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鸡染性法氏囊病(IBD)弱毒冻干苗与大肠杆菌共同接种组发病率和死亡率均为7%;新城疫(ND)Ⅳ系冻干苗与大肠杆菌共同接种组发病率和死亡率均为7%;单独大肠杆菌接种组发病率和死亡率均为13%,两种疫苗与大肠杆菌共同接种组发病率为33%;死亡率为20%.结果说明.IBD弱毒或ND Ⅳ系冻干苗接种对鸡感染大肠杆菌无影响;两种疫苗联合接种则大肠杆菌对鸡的致病性增强。IDB野毒和大肠杆菌共同接种组发病率为47%,死亡率为27%;隐性ND野毒和大肠杆菌共同接种组发病率为27%,死亡率为20%;IBD野毒、ND野毒和大肠杆菌共同接种组发病率为47%,死亡率为33%;单独IBD野毒接种发病率为33%,死亡率为20%;单独ND野毒接种组发病率为27%,死亡率为13%;单独大肠杆菌接种组发病率和死亡率均为13%。结果表明,IBD病毒、隐性ND野毒可以明显增加大肠杆菌对鸡的致病力,尤以HBD病毒明显. 相似文献
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几种病毒与禽病原性大肠杆菌的人工联合感染 总被引:6,自引:0,他引:6
以2种剂量的低致病性禽流感病毒(lowly pathogenic avian influenza virus,LPAIV),传染性支气管炎病毒(infectious bronchitis virus,IBV)疫苗株H120和H52,新城疫病毒(Newcastle disese viurs,NDV)Lasota株分别于气管内注射10日龄易感鸡,2d后,气管注射禽病原性大肠杆菌O37株(O78),连续观察5d,结果,除LPAIV单独感染组有6.25%的死亡率外,其余各病毒单独接种组均健活;大肠杆菌O37株单独接种组的死亡率为62.50%,较高剂量的LPAIV,IBV H120和H52,NDV Lasota株与大肠杆菌O37株有效强的协同致病作用,死亡率分别达到81.25%,100.00%,93.75%和87.50%,而较低剂量的上述病毒则无明显的协同作用,IBV,NDV疫苗株与大肠杆菌联合接种组的多数死亡鸡病程推迟。 相似文献
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点眼接种鸡传染性喉气管炎弱毒苗引发鸡眼睛应激反应点眼接种鸡传染性喉气管炎弱毒疫苗,是有效地预防该病的一种免疫方法。此种免疫方法,较之强毒苗擦肛法安全,但仍然对鸡群是一种刺激,能引起一定的应激。笔者自1993年起连续三年观察,鸡传染性喉气管炎弱毒苗点眼... 相似文献
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用不同批次、不同剂量、不同保存时间的猪细小病毒N株弱毒苗接种豚鼠 ,观察豚鼠对PPVN株弱毒苗的抗体反应。其结果如下 :用 4种不同剂量的PPVN株弱毒苗免疫豚鼠 ,免疫后 14天均产生抗体反应 ,PPVHI价分别为 :0 1ml剂量为 1:16~ 1:6 4;0 2ml为1:8~ 1:32 ;0 5ml为 1:16~ 1:32 ;1 0ml为 1:16~ 1:6 4,而对照豚鼠抗体反应为阴性 ,可见仅需 0 1mlPPVN株弱毒苗便可引起豚鼠产生抗体反应。同时比较了不同批次的PPVN株弱毒苗接种豚鼠产生抗体反应的情况 ;3批PPVN株弱毒苗接种豚鼠后 14天全部出现抗体反… 相似文献
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1接种程序1.1出壳后24h内无母源抗体的雏野鸭皮下或胸肌接种鸭肝炎弱毒苗;有母源抗体的雏野鸭7~10日龄时,接种上述疫苗。1.214日龄胸肌接种鸭瘟弱毒苗。1.342日龄颈部皮下接种禽出败灭活菌苗。1.460日龄胸肌接种鸭瘟弱毒疫苗。1.590日龄颈部皮下接种禽霍乱油乳剂菌苗。1.6120日龄母野鸭(开产前30d)胸肌接种鸭肝炎弱毒苗;135日龄时再接种鸭肝炎弱毒苗1次。1.7280日龄(母野鸭停产期)胸肌接种鸭瘟弱毒疫苗。1.8成年经产种野鸭每年春秋两季各注射一次鸭瘟弱毒苗和禽霍乱油乳剂苗。2… 相似文献
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目的观察高致病性猪蓝耳病弱毒疫苗对猪的免疫效果。方法从某猪场选取90头仔猪,随机分为A组、B组、对照组,各30头。A组接种高致病性猪蓝耳病弱毒疫苗,B组接种高致病性猪蓝耳病灭活疫苗,C组给予生理盐水作为对照组。在免疫后28d、60d、90d时对比三组的S/P值与PRRS抗体阳性率。结果免疫28d时,A组仔猪S/P值超过2.0,增速很快,其PRRS抗体检测阳性率高达93.3%,B组为33.3%,差异显著(P0.05),有统计学意义。结论与灭活苗相比,高致病性猪蓝耳病弱毒苗抗体水平与抗体增速均更明显,免疫效果更好,因此,可优先考虑弱毒疫苗。 相似文献
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气雾接种鸡新城疫和鸡痘联苗盘宝进编译郑儒标校广西兽医研究所530001对鸡群的免疫,气雾接种最为方便和有效。小鸡对鸡新城疫病毒(NDV)和鸡痘病毒(FPV)高度易感。用10日龄鸡胚增殖NDV疫苗F株和R2B株,已高度致弱的FPV疫苗HP1株用12日龄... 相似文献
