鸡体内肠球菌特异性抗体的血清学监测

IF 1.4 3区 农林科学 Q4 IMMUNOLOGY
Amanda Silberborth, Jana Schnug, Silke Rautenschlein, Arne Jung
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引用次数: 0

摘要

致病性盲肠球菌(EC)作为肉用型鸡生产中骨骼感染的病因,其重要性与日俱增。由于缺乏有效的干预策略,因此必须将重点放在预防措施上。通常的做法是为肉用种鸡群接种疫苗,以防止后代感染 EC。然而,目前尚无感染或接种疫苗后血清转换的数据。本研究的目的是使用一种新开发的鸡用欧共体特异性间接酶联免疫吸附试验(ELISA),对鸡的欧共体特异性免疫球蛋白 Y(IgY)进行血清学监测。检测方法的建立使用了以往感染研究中的血清。对确诊为欧共体阳性的肉用种鸡群、已接种疫苗和未接种疫苗的肉用种鸡群的血清样本进行欧共体特异性 IgY 分析。将酶联免疫吸附试验结果与实时 PCR 和/或细菌培养检查结果进行比较后发现,两者的结果基本一致。在受感染的鸡群中,ELISA 法检测的阳性样品多于实时 PCR 和/或细菌培养法检测的阳性样品。以孵出后 1 天(dph)的实验感染鸡为例,42 dph 时的阳性结果比例最高,S/P 比值也最高(p < 0.05)。自然感染鸡的样本也有类似趋势(p < 0.05)。免疫球蛋白 M (IgM) 二抗的调整为在生长期早期使用该检测方法提供了可能,因为此时仍有机会治疗感染。此外,在孵化后 4 周、10 周、15 周和 19 周对未接种疫苗的肉用种鸡群进行的监测显示,ELISA 阳性血清样本的持续增加与 S/P 比率的增加有关。这可能与平肠球菌抗体或天然抗体的交叉反应有关。总之,新开发的 ELISA 为在标准化条件下进行肠球菌实验研究期间对肉用型鸡进行血清学监测提供了一种合适的工具。值得注意的是,与目前可用的其他方法相比,该检测方法能检测出更高比例的欧共体阳性鸡。不过,由于本底较高,该检测方法尚不适合用于监测种鸡群。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Serological monitoring of Enterococcus cecorum specific antibodies in chickens

Pathogenic Enterococcus cecorum (EC) has gained increasing importance as the cause of skeletal infections in meat-type chicken production. Since effective intervention strategies are scarce, it must be focused on preventive measures. Vaccination of meat-type breeder chicken flocks is common practice to protect the progeny against infection with EC. However, no data are available on seroconversion after infection or vaccination. The aim of the present study was the serological monitoring of chickens for EC-specific immunoglobulin Y (IgY) using a newly established EC-specific, indirect ELISA for chickens. Sera from previous infection studies were used for the establishment of the assay. Serum samples from confirmed EC-positive meat-type chicken flocks, vaccinated, and non-vaccinated meat-type chicken breeder flocks were analyzed for EC-specific IgY. Comparison of ELISA results with results from real-time PCR and/or bacteriological examination via culture revealed fair to substantial agreement. In infected chickens, more samples were classified as positive via ELISA than via real-time PCR and/or bacteriological examination via culture. Focusing on chickens experimentally infected at 1 day post-hatch (dph), the highest proportion of positive results and highest S/P ratios were found at 42 dph (p < 0.05). A similar trend was observed for the samples from naturally infected chickens (p < 0.05). Adjustment of the secondary antibody against immunoglobulin M (IgM) may open possibilities to use the assay during the early phase of the growing period, when there is still a chance to treat the infection. The examination of samples from vaccinated and non-vaccinated meat-type breeder chickens revealed no significant differences of S/P ratios independent of farm and autogenous vaccine used. In addition to that, monitoring of a non-vaccinated meat-type breeder chicken flock at 4, 10, 15, and 19 weeks post-hatch showed a continuous increase of ELISA-positive serum samples associated with an increase of S/P ratios. This may be explained by cross reactivity with antibodies to Enterococcus hirae or natural antibodies. The usage of EC-specific, recombinant proteins for coating of the plates may help to reduce unspecific background and increase the assay’s specificity in future applications. In conclusion, the newly developed ELISA provides a suitable tool for serological monitoring of meat-type chickens during experimental studies with EC under standardized conditions. Remarkably, the assay is able to detect a higher proportion of EC-positive chickens than other methods, which are currently available. However, the assay is not yet suitable for the monitoring of breeder flocks due to high background.

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来源期刊
CiteScore
3.40
自引率
5.60%
发文量
79
审稿时长
70 days
期刊介绍: The journal reports basic, comparative and clinical immunology as they pertain to the animal species designated here: livestock, poultry, and fish species that are major food animals and companion animals such as cats, dogs, horses and camels, and wildlife species that act as reservoirs for food, companion or human infectious diseases, or as models for human disease. Rodent models of infectious diseases that are of importance in the animal species indicated above,when the disease requires a level of containment that is not readily available for larger animal experimentation (ABSL3), will be considered. Papers on rabbits, lizards, guinea pigs, badgers, armadillos, elephants, antelope, and buffalo will be reviewed if the research advances our fundamental understanding of immunology, or if they act as a reservoir of infectious disease for the primary animal species designated above, or for humans. Manuscripts employing other species will be reviewed if justified as fitting into the categories above. The following topics are appropriate: biology of cells and mechanisms of the immune system, immunochemistry, immunodeficiencies, immunodiagnosis, immunogenetics, immunopathology, immunology of infectious disease and tumors, immunoprophylaxis including vaccine development and delivery, immunological aspects of pregnancy including passive immunity, autoimmuity, neuroimmunology, and transplanatation immunology. Manuscripts that describe new genes and development of tools such as monoclonal antibodies are also of interest when part of a larger biological study. Studies employing extracts or constituents (plant extracts, feed additives or microbiome) must be sufficiently defined to be reproduced in other laboratories and also provide evidence for possible mechanisms and not simply show an effect on the immune system.
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