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Development of Real Time PCR to Study Experimental Mixed Infections of T. congolense Savannah and T. b. brucei in Glossina morsitans morsitans

机译:实时PCR技术的发展以研究浓密线虫萨凡纳和T. b。的实验性混合感染。布鲁斯在格拉西纳(Glossina morsitans)中

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摘要

Tsetse flies are able to acquire mixed infections naturally or experimentally either simultaneously or sequentially. Traditionally, natural infection rates in tsetse flies are estimated by microscopic examination of different parts of the fly after dissection, together with the isolation of the parasite in vivo. However, until the advent of molecular techniques it was difficult to speciate trypanosomes infections and to quantify trypanosome numbers within tsetse flies. Although more expensive, qPCR allows the quantification of DNA and is less time consuming due to real time visualization and validation of the results. The current study evaluated the application of qPCR to quantify the infection load of tsetse flies with T. b. brucei and T. congolense savannah and to study the possibility of competition between the two species. The results revealed that the two qPCR reactions are of acceptable efficiency (99.1% and 95.6%, respectively), sensitivity and specificity and can be used for quantification of infection load with trypanosomes in experimentally infected Glossina morsitans morsitans. The mixed infection of laboratory Glossina species and quantification of the infection suggests the possibility that a form of competition exists between the isolates of T. b. brucei and T. congolense savannah that we used when they co-exist in the fly midgut.
机译:采采蝇能够同时或依次自然或通过实验获得混合感染。传统上,采采蝇的自然感染率是通过解剖后的蝇蝇不同部位的显微镜检查以及体内寄生虫的分离来估算的。但是,直到分子技术出现之前,很难确定采采蝇中的锥虫感染和定量锥虫数量。尽管更昂贵,但由于实时可视化和结果验证,qPCR可以对DNA进行定量,并且耗时较少。目前的研究评估了qPCR在定量测定采采蝇对T.b感染量方面的应用。 Brucei和T. congolense稀树草原,并研究这两个物种之间竞争的可能性。结果表明,这两个qPCR反应具有可接受的效率(分别为99.1%和95.6%),敏感性和特异性,可用于量化实验感染的Glossina morsitans morsitans中锥虫的感染量。实验室Glossina物种的混合感染和定量感染表明,在T. b。分离株之间存在竞争形式的可能性。当它们在苍蝇中肠中共存时,我们使用的是布鲁塞和T. congolense萨凡纳。

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