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Expression analysis and biological characterization of Babesia sp BQ1 (Lintan) (Babesia motasi-like) rhoptry-associated protein 1 and its potential use in serodiagnosis via ELISA

机译:巴贝斯菌BQ1(Lintan)(巴贝斯motasi-like)流变相关蛋白1的表达分析和生物学特性及其在ELISA血清学诊断中的潜在应用

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摘要

Background: In China, ovine babesiosis is one of the most important tick-borne haemoparasitic diseases of small ruminants. It has a significant economic impact, and several Babesia motasi-like isolates have been recently shown to be responsible for ovine babesiosis in this country. Methods: Full-length and C-terminal-truncated forms of the rap-1a61-1 gene of Babesia sp. BQ1 (Lintan) were cloned into the pET-30a plasmid and subsequently expressed as His-fusion proteins. The resulting recombinant RAP-1a proteins (rRAP-1a61-1 and rRAP-1a61-1/CT) were purified and evaluated as diagnostic antigens using Western blot analysis and ELISA. The native Babesia sp. BQ1 (Lintan) RAP-1 protein was recognized using Western blots and IFAT by antibodies that were raised in rabbits against rRAP-1a61-1/CT. The specificity, sensitivity and positive threshold values for rRAP-1a61-1/CT in ELISA were evaluated. Results: Cross-reactivity was observed between rRAP-1a61-1/CT and positive sera for Babesia sp. BQ1 (Lintan), Babesia sp. BQ1 (Ningxian) and Babesia sp. Tianzhu isolates obtained from infected sheep. At one week post-inoculation, a significant increase was observed in the amount of antibodies produced against RAP-1a, and high levels of antibodies against RAP-1a were observed for 3 months (at 84 days p.i.). A total of 3198 serum samples were collected from small ruminants in 54 different regions in 23 provinces of China. These samples were tested using ELISA based on the rRAP-1a61-1/CT protein. The results indicated that the average positive rate was 36.02 %. Conclusions: The present study suggests that rRAP-1a61-1/CT might be a potential diagnostic antigen for detecting several isolates of B. motasi-like parasites infection.
机译:背景:在中国,羊杆状杆菌病是小反刍动物最重要的tick传血寄生虫病之一。它具有重大的经济影响,最近已证明该国有数个像巴贝斯(Babesia)motasi样的分离物与绵羊贝贝病有关。方法:巴贝斯虫的rap-1a61-1基因的全长和C末端截短形式。将BQ1(Lintan)克隆到pET-30a质粒中,然后表达为His-fusion蛋白。纯化得到的重组RAP-1a蛋白(rRAP-1a61-1和rRAP-1a61-1 / CT),并使用Western blot分析和ELISA将其评估为诊断抗原。原生巴贝斯虫。 BQ1(Lintan)RAP-1蛋白已通过Western印迹和IFAT被兔抗rRAP-1a61-1 / CT产生的抗体识别。评价了rRAP-1a61-1 / CT在ELISA中的特异性,敏感性和阳性阈值。结果:在rRAP-1a61-1 / CT和Babesia sp的阳性血清之间观察到交叉反应。 BQ1(林丹),Babesia sp。 BQ1(宁县)和巴贝斯虫。从被感染的绵羊身上获得天竺分离株。接种后一周,观察到针对RAP-1a的抗体产生量显着增加,并且针对RAP-1a的抗体水平持续3个月(p.i.为84天)被观察到。从中国23个省的54个不同地区的小反刍动物中收集了3198份血清样品。使用基于rRAP-1a61-1 / CT蛋白的ELISA测试这些样品。结果表明,平均阳性率为36.02%。结论:本研究表明,rRAP-1a61-1 / CT可能是检测几种分离的B. motasi样寄生虫感染的潜在诊断抗原。

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