Correlation between Hemagglutination Inhibition Titer and Protection against Infectious Bronchitis Virus Challenge in SPF Layers

[ Objective] To study the correlation between HI titer and protection against IBV challenge in SPF layers. [ Method ] SPF layers were randomly divided into four groups, namely group A1, A2, B1 and B2. The group A1 was immunized with H120 live vaccine. The group A2 was first immunized with H120 live vaccine and later boosted with ND-IB-EDS trivalent inactivated vaccine. The group B1 was used as unimmunized chal- lenge control. The group B2 was kept as unimmunized unchallenged control. The blood samples were taken prior and post-vaccination at intervals and HI tests were conducted. At the laying peak, the group A1, A2 and B1 were challenged with IBV M4t virulent strain. The clinical features and egg production of layers were monitored and recorded. [Result] After 30 d post vaccination with H120 live vaccine, the HI titer reached 4.45 log2; after 30 days boosting with ND-IB-EDS trivalent inactivated vaccine, the HI titer reached to 7.35 log2. Before challenge, HI antibody titer in group A1, A2, B1 and B2 were respectively 4.24 log2, 7.40 Iog2, 2.10 log2 and 2.10 log2. After challenge, chickens in unimmunized challenge control group B1 showed respiratory symptoms, egg production dropped by 30.9%, and they produced more soft-shelled, no-shelled or abnormal eggs. In the group A1, some chickens had light respiratory symptoms and egg production dropped by 11.7%. In the group A2, the egg production of all chickens was as normal as the group B2. [ Conclusion] When the HI titer was over 6 log2, challenge by virulent virus had no impact on egg produc- tion; when the HI titer was 5 log2, 4 log2 and less 3 log2, egg production dropped by 6.0%, 11.3% and 29.6%, respectively. Thus, the HI anti- body level in chickens has close correlation with protection against IBV challenge.

减蛋综合征病毒抗体胶体金免疫层析试纸条的研制及初步应用

为建立快速检测减蛋综合征病毒(EDSV)抗体的方法,基于EDSV的Fiber蛋白,制备快速检测EDSV抗体的免疫层析试纸条,为养禽业提供针对病原微生物的感染预警及免疫评估。利用胶体金标记EDSV Fiber蛋白抗原为探针,将羊抗鸡IgG和抗Fiber蛋白的抗体包被到硝酸纤维膜上,分别作为质控线和检测线,对家禽EDSV抗体水平进行监测。结果表明,制备的EDSV免疫层析试纸条具有高度特异性,与其他家禽病毒抗体无交叉反应,仅与EDSV抗体反应,在试纸条上产生可见的检测线;并且制备的试纸条具有高度稳定性,在室温条件下可至少保存6个月。应用制备的检测EDSV抗体的免疫层析试纸条对从河南、安徽、山东等地养鸡场采集的576份鸡血清样本检测,与血凝抑制试验(HI)结果进行平行比较,二者的Kappa值为0.878,具有良好一致性。综上,制备的检测ESDV抗体的免疫层析试纸条具有高度的特异性、敏感性、稳定性和易操作性,对EDSV抗体的临床检测具有实际应用价值。

离子交换树脂法规模化生产乳源酪蛋白糖巨肽及其对流感病毒的血凝抑制活性

目的:优化规模化生产乳源酪蛋白糖巨肽(CGMP)的工艺条件,并探讨其对流感病毒的血凝抑制能力。方法:以阴离子交换树脂为分离介质,唾液酸含量为产品的活性检测指标,分别从上样体积、上样流量、洗脱液浓度、洗脱液体积和树脂使用周期5个工艺条件,在前期小试和中试的基础上,考察从乳清粉中规模化生产CGMP;同时利用血球凝集抑制试验验证产品CGMP对流感病毒的抑制活性。结果:优化的CGMP产品技术路线为上样体积3BV、上样流量0.8 L/min、洗脱体积1BV、洗脱液浓度0.6 mol/L、树脂适宜使用周期4次。该工艺条件下处理乳清粉溶液体积为108 L(2160 g)、树脂36 L,得到CGMP产品21.183 g,得率为0.981 g/100 g,产品纯度为89.032%,回收率为51.972%,唾液酸含量为21.503 g/100 g,蛋白CGMP产品对流感病毒A(H1N1)和流感病毒B的最低抑制质量浓度分别为1.0000,1.2500 mg/mL。结论:利用优化的技术路线生产获得CGMP产品的纯度和唾液酸含量均优于市售商品CGMP,且对流感病毒有明显的抑制作用。

