、牛血清和猪血清与Jeno试剂盒总体符合率分别为90.0%、91.8%和89.0%。表明该方法的检测结果较为准确。本研究为建立A型口蹄疫检测方法奠定了基础。 相似文献
2.
《中国预防兽医学报》2016,(3)
为建立Asia1型口蹄疫(FMD)快速病原学诊断方法,本研究采用纯化的Asia1型口蹄疫病毒(FMDV)免疫BALB/c小鼠,取免疫小鼠脾细胞与SP2/0骨髓瘤细胞进行融合并筛选到一株能够稳定分泌抗Asia l型FMDV单克隆抗体(MAb)2E10。经间接免疫荧光试验特异性鉴定,2E10为FMDV型特异型MAb。其抗体亚类为Ig G1/资,杂交瘤细胞上清和腹水抗体效价分别为1颐256和1颐104,相对亲和力常数为2.5 mol/L。在此基础上,以本实验室前期制备的MAb 2D8为包被抗体,以HRP标记的MAb 2E10为检测抗体建立了检测Asia1型FMDV抗原的双抗体夹心ELISA(DAS-ELISA)方法。该方法针对FMDV细胞毒的最低检出量为103TCID50,对O型FMDV、A型FMDV、牛肠道病毒、牛呼肠孤病毒及牛传染性鼻气管炎病毒检测结果均为阴性。本研究建立的Asia1型FMDV DAS-ELISA方法为Asia1型FMD病原学诊断试剂盒的研发奠定了基础。 相似文献
3.
为建立检测牛传染性鼻气管炎病毒(IBRV)血清抗体的阻断ELISA方法,本研究以经蔗糖密度梯度离心法纯化的IBRV作为免疫原制备1株单克隆抗体(MAb),命名为cp-1-1。经间接ELISA、IFA和western blot鉴定,该MAb与IBRV呈阳性反应,与牛病毒性腹泻病毒(BVDV)及牛副流感病毒3型(BPIV3)呈阴性反应,具有较强的特异性。质谱分析结果显示MAb cp-1-1识别的表位位于IBRV VP8蛋白。以纯化的IBRV作为包被抗原、MAb cp-1-1作为检测抗体,建立检测IBRV血清抗体的阻断ELISA方法。该检测方法的抗原包被量为0.89μg/孔,样品稀释度为12,检测抗体MAb量为1.3μg/孔,二抗稀释度为15000。利用50份IBRV抗体呈弱阳性的牛血清(中和抗体效价为14~116)作为标准参考血清,确定该检测方法的阻断率Cut Off值为52.06%,即阻断率高于52.06%时判为阳性,低于52.06%时判为阴性。阻断ELISA方法特异性试验显示仅IBRV阳性血清检测为阳性,而BVDV、BPIV3、牛腺病毒3型(BADV-3)和O型口蹄疫病毒(O-FMDV)阳性牛血清均检测为阴性,表明该方法具有较强的特异性;该方法可检测的最低中和抗体效价为14,与病毒中和试验的敏感性一致,表明该方法具有较高的敏感性;重复性试验显示该方法批内、批间变异系数均小于10%,显示较好的重复性。对130份现地牛血清检测结果显示,该方法与病毒中和试验的符合率为98.46%。用该方法对某牛场接种IBRV灭活疫苗的牛血清进行检测,抗体阳性率为99.51%(205/206)。另外,采用该方法对我国8个省(市、自治区)的801份牛血清进行检测,IBRV的抗体阳性率为41.6%(333/801)。本研究建立的阻断ELISA方法可以用于IBRV疫苗免疫监测和血清流行病学调查,为我国IBR的防控提供技术支持。 相似文献
4.
