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Immune Status Assessment by Abundance of IFN-alpha and IFN-gamma mRNA in Chicken Blood.

机译:通过鸡血中IFN-α和IFN-γmRNA的丰度进行免疫状态评估。

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Avian diseases, including such viral infection as infectious bursal disease, infectious anemia, and Marek's disease, often cause immunosuppression, leading to more severe infection, problems with secondary infection, and inadequate responses to vaccination. Immunosuppression thus causes serious economic losses in commercial poultry production. To date, methods for assessing immune status have been too slow to be of practical help. Reasoning that immunosuppression should be reflected by reduced production of interferons (IFN) in response to a viral antigen, we have developed competitive nucleic acid hybridization microtiter plate assays for chicken IFN-alpha (ChIFN-alpha) and ChIFN-gamma mRNA. To evaluate the assay, chickens were challenged with inactivated Newcastle disease virus (iNDV). Whole blood samples were collected at various times subsequently and preserved with a cationic detergent. Later, total RNA was extracted, and mRNA for both ChIFN-alpha and ChIFN-gamma was measured. Both rose from undetectable levels to reach a peak by 4 h, remained high for about 3 days, and fell to undetectable levels by day 5. Results were similar in chickens aged between 1 and 28 days. In later experiments, blood was collected 4 h after viral challenge. When chickens were immunosuppressed by administering 4-5 mg cyclophosphamide (CY) daily for 3 days and challenged with iNDV, they transcribed less ChIFN-alpha and ChIFN-gamma mRNA, and their antibody response was impaired. Our results suggest that suspected immunosuppression in a commercial flock could be assessed within 2-3 days by challenging birds with iNDV and measuring the amounts of ChIFN-alpha and ChIFN-gamma mRNA in blood obtained 2-4 h later.
机译:禽类疾病,包括诸如传染性法氏囊病,传染性贫血和马立克氏病等病毒感染,通常会导致免疫抑制,导致更严重的感染,继发感染问题以及对疫苗接种的反应不足。因此免疫抑制在商业家禽生产中造成严重的经济损失。迄今为止,评估免疫状态的方法太慢,无法提供实际帮助。推理免疫抑制应通过减少对病毒抗原的干扰素(IFN)的产生来反映,我们开发了针对鸡IFN-α(ChIFN-alpha)和ChIFN-γmRNA的竞争性核酸杂交微量滴定板检测法。为了评估测定,鸡用灭活的新城疫病毒(iNDV)攻击。随后在不同时间收集全血样品,并用阳离子去污剂保存。之后,提取总RNA,并测量ChIFN-α和ChIFN-γ的mRNA。两者都从无法检测的水平上升到4 h达到峰值,在3天左右保持高水平,并在第5天下降到不可检测的水平。在1至28天之间的鸡中结果相似。在随后的实验中,病毒攻击后4小时收集血液。每天给鸡施用4-5 mg环磷酰胺(CY)进行免疫抑制3天,并用iNDV攻击时,它们转录的ChIFN-α和ChIFN-γmRNA较少,因此抗体反应受到损害。我们的结果表明,可以通过用iNDV攻击鸟类并测量2-4小时后获得的血液中ChIFN-α和ChIFN-γmRNA的量,在2-3天之内评估商业鸡群中的免疫抑制。

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