三种血清学方法和qPCR方法在鸡滑液囊支原体检测中的综合应用研究

为评价不同方法对鸡滑液囊支原体(MS)活疫苗免疫和非免疫状态鸡群的监测效果,研究分别采用HI、SPA与ELISA三种抗体检测方法和qPCR方法同步对某养殖场A、B和C三组鸡群进行MS感染和抗体水平监测,其中A鸡群23日龄免疫MS活疫苗(MS-H株),B、C鸡群不免疫MS疫苗。结果显示:三种血清学检测方法所测MS抗体阳性率趋势基本一致,HI抗体效价变化规律和ELISA抗体效价变化规律相似,但血清学方法相对于qPCR方法具有一定的滞后性,qPCR可以最早发现MS野毒感染,且在使用活疫苗免疫的情况下对疫苗和野毒进行鉴别检测。研究提示:在条件允许的情况下,qPCR可以作为MS首选的监测方法;当检测条件受限时,上述三种血清学方法同样也可以用于评估MS野毒感染状况,但对结果的判断受母源抗体水平、疫苗免疫状况、野毒感染时间等多重因素的影响,在结果判断时应进行综合分析。

猪细小病毒血凝抑制试验抗原、阳性血清与阴性血清的制备与鉴定

猪细小病毒(Porcine parvovirus,PPV)血凝抑制试验抗原、阳性血清和阴性血清在猪细小病毒制品的效力检验中不可或缺,对猪细小病毒相关生物制品的质量控制至关重要。试验采用PPV 7909株病毒同步接种PK-15细胞制备血凝抑制试验抗原,用制备的抗原乳化后免疫豚鼠制备阳性血清,同时用未免疫的阴性豚鼠制备阴性血清。对抗原、阳性血清和阴性血清进行鉴定,结果表明,制备的PPV血凝抑制试验抗原HA效价达1∶512;阳性血清HI效价达1∶1024;阴性血清HI效价小于1∶8,且特异性均良好。用制备的HI试验抗原与不同PPV疫苗株的阳性血清进行HI试验,同时,用制备的阳性血清、阴性血清与不同PPV疫苗株的灭活抗原进行HI试验。结果表明,制备的抗原与阳性血清具备良好的血清学交叉反应性,制备的阴性血清与不同疫苗株抗原均呈阴性反应,可用于PPV制品的统一评价。

免疫鸡群新城疫强毒感染及其与HI抗体的相关性研究

为调查新城疫强毒(vNDV)在免疫鸡群中的感染情况及其与抗ND抗体效价的相关性,用自行建立的检测vNDV的荧光定量RT-PCR(RRT-PCR)对采自川、渝两地36个免疫鸡群的360份肛门棉拭子进行检测,同时采血测定其血凝抑制抗体效价。结果共检出5个vNDV阳性鸡群,每个阳性鸡群检出1例阳性样本,经病毒分离鉴定证实为NDV;36个受检鸡群HI抗体平均效价在4.5～10.1,标准偏差(SD)在0.70～3.19,变异系数在9.5%～44.3%。当SD大于2.0时,vNDV感染鸡群阳性率为50%(5/10),当CV大于32%时,vNDV感染鸡群阳性率为62.5%(5/8);vNDV感染个体HI抗体效价分别为210、29、28、26、23;阳性样本RT-PCR产物经测序分析证实为vNDVF基因序列,发育进化分析显示,2株vNDV属基因Ⅶ型,3株属基因Ⅸ型。研究结果表明,RRT-PCR适合vNDV感染及传播的监测和分子流行病学调查;免疫鸡群是否感染vNDV可能与个体HI抗体水平高低无关,而与群体HI抗体离散度有关,SD和CV值有助于判定鸡群感染vNDV的风险。

水禽禽流感H5N1亚型改良HI抗体检测方法的研究

鉴于在采用1%鸡红细胞悬液作为指示细胞检测水禽血清的HI抗体效价水平过程中常出现非病毒性凝集情况,亟需要建立一种快速简便经济的适合水禽血清抗体效价检测的方法。本研究通过对未经处理与采用不同红细胞吸附处理被检水禽血清以1%鸡、鸭或鹅红细胞悬液进行测定其HI抗体效价的结果对比,结果表明建立采用1%与待检水禽血清同源1%红细胞悬液做指示细胞的改良HI试验比采用鸡红细胞悬液测定结果高1～1.5log2,且可以有效避免非病毒性凝集情况的出现。