《黑龙江畜牧兽医》2016,(19)
为了缩短病毒中和试验(VNT)在口蹄疫病毒(FMDV)疫苗毒株选择以及病原检测中的时间,减少结果判断时人为因素的影响,试验采用qRT-PCR方法改进了传统的VNT,首先建立基于FMDV 3D序列的Taqman探针法qRT-PCR,之后使用FMDV Asia-1/JSL/06毒株感染IBRS-2细胞,提取不同时间收集的细胞病毒混合物的RNA进行qRT-PCR定量检测,获得FMDV Asia-1/JSL/06毒株在IBRS-2细胞中的病毒复制曲线,确定病毒复制的终点时间,即病毒中和试验中加入细胞维持液之后的第20小时,此时使用TRIzol裂解细胞并提取RNA进行qRT-PCR定量检测。以6作为拷贝浓度对数的临界值,拷贝浓度对数大于6的最低稀释度作为终点稀释度,建立了qRTPCR-VNT方法的终点稀释度判断标准,并应用该方法对19份阴性血清以及4份阳性血清进行qRT-PCR-VNT检测。结果表明:该方法获得的阴性、阳性结果与传统VNT检测获得的结果完全相符。说明该方法具有快速、有效、重复性好等优点,具有代替传统VNT的潜能。 相似文献
5.
抗A型口蹄疫病毒单克隆抗体的制备及抗原捕获ELISA检测方法的建立 总被引:1,自引:0,他引:1
为建立A型口蹄疫病毒(FMDV)病原学诊断方法,本研究应用纯化的A型FMDV免疫BALB/c小鼠,取其脾细胞与SP2/0细胞融合,筛选获得一株稳定分泌单克隆抗体(MAb)的杂交瘤细胞株5F7.经IFA特异性鉴定,5F7为一株血清型特异性MAb.亚类为IgG1/k.间接ELISA检测杂交瘤细胞上清和腹水抗体效价分别为1:12 800和1:105.硫氰酸盐洗脱法测定其相对亲和力常数为1.5 mol/L.应用该A型特异性MAb及实验室已制备的MAb 3D9初步建立了检测A型FMDV的抗原捕获ELISA方法.该方法可以检出2.0 ng纯化FMDV和1.0×104 TCID50病毒,与O型、Asial型FMDV及牛肠道病毒、牛呼肠孤病毒、牛传染性鼻气管炎病毒等均无交叉反应,组内及组间重复性试验显示变异系数小于8%.本研究建立的抗原捕获ELISA方法为A型FMDV抗原检测提供了一种实用有效的技术手段. 相似文献
6.
为建立检测非洲猪瘟病毒(ASFV)血清抗体的阻断ELISA方法,本研究对ASFV p72蛋白进行原核表达并纯化,将其免疫BALB/c小鼠并通过间接ELISA方法筛选到1株稳定分泌p72蛋白的杂交瘤细胞株3F8。以纯化的p72蛋白作为包被抗原,辣根过氧化物酶(HRP)标记的单克隆抗体(MAb)作为检测抗体,采用方正滴定法对反应条件优化后初步建立了检测ASFV的阻断ELISA方法。利用该方法检测133份ASFV阳性血清和73份ASFV阴性血清,通过ROC曲线分析确定临界值。结果显示,该方法的临界值为25.62%时,ROC的曲线面积最大,为0.9989,诊断敏感性和特异性分别为98.63%和98.5%。利用该方法检测ASFV、O型口蹄疫病毒(FMDV)、A型FMDV、猪繁殖与呼吸综合征病毒、猪流行性腹泻病毒、猪伪狂犬病毒、猪瘟病毒阳性血清,结果显示,除ASFV阳性血清外,其他阳性血清均为阴性,表明特异性强;利用该方法和商品化试剂盒对2倍倍比稀释(1∶4~1∶2 048)的两种ASFV灭活阳性血清(P1、P2)检测,结果显示该方法检测结果与商品化试剂盒基本一致,敏感性高。利用该方法对3份灭活的... 相似文献
7.
为了满足我国现阶段猪伪狂犬病病毒(PRV)高频突变引发新疫情诊断的需求,本实验通过生物信息学分析比较,设计合成了针对PRV g B糖蛋白高度保守的抗原优势表位区肽段,命名为g B872。以此肽段为包被抗原,经条件优化建立了新型的PRV-g B间接ELISA抗体检测方法。该ELISA方法检测结果显示,其仅对PRV血清检测为阳性,而与猪瘟病毒、猪繁殖与呼吸综合征病毒、口蹄疫病毒(O型)、猪细小病毒、猪圆环病毒2型等主要猪源病毒阳性血清均无交叉反应,表明该方法具有较强的特异性;最低检测下限血清稀释度为1∶128,高于IDEXX PRV/ADV g B抗体检测试剂盒检测下限稀释度(1∶4),表明该方法敏感性高;批内、批间重复性试验结果显示,变异系数均低于10%,重复性良好。利用该方法与Bio Chek PRV-g B抗体检测试剂盒检测90份临床血清样品,对比结果分析显示,两者阳性符合率为100%,阴性符合率为97.67%,总体符合率为97.78%;同时,采用该方法与IDEXX-g I(gE)和IDEXX-g B试剂盒分别对野毒感染血清和疫苗免疫血清同时检测,该方法可以准确识别野毒阳性血清和疫苗免疫阳性血清,与IDEXX两种试剂盒的结果一致。本研究建立的间接ELISA检测方法对PRV疫苗免疫效果评价、流行病学调查及防控提供了可靠的方法。 相似文献
8.