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将16只SPF鸡分成4组,每组4只,分别接种新城疫油乳剂苗,新城疫、传染性支气管炎、传染性法氏囊病三联油乳剂苗,LaSota弱毒苗和Mukteswer苗。接种后每隔2d采血1次,用ELISA测定新城疫特异性IgM和IgG抗体。结果:油乳剂灭活苗接种组均无特异性IgM抗体出现,特异性IgG抗体高峰期出现在接种后22d,LaSota弱毒苗和Mukteswer苗接种组均有特异性IgM抗体出现,高峰期为接种后第9d。各接种组经强毒攻击后,均出现IgM反应,IbG呈典型的回忆反应。进一步试验用LaSota灭活苗经肌肉、静脉接种和加氢氧化铝胶佐剂后肌肉接种,经测定,接种鸡均无或仅有很低水平的特异性IgM抗体产生。 相似文献
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1 流行病学调查
2005年4月3日,菏泽市牡丹区黄堽镇某养鸡场购入AA雏鸡4 000只,网上育雏.1日龄时接种马立克氏病疫苗,7日龄接种鸡新城疫Ⅰ系弱毒疫苗.10日龄时,雏鸡开始发病,并出现死亡,至15日龄时,共发病880只,死亡341只,发病率为22%,死亡率为8.5%.经菏泽市兽医卫生检验所检测,确诊为雏鸡大肠杆菌病.…… 相似文献
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Studies on transmission of maedi virus to lambs 总被引:4,自引:0,他引:4
L Sihvonen 《Acta veterinaria Scandinavica》1980,21(4):689-698
Lambs born to 5 ewes in 3 successive years were studied for presence of maedi virus and its antibodies. In the middle of the first-year pregnancies the ewes and the only ram of the colony were inoculated with maedi virus. No antibodies or viraemia could be detected in the lambs at birth. After sucking colostrum, antibodies appeared in the lambs of the ewes which themselves were seropositive, and reached their peak in a few days. Maternal antibodies disappeared within 12 weeks in all the lambs. Neutralizing antibodies were demonstrated in the colostrum and their content declined rapidly after lambing. Virus was isolated from the milk of 2 ewes in the third year of the studyIn the first year the spread of maedi virus was demonstrated to only 1 of the lambs, but in the other 2 years maedi virus was detected in tissues of half of the lambs sacrificed at 3–12 weeks of age. It was concluded that lambs born to chronically infected ewes are readily infected, indicating excretion of virus by ewes. The study yielded no information on the specific routes of transmission, except for the finding of the virus in milk of 2 ewes in the third year of the study. No evidence was obtained of transplacental transmission of maedi. 相似文献
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流感病毒是一类危害人和动物健康的RNA病毒,其在宿主细胞内的有效复制离不开宿主蛋白酸性核磷蛋白32家族成员A (ANP32A)和病毒RNA聚合酶的协助和支持。病毒RNA聚合酶由3种蛋白PB1、PB2和PA组成,且ANP32A与病毒RNA聚合酶的最强相互作用需要这3种蛋白的共同参与。ANP32A是酸性富含亮氨酸的核磷蛋白32(ANP32)家族成员,其被确认为支持细胞核中病毒RNA聚合酶活性的关键宿主因子,对流感病毒的复制具有重要的作用。ANP32A的物种特异性差异决定了病毒RNA聚合酶的宿主范围:独特的33个氨基酸序列存在于禽类ANP32A (avANP32A),而在哺乳动物ANP32A中缺乏此氨基酸序列。avANP32A中特有的33个氨基酸序列能增强ANP32A的功能,从而增加禽源特征流感病毒聚合酶活性。禽流感病毒(Avian influenza virus,AIV)不能有效利用较短的ANP32A (即缺乏独特33个氨基酸序列的ANP32A),因而哺乳动物ANP32A无法支持禽源特征聚合酶活性,然而在人ANP32A (huANP32A)中插入这33个氨基酸能促进其对AIV聚合酶的支持作用。此外,流感病毒的适应性突变也能增强AIV在哺乳动物中的传播力和致病性。AIV适应哺乳动物时往往会发生E627K突变,以增强其在哺乳动物中的复制能力。作者主要介绍了宿主蛋白ANP32A对流感病毒复制、转录的影响和流感病毒发生适应性突变的作用机制,简要论述了ANP32A与聚合酶的相互作用对流感病毒跨物种感染的分子机制。 相似文献