几种常用ND HI试验方法的比较与分析

对几种常用 ND HI试验方法作比较 ,结果表明 ,在全量法和微量法中以生理盐水为稀释液 ,以 1 %红细胞悬液作反应指示剂和 1 0 0 %凝集抑制为判定终点的方法效果为佳。全量法测得的 HI滴度较微量法的约高 0 .5～ 1个滴度 ,其灵敏度和准确性较高 ,从而更适于实际工作中 ND抗体水平的免疫监测。

间接EL ISA与HI检测鸡新城疫抗体相关性

应用间接 EL ISA和微量红细胞凝集抑制试验 ,同时对来自两个鸡场的 1 71份血样进行常规鸡新城疫抗体检测。结果表明 ,二种方法的抗体效价检测结果呈显著相关 ,其相关系数为 0 .92 49(r2= 0 .8560 ) ,设置 t检验 ,差异显著 t<0 .0 0 0 1 ,(n= 1 71 ) ,并测得总体和各鸡群的回归方程 ,其中总体的回归方程式为 EL ISA =0 .2 80 5× HI-0 .450 9。 EL ISA方法具有敏感 ,特异 ,快速 ,简便的优点 。

鸡传染性支气管炎HA抗原的制备及HI试验方法的建立

用１０％Ａ型魏氏梭菌滤液处理１００倍浓缩ＩＢＶＭ４１株病毒液，成功地制备了ＩＢＶＨＡ抗原，效价为１∶６４～１∶１０２４。用该抗原建立了ＩＢＶＨＩ试验方法。抗原在４℃保存，５个月效价不变；加入０．１％的甲醛及１／万的硫柳汞使抗原效价下降１～２个滴度。对ＳＰＦ鸡血清、Ｍ４１阳性血清、其它鸡病标准阳性血清以及疫苗免疫试验鸡只血清的ＩＢＶＨＩ抗体监测结果证明，该方法操作简便、快速、敏感性高、特异性强。

His-N2蛋白体外排除抑制大肠杆菌DH5α黏附猪肠黏液蛋白的研究

以植物乳杆菌KLDS1.0320候选表面黏附蛋白NP_785232 N端前两个结构域组成的融合表达蛋白为研究对象,采用体外模拟肠道环境的方法研究其对大肠杆菌DH5α黏附猪肠黏液的排除抑制作用。对猪肠黏液进行固定,加入His-N2融合表达蛋白37℃孵育1h,再加入大肠杆菌DH5α菌悬液37℃孵育1h,洗去未黏附的菌体,之后用1%Triton?X-100进行裂解,将裂解液涂布LB琼脂平板以进行菌落计数。结果表明:pH值为6.6时,相对于缓冲液阴性对照组,His-N2蛋白对大肠杆菌DH5α黏附猪肠黏液的抑制率为(50.37±3.66)%,相对于BSA蛋白对照组的抑制率为(38.33±4.55)%;pH值为7.5时,相对于缓冲液阴性对照组,His-N2蛋白对大肠杆菌DH5α黏附猪肠黏液的抑制率为(42.18±3.44)%,相对于BSA蛋白对照组的抑制率为(34.48±3.90)%。在体外模拟条件下,由植物乳杆菌KLDS1.0320的候选表面黏附蛋白NP_785232 N端前两个结构域组成的His-N2蛋白能排除抑制大肠杆菌DH5α对猪肠黏液蛋白的黏附。

RPHI和HI对EHF患者进行血清学分型的比较研究

作者应用RPHI和HI两种方法,对EHF患者进行血清学分型的比较。通过对57例不同病日的EHF患者血清与野鼠型及家鼠型病毒血凝素抗原(分别称为A-Ag及R-Ag)同时进行HI、RPHI。在EHF疾病过程中,两种抗体的效价呈平行性升降,存在明显的正相关(用A-Ag时,r=0.94;用R-Ag时r=0.98),对3,5,7,10,17病日的患者进行可分型率的统计发现,HI,RPHI的可分型符合率为58,75,96,36,100,100％;另对189份荧光阳性的患者血清检测的结果,HI,RPHI两法判别家、野鼠型的总符合率为90.5％。上述结果表明:与HI相比,RPHI用于EHF患者的血清学分型,不仅操作简便,勿需复杂费时的血清处理,并具有更高的特异性和灵敏度,可普遍应用于患者的早期诊断和血清流行病学的分型研究。