间接ELISA检测鸭疫里默氏杆菌血清抗体方法的建立 总被引:2,自引:2,他引:0
应用1型鸭疫里默氏杆菌(云南株)超声粉碎物作为包被抗原,建立检测鸭疫里默氏杆菌血清抗体的间接ELISA方法。用倍比稀释法确定HRP标记羊抗鸭二抗最佳稀释倍数为1∶3500,并用棋盘测定法确定抗原的最佳包被浓度为2.7mg/mL,血清最佳稀释倍数为1∶300,阴性血清临界值为0.381;阻断试验结果表明,1型鸭疫里默氏杆菌与其抗血清阻断阳性,与鸭大肠杆菌O78、O132菌株和FJ4型鸭疫里默氏杆菌阻断阴性(无交叉反应)。重复性试验结果表明,该ELISA方法批内变异系数≤0.246,批间变易系数≤0.889。结果表明,该ELISA方法特异性强,重复性好,可用于1型鸭疫里默氏杆菌(云南株)血清抗体的检测。 相似文献
9.
为建立检测牛边缘无浆体(Anaplasma marginale)抗体的方法,本研究以牛A.marginale膜表面重组MSP5蛋白作为包被抗原,抗MSP5单克隆抗体(MAb)作为竞争抗体,建立一种用于检测牛A marginale抗体的重组MSP5蛋白竞争抑制ELISA(CI-ELISA)方法.经优化确定CI-ELISA的最佳反应条件为:抗原包被浓度为2μg/孔,封闭液为2%脱脂乳,MAb的稀释度为1:400,酶标二抗的稀释度为1:1000,阴性和阳性血清临界值分别为33%和40%;该方法具有良好的特异性和重复性;2 348份临床血清样品的检测结果表明,217份为阳性,阳性率为9.2%,与IDEXXA marginale抗体检测试剂盒的阳性符合率为95.3%,阴性符合率为100%.本实验建立的ELISA方法具有较高的特异性和重复性,可用于流行病学调查研究. 相似文献
10.
为建立评价猪流行性腹泻病毒(PEDV)疫苗免疫效力的方法,本研究利用纯化的PEDV免疫BALB/c小鼠,按照常规方法制备PEDV全病毒单克隆抗体(MAb)作为捕获抗体,PEDV细胞培养上清为夹心抗原,HRP标记的羊抗猪IgA为二抗,采用棋盘滴定法对各反应条件优化后建立了用于猪初乳中PEDV IgA检测的捕获ELISA方法,并确定其临界值为0.25。采用该捕获ELISA对PEDV、PCV2b、PRRSV、PRV、JEV、PPV、FMDV与CSFV IgA抗体阳性猪初乳进行检测,结果显示,除PEDV IgA抗体阳性猪初乳检测结果为阳性外,其他病毒抗体阳性猪初乳检测结果均为阴性,表明该方法特异性强。采用该方法和BIONOTE PEDV IgA试剂盒对从1∶10开始2倍倍比稀释的16个稀释度的阳性猪初乳样品检测,结果显示该方法对阳性样品检测的最大稀释度为1∶40 960,是BIONOTE PEDV IgA试剂盒敏感性的16倍(1∶2 560),表明本研究建立方法的敏感性高。分别采用同一批次和不同批次制备的MAb包被的ELISA板分别检测5份PEDV IgA抗体阳性和1份PEDV IgA抗体阴性... 相似文献
11.
