用于检测家畜日本血吸虫感染的巢式聚合酶链反应检测法
Nested-PCR assay for detection of Schistosoma japonicum infection in domestic animals.
作者信息
Zhang Xin, He Chuan-Chuan, Liu Jin-Ming, Li Hao, Lu Ke, Fu Zhi-Qiang, Zhu Chuan-Gang, Liu Yi-Ping, Tong Lai-Bao, Zhou De-Bao, Zha Li, Hong Yang, Jin Ya-Mei, Lin Jiao-Jiao
机构信息
Shanghai Veterinary Research Institute, Chinese Academy of Agricultural Sciences, Key Laboratory of Animal Parasitology, Ministry of Agriculture, Shanghai, 200241, People's Republic of China.
Anhui Center for Animal Disease Control and Prevention, Hefei, People's Republic of China.
出版信息
Infect Dis Poverty. 2017 Apr 13;6(1):86. doi: 10.1186/s40249-017-0298-y.
BACKGROUND
Schistosomiasis japonica is a common zoonosis. Domestic animals are the primary source of infection and play an important role in disease transmission. The prevalence and infectivity of this disease in domestic animals in China have significantly decreased and, for this reason, diagnostics with a higher sensitivity have become increasingly necessary. It was reported that polymerase chain reaction (PCR)-based methods could be used to detect schistosome infection in humans and animals and presented a high sensitivity and specificity. The present study aimed to develop a PCR-based method for detection of Schistosoma japonicum infection in domestic animals.
METHODS
A specific nested-PCR assay was developed to detect S. japonicum infection in domestic animals via amplification of a 231-bp DNA fragment of retrotransposon SjR2. The developed assay was first used in sera and dry blood filter paper (DBFP) from goats and buffaloes at different time points of infection. Then, 78 DBFPs from 39 artificially-infected bovines at 14 and 28 days post-infection and 42 DBFPs from schistosome-negative bovines from the city of Huangshan in the Anhui province were used to evaluate the diagnostic validity. Furthermore, this assay was used to detect S. japonicum infection in domestic animals in Dongzhi and Wangjiang counties.
RESULTS
The expected PCR product was detected in eggs and adult worms of S. japonicum and blood samples from S. japonicum-infected goats and water buffaloes, but not from Fasciola and Haemonchus contortus worms. The nested-PCR assay could detect the target S. japonicum DNA in DBFPs from goats and buffaloes after day 3 post-infection. The sensitivity in buffaloes at 14 and 28 days post-infection was 92.30% (36/39) and 100% (39/39), respectively. The specificity was 97.60% (41/42). The positivity rates in Dongzhi and Wangjiang counties were 6.00% and 8.00% in bovines and 22.00% and 16.67% in goats, respectively. The positivity rates in goats in both counties were higher than those in bovines with a significant difference in Dongzhi County but not in Wangjiang County (P < 0.05 and P = 0.23, respectively).
CONCLUSIONS
Our results suggest that the developed nested-PCR assay may be used for the diagnosis of S. japonicum infection in domestic animals, and the control of S. japonicum infection in goats should be paid more attention.
背景
日本血吸虫病是一种常见的人畜共患病。家畜是主要传染源,在疾病传播中起重要作用。中国家畜中该疾病的流行率和感染性已显著下降,因此,开发具有更高灵敏度的诊断方法变得越来越必要。据报道,基于聚合酶链反应(PCR)的方法可用于检测人和动物的血吸虫感染,且具有高灵敏度和特异性。本研究旨在开发一种基于PCR的方法来检测家畜中的日本血吸虫感染。
方法
开发了一种特异性巢式PCR检测方法,通过扩增反转录转座子SjR2的231bp DNA片段来检测家畜中的日本血吸虫感染。所开发的检测方法首先应用于不同感染时间点山羊和水牛的血清及干血滤纸片(DBFP)。然后,使用来自39头人工感染牛在感染后14天和28天的78份DBFP以及来自安徽省黄山市血吸虫阴性牛的42份DBFP来评估诊断有效性。此外,该检测方法还用于检测东至县和望江县家畜中的日本血吸虫感染。
结果
在日本血吸虫的虫卵和成虫以及感染日本血吸虫的山羊和水牛的血液样本中检测到预期的PCR产物,但在肝片吸虫和捻转血矛线虫中未检测到。巢式PCR检测方法可在感染后第3天检测到山羊和水牛DBFP中的日本血吸虫目标DNA。感染后14天和28天水牛的灵敏度分别为92.30%(36/39)和100%(39/39)。特异性为97.60%(41/42)。东至县和望江县牛的阳性率分别为6.00%和8.00%,山羊的阳性率分别为22.00%和16.67%。两县山羊的阳性率均高于牛,东至县差异显著,望江县差异不显著(P分别为<0.05和P = 0.23)。
结论
我们的结果表明,所开发的巢式PCR检测方法可用于诊断家畜中的日本血吸虫感染,应更加关注山羊日本血吸虫感染的控制。
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