SPF鸡新城疫非特异性HI抗体的血涂片鉴别研究

试验以某SPF鸡场的30份HI抗体效价疑似阳性血清为研究对象,建立了快速准确的血涂片鉴别诊断法。以间接免疫荧光法进行验证,结果提示血涂片法与间接免疫荧光法的结果完全一致,证明了血涂片法可以用于新城疫非特异性HI抗体的鉴别诊断,具有简单、方便的优点。

反向血凝抑制试验(RIHI)检测鼠疫F1抗体在疫情监测和疫源地调查中的应用

在鼠疫疫情监测和疫源地调查工作中,将鼠疫 Fl 单克隆抗体致敏红细胞 (FlM_cAb-RBC) 用于反向间接血凝抑制试验 (RIHI),以间接血凝试验为对照,检测鼠疫 Fl 抗体,检测结果用 ELISA 和 SPRIA 验证,非鼠疫疫区6种动物血清1375份,RIHI 全部阴性,IHA 出现假阳性反应89份。鼠疫疫区3种动物血清713份,RIHI 检出 Fl 抗体阳性反应72份,未出现假阳性反应,IHA 检出 F1 抗体阳性反应44份,出现假阳性反应21份,几何平均滴度 RlHl 比 IHA 高2^(1.45)。RIHI 的特异性和敏感性均高于 IHA ,且简便、稳定、快速,是取代 IHA 检测鼠疫 Fl 抗体的理想方法。

鸡新城疫抗体消长规律及血清抗体稳定性

为研究鸡新城疫灭活疫苗免疫后抗体消长规律及血清抗体稳定性,采用血凝抑制试验方法测定新城疫病毒-禽流感病毒(H9亚型)二联灭活疫苗免疫鸡血清新城疫抗体效价及经室温、4℃、-20℃、-80℃反复冻融和加热等不同方式处理的血清中新城疫抗体效价。结果表明,试验鸡于1日龄和21日龄用灭活疫苗免疫两次后,在第二次免疫后14 d新城疫抗体平均效价达到8.1 log_(2),35 d达到最高值为8.9 log_(2);免疫后70 d抗体效价保持在7.8 log_(2),且自二免后14~70 d,新城疫抗体效价维持在7.8 log_(2)~8.9 log_(2)。血清新城疫抗体在室温和4℃相对稳定,室温下放置13 d对新城疫抗体效价几乎无影响;但4℃保存9 d,对新城疫抗体效价有一定影响,且差异显著(P<0.05);56℃下30 min对新城疫抗体效价无影响;反复冻融3次对新城疫抗体效价影响极显著(P<0.01)。肉鸡于1日龄和21日龄用灭活疫苗免疫两次后,新城疫抗体水平高,且高水平抗体维持时间长。鸡血清新城疫抗体可耐56℃加热,室温保存活性稳定,反复冻融则影响其效价。

用HI和ELISA方法检测SPF鸡血清和蛋黄中ND抗体的比较

分别用血凝抑制试验(HI)和酶联免疫吸附试验(ELISA)检测42周和48周SPF鸡血清、以及同期SPF鸡蛋蛋黄中新城疫(ND)抗体。结果表明,两种方法检测的120份血清中均无ND抗体,呈阴性;120枚SPF鸡蛋蛋黄检测,ELISA方法检测结果全为阴性;HI方法检测结果25份阳性,差异较为明显。

Evidence of Synergistic Activity of Medicinal Plant Extracts against Neuraminidase Inhibitor Resistant Strains of Influenza Viruses