An indirect ELISA for detecting the IgA antibody against porcine foot-and-mouth disease virus (FMDV) type A was developed by using purified FMDV structural protein VP1 as coating antigen, mouse anti-pig IgA monoclonal antibody as second antibody and HRP-conjugated goat anti-mouse IgG as third antibody.The concentration of coating antigen was optimized as 3.50 μg/mL,the dilution and reaction time of second antibody and third antibody were optimized as 1:10 000 and 30 min, respectively.There was no cross-reactivity with anti-CSFV, PRRSV and other pathogen specific IgA antibodies.The positive detection rate of FMDV type A infectedsamples was above 90%.The coefficient variation of intra-and inter-assay was ranged from 3.16% to 9.76%.The ELISA method described in this study was proved to be specific and rapid for the detection of FMDV specific IgA antibody.It was potential to be applied for detection the level of FMDV specific IgA and evaluate the effect of mucosal immunity.Besides,it provided a new method for clinical diagnosis of foot-and-mouth disease. 相似文献
12.
为建立一种检测口蹄疫病毒(foot-and-mouth disease virus,FMDV)特异性IgA抗体的检测方法,本研究以原核表达系统表达纯化的FMDV结构蛋白VP1作为包被抗原,以鼠抗猪IgA单克隆抗体为二抗,辣根过氧化酶标记的羊抗鼠IgG抗体为三抗,建立猪A型FMDV特异性IgA抗体间接ELISA检测方法。确定抗原包被浓度为3.50 μg/mL,二抗与三抗的最佳稀释度为1∶10 000,二抗和三抗作用时间均为30 min。所建立的方法与抗猪瘟病毒、猪繁殖与呼吸道综合征病毒等病原的特异性IgA抗体间无交叉反应,A型口蹄疫感染样品的阳性检出率在90%以上,批内和批间重复性试验的变异系数介于3.16%~9.76%。该方法为监测FMDV特异性IgA抗体水平变化规律及猪的黏膜免疫效果评价及口蹄疫的早期诊断提供了一种新方法。 相似文献
13.
为建立检测血清中非洲猪瘟病毒(African swine fever virus,ASFV)抗体的间接ELISA方法,本试验将ASFV p30基因进行原核表达,采用SDS-PAGE和Western blotting方法对重组蛋白进行表达鉴定和免疫原性分析,随后以纯化的重组蛋白为包被抗原,经条件优化、特异性试验、敏感性试验和重复性试验,建立一种血清中ASFV抗体的检测方法。结果显示,ASFV p30基因成功克隆到原核表达载体pET-32a (+)中,获得pET-32a-p30重组质粒;转化大肠杆菌BL21(DE3)感受态细胞进行诱导表达,得到P30重组蛋白,重组蛋白大小约为42 ku,主要以包涵体形式存在;Western blotting结果显示,纯化后的蛋白具有良好的免疫原性;以纯化的P30重组蛋白为包被抗原,建立了检测ASFV抗体的间接ELISA方法,通过方阵试验对间接ELISA方法进行优化,最终确定了抗原最佳包被浓度为1.2 μg/mL,待检血清最佳稀释倍数为1:100,最佳封闭液为1% BSA,酶标抗体最佳稀释度为1:4 000,以此建立的ASFV间接ELISA方法临界值为0.322。本方法仅与ASFV阳性血清发生特异性反应,与猪瘟病毒、猪繁殖与呼吸综合征病毒、口蹄疫病毒、伪狂犬病病毒、猪圆环病毒2型及猪流行性腹泻病毒阳性血清均无交叉反应,具有较强的特异性。该方法检测ASFV阳性血清灵敏度可达到1:1 600;批内重复性和批间重复性变异系数均<10%。本试验建立的间接ELISA方法具有良好的特异性、灵敏度和重复性,可初步应用于ASFV抗体的检测。 相似文献
14.
Maddur MS Mohan MS Gajendragad MR Kishore S Gopalakrishna S Singh N 《Veterinary research communications》2009,33(2):103-109
Humoral and mucosal (secretory antibody)immune response to FMDV type Asia 1 in cattle was analyzed after vaccination and infection
using virus neutralizing test (VNT). Vaccination (1/16th the usual dose) failed to protect cattle from generalized clinical
disease following experimental FMDV Asia 1 infection. Our results showed that infection induced higher and prolonged serum
antibody titres indicating antigen mass is important for optimal immune response. Experimental FMDV infection induced significant
secretory antibody (mucosal) response in cattle. Though, there was no difference in the serum antibody response between the
cattle that developed generalized infection (unprotected) and those with only localized infection (protected), secretory antibody
response differed, wherein the unprotected cattle had higher secretory response than protected cattle. Thus, FMDV Asia 1 infection
stimulates a similar serum antibody response and a unique secretory antibody response among the infected cattle.