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鸡痘母源抗体对重组鸡痘疫苗免疫效果的影响 总被引:2,自引:1,他引:1
为了检测抗鸡痘病毒母源抗体对喉气管炎重组鸡痘疫苗的影响,孵化一批来自禽痘病毒高免母鸡的雏鸡,采用ELISA方法检测鸡痘疫苗免疫鸡后代的血清抗体。检测结果表明,雏鸡自孵出2d开始,血清鸡痘病毒抗体水平就开始缓慢下降,到15日龄时下降至临界值,已有部分鸡开始出现抗体阴性反应;到21日龄时,全部被检血清抗体水平均转为阴性。分别于不同日龄对试验雏鸡免疫接种重组鸡痘疫苗,结果只有当鸡体内的鸡痘病毒母源抗体全部为阴性(21日龄)后免疫时才能产生可靠的保护作用,保护率达到80%以上。这说明鸡痘病毒母源抗体对重组鸡痘疫苗的效果有一定的影响,因此重组疫苗合理的首免时间应选择在3周龄以后。 相似文献
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蜜蜂KBV和APV病毒RT-PCR检测技术研究 总被引:2,自引:0,他引:2
根据蜜蜂克什米尔病毒(Kashmir bee virus.KBV)和急性麻痹病毒(Acute paralysis virus,APV)的RNA聚合酶基因序列,参照Don Stoltz报道的引物KBV1、KBV2,美国农业部提供的引物DC62F、DC682R,对美国农业部惠赠的标准KBV和APV的RNA聚合酶基因片段,以及2001—2002年收集到的中国21个省市的180份疑似KBV和APV病蜂RNA聚合酶基因片段进行RT—PCR。对以KBV1、KBV2和DC62F、DC682R为引物扩增出的RNA聚合酶基因片段进行克隆、转化,并对克隆结果测序,证明其可靠性。建立了用分子生物学方法检测蜜蜂KBV和APV病毒的技术,有一定的应用前景。检测结果表明:到目前为止,我国蜜蜂群中未发现KBV和APV病毒病。 相似文献
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R Peshev L Christensen L Christova 《Comparative immunology, microbiology and infectious diseases》1998,21(4):247-255
Eight Bulgarian bovine herpes viruses, two Hungarian herpes viruses 1A, 3A, calves isolate named Mramor, buffalo isolate 723 and two referents BHV 1 strains were investigated by restrictase fragment pattern analysis. Migration profile of viral DNA by using different restrictase enzymes Hpa I, BamH I and Hind III were compared. Clearly differences among two Hungarian strains, calves isolate Mramor, buffalo isolate 723 and 8 Bulgarian and two referents BHV 1 strain was observed. The strain Sartze was determined as a genital type BHV 1, whereas Ozet, Tch.voda, Slivnitza, B. Budinov, Ptcelarovo, Vrana and Podgumer as a respiratory type. Hungarian strains 1A, 3A, calves isolate Mramor and buffalo isolate 723 had similar migration profile as swine herpes viruses. Hybridisation between the K 22 fragment and 8 bovine herpes viruses after Southern blotting were observed. That is evidence for genetic relation of these strains. Such hybridisation with Hungarian 1A, 3A, Mramor and buffaloes 723 strains were not observed. This fact allowed us to conclude that these strains are genetically different from BHV 1.