The frequent emergence of drug resistant influenza viral strains emphasizes the urgent and continual need to develop new antiviral drugs. Given the encouraging findings of previous studies on antiviral compounds from plant sources, this study focused on medicinal plants from Borneo that were traditionally used to treat symptoms of influenza infection. Following the promising results of earlier investigations, four plant extracts that demonstrated multiple modes of viral inhibition were studied against wild-type and neuraminidase (NA) inhibitor-resistant strains of Types A and B influenza viruses. The extracts exhibited more pronounced activities against the wild-type viruses than the NA inhibitor-resistant strains. Variations in the antiviral potential of the extracts collected from different parts of the same plant were also evidenced in the in vitro micro-inhibition assays. Even though all plant extracts affected NA activity of all viruses, only two extracts demonstrated hemagglutination inhibitory (HI) activities against Type A pandemic H1N1 and Type B viruses. Furthermore, Receptor Destroying Enzyme (RDE) treatments of extracts exhibiting HI activities indicated the presence of sialic acid (SA)-like component(s) that may be responsible for HI activity. Since the antiviral potential of extracts was not completely suppressed by RDE, the possibility of non SA-like antiviral components cannot be ruled out. Therefore, synergistic activity between SA-like and non SA-like components contained in the plant extracts may be responsible for the demonstrated antiviral potential. The results also indicated the presence of non SA-like components that may act against other viral proteins apart from hemagglutinin (HA) and NA. Hence, this study supports the presence of multiple antiviral components that act against different viral proteins or interfere with different stages of viral replication. Our results suggest that these plant extracts have the potential to be developed as therapeutic agents for the treatment of influenza and could be a solution to the global occurrence of viral strains resistant to NA inhibitors.

Comparative Study of Serologic Results Obtained by HI Test of Avian Influenza and Newcastle Disease Performed in Four Mexican Laboratories

In the poultry industry, it is common to evaluate the humoral immune response associated to the vaccination calendar used for the different zootechnical purposes. When the vaccine against avian influenza and Newcastle disease currently used in a farm is going to be changed, an important parameter observed to choose a product over the others is based on the antibody titers reached by the application of the new vaccine. This study aimed to compare the serologic results obtained by hemagglutination inhibition （HI） test of avian influenza and Newcastle disease reported in four different national laboratories. One-day-old Ross broiler chickens were kept in Horsfall-Bauer isolation units and were vaccinated subcutaneously for the prevention of avian influenza and Newcastle disease. Then, serum of all the birds was extracted at three, six and seven weeks old and sent to four different national diagnostic laboratories, where HI test was performed for avian influenza and Newcastle disease. The treatments were designed in 4 × 3 factorial. Data showed significant statistical differences between laboratory results （up to six logarithms for influenza at six and seven weeks）. This study confirms that the results of the HI test can vary from one laboratory to another, thus it is important to consider this, when the vaccines against avian influenza and Newcastle disease are evaluated at field.

禽流感H9非免疫鸡场与免疫鸡场鸡群HI抗体的比较研究

为了解禽流感H9在非免疫鸡群的感染情况和免疫鸡场的免疫效果,本试验在四川分别选择一个非免疫鸡场和免疫鸡场,用微量HI试验对187份不同日龄的非免疫鸡血清(56、85、92、149、256、410日龄)和222份不同日龄的免疫鸡血清(53、87、145、264、398日龄)进行了抗体检测,结果显示:非免疫鸡群禽流感H9阳性率分别为34.38%、37.14%、29.41%、38.71%、46.67%、52.00%,免疫鸡群阳性率分别为76.27%、84.31%、88.37%、91.89%、81.25%。试验表明非免疫鸡群的禽流感H9感染较严重,免疫鸡群免疫后的效果较好。

2019~2021年花溪区H5、H7亚型禽流感免疫抗体监测情况及分析

为了解2019~2021年花溪区的禽流感免疫效果,对其管辖的部分涉农乡镇(街道)随机采集120~400日龄的鸡群血清样品4 391份,采用血凝抑制试验对禽流感H5和H7亚型进行免疫抗体检测,根据高致病性禽流感诊断技术中抗体效价标准进行判定,HI抗体效价≥4log2,判定个体免疫效力合格;群体免疫抗体合格率≥70%,判为群体抗体合格率达标。检测结果显示,花溪区(H5+H7亚型)禽流感免疫抗体合格率2019、2020、2021年依次为91.03%、91.78%、96.19%,呈现逐年上升趋势;H7亚型抗体合格率高于H5亚型,规模化鸡场抗体合格率高于大户和散养户。综上所述,禽流感免疫抗体合格率均高出国家标准,说明全区免疫工作较扎实有效;监测禽流感免疫抗体为花溪区科学预防H5、H7亚型禽流感的流行提供数据支撑,推动花溪区的家禽业健康持续发展。