首页> 外文期刊>Avian Diseases >Comparison of vaccine subpopulation selection, viral loads, vaccine virus persistence in trachea and cloaca, and mucosal antibody responses after vaccination with two different Arkansas Delmarva Poultry Industry-derived infectious bronchitis virus vaccines.
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Comparison of vaccine subpopulation selection, viral loads, vaccine virus persistence in trachea and cloaca, and mucosal antibody responses after vaccination with two different Arkansas Delmarva Poultry Industry-derived infectious bronchitis virus vaccines.

机译:比较疫苗亚群选择,病毒载量,疫苗病毒在气管和泄殖腔中的持久性以及接种两种不同的阿肯色州德尔马瓦家禽业衍生的传染性支气管炎病毒疫苗后的粘膜抗体反应。

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Factors responsible for the persistence of Arkansas Delmarva Poultry Industry (ArkDPI)-derived infectious bronchitis vaccines in commercial flocks and the high frequency of isolation of ArkDPI-type infectious bronchitis viruses in respiratory cases are still unclear. We compared dynamics of vaccine viral subpopulations, viral loads, persistence in trachea and cloaca, and the magnitude of infectious bronchitis virus (IBV)-specific antibody induction after vaccination with two commercial ArkDPI-derived Arkansas (Ark) serotype vaccines. One of the vaccines (coded vaccine B) produced significantly higher vaccine virus heterogeneity in vaccinated chickens than the other vaccine (coded A). Chickens vaccinated with vaccine B had significantly higher viral loads in tears at 5 days postvaccination (DPV) than those vaccinated with vaccine A. Vaccine B also induced a significantly higher lachrymal immunoglobulin M response at 11 DPV, an earlier peak of IBV-specific lachrymal immunoglobulin A, and higher serum antibodies than vaccine A. In addition, a significantly higher proportion of birds vaccinated with vaccine B had vaccine virus detected in the trachea at 20 DPV than those vaccinated with vaccine A. Furthermore, the virus detected at 20 DPV in most of the chickens vaccinated with vaccine B was a single specific subpopulation (subpopulation 4) selected from multiple vaccine subpopulations detected earlier at 5 and 7 DPV in the same chickens. On the other hand, a higher proportion of chickens vaccinated with vaccine A had virus detected in cloacal swabs at 20 DPV. Thus we found differences in mucosal antibody induction and selection and persistence of vaccine viruses between two ArkDPI-derived vaccines from different manufacturers. The higher vaccine virus heterogeneity observed in chickens vaccinated with vaccine B compared with those vaccinated with vaccine A may be responsible for these differences. Thus the high frequency of Ark IBV viruses in the field may be due to the inherent ability of some ArkDPI-derived vaccine viruses to be selected and persist in vaccinated chickens. Vaccine virus persistence may offer genetic material for recombination or may undergo mutations with the potential to result in increased virulence.
机译:在商业鸡群中,源自阿肯色州德尔马瓦家禽业(ArkDPI)的传染性支气管炎疫苗持续存在的因素以及呼吸道病例中ArkDPI型传染性支气管炎病毒的高分离频率仍不清楚。我们比较了两种商业ArkDPI衍生的阿肯色州(Ark)血清型疫苗接种疫苗后疫苗病毒亚群,病毒载量,气管和泄殖腔中的持久性以及传染性支气管病毒(IBV)特异性抗体诱导程度的变化。其中一种疫苗(编码疫苗B)在接种鸡中产生的疫苗病毒异质性明显高于另一种疫苗(编码A)。接种疫苗B的鸡在接种疫苗后5天(DPV)的泪液中的病毒载量明显高于接种疫苗A的鸡。疫苗B还在11 DPV时诱导出明显更高的泪液免疫球蛋白M反应,这是IBV特异性泪液免疫球蛋白的早期峰值。 A,并且血清抗体的水平要高于疫苗A。此外,接种疫苗B的鸟在20 DPV时在气管中检出的疫苗病毒要比接种疫苗A的鸟高。此外,大多数疫苗在20 DPV时检出的病毒接种疫苗B的鸡只中,有一个是单个特定的亚群(亚群4),该群是较早在同一只鸡中以5和7 DPV检出的多个疫苗亚群。另一方面,接种疫苗A的鸡比例较高,在20 DPV时在泄殖腔拭子中检测到病毒。因此,我们发现了来自不同制造商的两种ArkDPI衍生疫苗在粘膜抗体诱导,疫苗病毒选择和持久性方面的差异。与使用疫苗A接种的鸡相比,在接种疫苗B的鸡中观察到的疫苗病毒异质性更高,这可能是造成这些差异的原因。因此,本领域中高频率的Ark IBV病毒可能是由于某些ArkDPI衍生的疫苗病毒被选择并在接种鸡中持久存在的固有能力所致。疫苗病毒的持久性可能会为重组提供遗传物质,也可能会发生突变,从而可能增加毒力。

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