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利用重组蛋白作为抗原的间接 ELISA 的验证,以鉴定感染双芽巴贝斯虫的动物。

Validation of an indirect ELISA using recombinant proteins as antigen to identify animals exposed to Babesia bigemina.

机构信息

CENID- Salud Animal e Inocuidad, INIFAP, Jiutepec, Mexico.

出版信息

Transbound Emerg Dis. 2020 Jul;67 Suppl 2:201-207. doi: 10.1111/tbed.13522. Epub 2020 Mar 25.

Abstract

The objective of this study was to instrument a serological assay for the epidemiological diagnosis of bovine babesiosis in Mexico, using the Babesia bigemina recombinant protein RAP-1 (rRAP-1α) as antigen. rRAP-1α, r12d3 and rGP45 were the three recombinant antigens initially tested. Based on the highest titres obtained in the indirect ELISA (iELISA) with the positive control serum, using similar antigen concentrations, rRAP-1α was selected for further use. The diagnostic sensitivity and specificity rates estimated for the iELISA with rRAP-1α as antigen were 89.9% and 86.5%, respectively, while for the Indirect Fluorescent Antibody Test (IFAT), the gold standard assay, the sensitivity was 86.66% and the specificity was 95%. The ĸ agreement value determined was 0.52, indicating a moderate agreement between the iELISA and IFAT assays. The instrumented iELISA with rRAP-1α as antigen shows an excellent specificity rate and an acceptable sensitivity that allows for the detection of antibodies to B. bigemina in cattle naturally exposed to the vector tick Rhipicephalus microplus. By using the iELISA-rRAP-1α, along with an iELISA with recombinant Merozoite Surface Antigen (rMSA-1) for antibody determination against Babesia bovis in the serum samples collected from cattle at 'La Posta' experimental station in Mexico, a seroprevalence of 20.3% was estimated for B. bigemina and 19.4% for B. bovis, while 36.89% of samples were positive for both Babesia species. The iELISA test promises to be a safe and low-cost type of diagnosis available to cattle producers in Mexico and would facilitate the definition of herd immunity status to implement measures of control adapted for the prevention of bovine babesiosis outbreaks.

摘要

本研究旨在为墨西哥的牛巴贝斯虫病的流行病学诊断建立一种血清学检测方法,使用巴贝斯虫二联重组蛋白 RAP-1(rRAP-1α)作为抗原。最初测试了 rRAP-1α、r12d3 和 rGP45 这三种重组抗原。根据与阳性对照血清在间接酶联免疫吸附试验(iELISA)中获得的最高效价,使用类似的抗原浓度,选择 rRAP-1α 用于进一步研究。以 rRAP-1α 作为抗原的 iELISA 的诊断灵敏度和特异性估计值分别为 89.9%和 86.5%,而间接荧光抗体试验(IFAT)作为金标准检测方法,其灵敏度为 86.66%,特异性为 95%。确定的κ一致性值为 0.52,表明 iELISA 和 IFAT 检测方法之间存在中度一致性。使用 rRAP-1α 作为抗原的 iELISA 具有优异的特异性和可接受的灵敏度,可以检测到在自然暴露于载体蜱 Rhipicephalus microplus 的牛中的抗巴贝斯虫双联体抗体。通过使用 iELISA-rRAP-1α 以及针对血清样本中的重组裂殖体表面抗原(rMSA-1)的 iELISA 来确定抗 Babesia bovis 的抗体,在墨西哥“La Posta”实验站收集的牛血清样本中,估计了 20.3%的双联体巴贝斯虫血清阳性率和 19.4%的牛巴贝斯虫血清阳性率,而 36.89%的样本同时对这两种巴贝斯虫呈阳性。iELISA 检测有望成为一种安全且低成本的诊断方法,可供墨西哥的牛养殖户使用,并有助于确定牛群的免疫状态,以实施适合预防牛巴贝斯虫病爆发的控制措施。

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