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Detection of Sarcocystis aucheniae in blood of llama using a duplex semi-nested PCR assay and its association with cyst infestation

机译:半双工PCR检测羊驼血液中的奥氏囊藻及其与囊肿的关系

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摘要

The protozoon Sarcocystis aucheniae is the causative agent of South American camelid (SAC) sarcocystosis. Infections are characterized by the presence of cysts in muscles which are in size and appearance similar to rice grains. As consumption of insufficiently cooked infected meat produces gastroenteritis, cyst-containing SAC meat is confiscated by sanitary authorities or depreciated with serious economic consequences for SAC breeders. In this work, a duplex semi-nested PCR was designed to simultaneously detect parasite and llama DNA in host blood samples. Species-specific regions of S. aucheniae 18S rRNA gene and Lama glama 16S mitochondrial gene were amplified, yielding bands of 583 and 257 bp, respectively, and separated by gel electrophoresis. The method proved to be highly sensitive, with a detection limit lower than one parasite per milliliter blood, and the inclusion of primers to detect llama-specific DNA resulted useful as a methodological control. Blood samples collected from llamas of Argentina and Bolivia (n = 225) were analyzed using this method, and 18.7 % resulted positive for S. aucheniae. No correlation was found between PCR results and llama age, sex or the finding of macroscopic cysts in meat after slaughter. Lack of molecular detection in the blood of some llamas harboring macrocysts suggests that parasite circulation in the bloodstream after encystment is under the detection threshold of the test or even absent, while PCR positive results in cyst-infested animals suggests that prior exposure to the parasite does not impede subsequent infections. The described method can be useful to detect active foci of infection, to assess the effectiveness of parasiticide treatments, and for the surveillance and tracing of definitive hosts.
机译:原生动物Sarcocystis aucheniae是南美骆驼科(SAC)结囊病的病原体。感染的特征是肌肉中存在囊肿,囊肿的大小和外观与米粒相似。由于食用未煮熟的受感染肉会引起肠胃炎,卫生当局会没收含有囊肿的SAC肉,或者贬值对SAC育种者造成严重的经济后果。在这项工作中,设计了一种双联半嵌套式PCR,以同时检测宿主血液样本中的寄生虫和美洲驼DNA。扩增了葡萄球菌18S rRNA基因和喇嘛喇嘛16S线粒体基因的物种特异性区域,分别产生了583和257 bp的条带,并通过凝胶电泳进行了分离。该方法被证明是高度灵敏的,检出限低于每毫升血液中一个寄生虫,并且包含用于检测美洲驼特异性DNA的引物可作为方法学对照。使用这种方法分析了从阿根廷和玻利维亚的骆驼采集的血液样本(n = 225),其中18.7%的结果为奥氏假单胞菌阳性。 PCR结果与美洲驼年龄,性别或屠宰后肉中肉眼可见的囊肿之间没有相关性。一些带有大囊的美洲驼血液中分子检测不足,表明囊肿后囊体内血液中的寄生虫循环低于测试的检测阈值,甚至不存在,而囊肿感染动物的PCR阳性结果表明,事先暴露于寄生虫中确实不妨碍后续感染。所描述的方法可用于检测感染的活跃病灶,评估杀寄生虫剂治疗的有效性以及用于确定宿主的监测和追踪。

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