An erratum to this article can be found at 相似文献
15.
16.
Serology for diagnosis and epizootiological studies of bovine respiratory syncytial virus infections 总被引:2,自引:0,他引:2
The complement fixation test (CFT) and the virus neutralisation test (VNT), performed as a plaque reduction test, were employed to measure antibodies to bovine respiratory syncytial virus. The CFT with bovine sera was performed with supplementation of the complement factors in fresh guinea pig serum by an adequate amount of Clq-factor of the bovine species. Kinetics of maternally derived antibodies and the antibody response after spontaneous and experimental infections and after intramuscular vaccination were studied by both tests. Patterns of development of complement fixing and virus neutralising antibodies were generally similar and titres equalled each other in the test systems that are described. However a VNT detected antibodies a few days earlier after an infection than a CFT and peak-levels reached after a naturally acquired infection decreased faster in a CFT than in a VNT: a mean decrease of 3.1 and 1.4 log2 units was found in 13 weeks respectively. Mean half-life of passive antibodies was 25 days in a VNT. An infection with bovine respiratory syncytial virus could be diagnosed by serology, using a CFT on acute and convalescent serum samples of a number of animals in a group. Serology is preferable to virus isolation for routine diagnosis of bovine respiratory syncytial virus infections. Paired sera, collected at 14-day intervals and examined by CFT, are recommended for the diagnosis of the cause of respiratory disease. A VNT is preferable if low antibody levels are to be detected because non-specific reactions occur in a CFT at low serum dilutions. 相似文献
17.
18.
E. N. Smitsaart M. Zanelli I. Rivera N. Fondevila D. Compaired E. Maradei T. Bianchi V. O''Donnell A. A. Schudel 《Preventive veterinary medicine》1998,33(1-4):283-296
The development of a liquid-phase blocking sandwich ELISA (LPBE) to measure antibodies (Ab) produced in cattle with the O, A and C foot-and-mouth disease virus (FMDV) types of commercial vaccines used in Argentina is described. The test was specific: 99% of naïve cattle sera (n = 130) gave titres below log10 = 1.2, and none had a titre above log10 = 1.5. Comparative studies with serum neutralization test (SNT) using sera from cattle which received one or more vaccine doses is reported. The overall rank correlation coefficient (Spearman's , rs) between SNT and LPBE were highly significant (rs > 0.67, P < 0.0001) for all vaccine strains. LBPE Ab titres on sera collected 90 days post vaccination were compared with results of cattle protection tests by applying a logistic regression. The minimum Ab titres at which 85% and 75% of the cattle were protected for each FMDV type were determined in order to interpret field Ab data in terms of protection. Application of this method allows large scale serological examinations to monitor antibody levels in vaccinated animals as an indirect indicator of the FMD control program status in the field. Its use in the evaluation of commercial batches of FMD vaccine is discussed. 相似文献
19.
M Puntel N A Fondevila J Blanco Viera V K O'Donnell J F Marcovecchio B J Carrillo A A Schudel 《Zentralblatt für Veterin?rmedizin. Reihe B. Journal of veterinary medicine. Series B》1999,46(3):157-161
This study analysed sera from 390 llamas (Lama glama) from nine farms located in three different Argentine provinces: Buenos Aires, Cordoba and Jujuy. The samples were tested for antibodies against 8 virus known to infect cattle: bovine herpesvirus type 1 (BHV-1), bovine viral diarrhea virus (BVDV), bovine adenovirus (BAdV III), bovine enterovirus (BEV), bovine rotavirus (BRV), bluetongue virus (BTV), bovine leukaemia virus (BLV), and foot-and-mouth virus (FMDV) by conventional methods such as seroneutralization, immunoperoxidase staining, and agar gel immunodiffusion. The antibody prevalences detected in llamas were: BHV-1 in 0.77% (3/390), BVDV in 2.05% (8/390), BAdV III in 5.13% (20/390), BEV in 4.10% (16/390), BRV in 87.69% (342/390). No antibodies against BTV, BLV and VIAA (FMDV infection associated antigen) were detected. 相似文献