Résumé
On a examiné par l'analyse de la restrictase huit souches bulgares de virus herpès bovins, deux souches hongroises de virus herpès (1A et 3A), l'une isolée d'un buffle 723, l'autre isolée d'un veau nommé ‘Mramor’ et deux souches de virus de référence BHVI. Le profil migratoire des virus a été comparé à l'aide d'enzymes restrictase Hpa I, BamH I, Hind III. Une nette différence a été constatée entre les deux souches hongroises, la souche isolée du veau ‘Mramor’, celle isolée du buffle 723 et les huit souches bulgares. La souche Sartze a été déterminéee comme type génital, alors que Ozet, Tch.voda, Slivnitza, B. Budinov, Ptcelarovo, Vrana, Podgumer sont des types respiratoires. Le deux virus hongrois 1A et 3A, la souche isolée du veau ‘Mramor’, et celle isolée du buffle 723 ont un profil migratoire comparable à celui des virus herpès du porc. Après Soutchern blotting, une hybridation entre fragment K 22 et les huit virus herpès bovins a été constatée. Il y a une liaison génétique entre ces souches. Il n'y a pas d'hybridation entre les souches hongroises 1A et 3A, celle isolée du veau Mramor et celle isoléee du buffle 723. Cette observation nous permet de conclure que les souches sont génétiquement différentes de BHV 1. 相似文献
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Pinches MD Diesel G Helps CR Tasker S Egan K Gruffydd-Jones TJ 《Veterinary clinical pathology / American Society for Veterinary Clinical Pathology》2007,36(2):141-147
BACKGROUND: Screening tests for feline retroviruses are thought to have high sensitivity and specificity, although previous studies that evaluated these tests have limitations. Novel statistical approaches have been developed that allow the estimation of sensitivity and specificity in situations where the true state of the disease in individual animals cannot be assured. OBJECTIVE: The purpose of this study was to evaluate the sensitivity and specificity of a variety of retrovirus tests, including some screening tests, in a population of cats potentially infected with either feline leukemia virus (FeLV) and/or feline immunodeficiency virus (FIV) by using a Bayesian statistical approach. METHODS: Four hundred and ninety blood samples from cats being evaluated for FIV infection were tested by 2 rapid immunomigration tests (Witness single [WS], Witness combi [WC]) and a plate-based ELISA (Petcheck) for FIV antibody, and by a newly designed real-time polymerase chain reaction (PCR) assay for FIV provirus. Four hundred and ninety-five blood samples from cats being evaluated for FeLV infection were tested by 2 rapid immunomigration tests (WS, WC) and a plate-based ELISA (Petcheck) for FeLV antigen, and by a FeLV virus isolation technique. Results were then analyzed by using a Bayesian statistical method. RESULTS: For FIV tests, median sensitivity estimates were 0.98 for WS, 0.97 for WC, 0.98 for ELISA, and 0.92 for PCR. Median specificity estimates were 0.96 for WS, 0.96 for WC, 0.93 for ELISA, and 0.99 for PCR. For FeLV tests, median sensitivity estimates were 0.97 for WS, 0.97 for WC, 0.98 for ELISA, and 0.91 for virus isolation. Median specificity estimates were 0.96 for WS, 0.96 for WC, 0.98 for ELISA, and 0.99 for virus isolation. CONCLUSIONS: The use of Bayesian statistical methods overcomes a variety of methodologic problems associated with diagnostic test evaluations, including the lack of a definitive reference test. The sensitivity and the specificity of all 6 evaluated screening tests was high: however, specificity estimates were slightly lower than those reported by most recent studies. 相似文献