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A rapid and sensitive intracellular flow cytometric assay to identify Theileria parva infection within target cells

机译:一种快速灵敏的细胞内流式细胞仪检测方法,用于鉴定靶细胞内的Theileria parva感染

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摘要

Theileria parva is an intracellular protozoan parasite transmitted by ticks that causes a fatal lymphoproliferative disease of cattle known as East Coast Fever. Vaccination against the disease currently relies on inoculation of the infective sporozoite stage of the parasite and simultaneous treatment with long-acting formulations of oxytetracycline. Sporozoites are maintained as frozen stabilates of triturated infected ticks and the method requires accurate titration of stabilates to determine appropriate dose rates. Titration has traditionally been undertaken in cattle and requires large numbers of animals because of individual variation in susceptibility to infection. An alternative tissue culture-based method is laborious and time consuming. We have developed a flow cytometric method for quantifying the infectivity of sporozoite stabilates in vitro based on the detection of intracellular parasite antigen. The method allows clear identification of parasitized cells with a high degree of sensitivity and specificity. Analysis of infected cells between 48 and 72 h post-infection clearly defines the potential transforming capability of different stabilates.
机译:泰勒虫幼虫是由壁虱传播的细胞内原生动物寄生虫,可导致牛的致命性淋巴增生性疾病,称为东海岸热。目前,针对该疾病的疫苗接种依赖于寄生虫感染性子孢子期的接种以及用土霉素的长效制剂同时治疗。将子孢子维持为磨碎的感染infected的冷冻稳定剂,并且该方法需要精确滴定稳定剂以确定合适的剂量率。传统上在牛中进行滴定,由于感染敏感性的个体差异,需要大量的动物。另一种基于组织培养的方法既费力又费时。我们已经开发了一种流式细胞术方法,用于基于细胞内寄生虫抗原的检测定量体外子孢子稳定剂的感染性。该方法允许以高度的敏感性和特异性清楚地鉴定被寄生的细胞。感染后48至72小时之间对感染细胞的分析清楚地定义了不同稳定剂的潜在转化能力。

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