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首页> 外文期刊>Journal of Clinical Microbiology >Development and Evaluation of a Seminested PCR for Detection and Differentiation of Babesia gibsoni (Asian Genotype) and B. canis DNA in Canine Blood Samples
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Development and Evaluation of a Seminested PCR for Detection and Differentiation of Babesia gibsoni (Asian Genotype) and B. canis DNA in Canine Blood Samples

机译:半巢式PCR的开发和评估,用于检测和区分犬血样中的巴贝斯希氏小球藻(亚洲基因型)和犬双歧杆菌DNA

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Canine babesiosis has recently been recognized as an emerging infectious disease of dogs in North America. We sought to develop a seminested PCR to detect and differentiate Babesia gibsoni (Asian genotype), B. canis subsp. vogeli, B. canis subsp. canis, and B. canis subsp. rossi DNA in canine blood samples. An outer primer pair was designed to amplify an ~340-bp fragment of the 18S rRNA genes from B. gibsoni (Asian genotype), B. canis subsp. vogeli, B. canis subsp. rossi, and B. canis subsp. canis but not mammalian DNA. Forward primers were designed that would specifically amplify a smaller fragment from each organism in a seminested PCR. The practical limit of detection was 50 organisms/ml of mock-infected EDTA anticoagulated whole blood. The primer pair also amplified an ~370-bp fragment of the B. gibsoni (USA/California genotype) 18S rRNA gene from the blood of an experimentally infected dog with a high percentage of parasitemia. Amplicons were not detected when DNA extracted from the blood of a dog that was naturally infected with Theileria annae at a low percentage of parasitemia was amplified. Due to limited sensitivity, this test is not recommended for the routine diagnosis of B. gibsoni (USA/California genotype) or T. annae. The PCR test did not amplify Toxoplasma gondii, Neospora caninum, Leishmania infantum, Cryptosporidium parvum, or canine DNA under any of the conditions tested. The seminested PCR test was able to detect and discriminate B. gibsoni (Asian genotype), B. canis subsp. vogeli, B. canis subsp. canis, and B. canis subsp. rossi DNA in blood samples from infected dogs.
机译:犬幼犬病最近在北美被公认为是一种新兴的犬传染病。我们试图开发一种半巢式PCR,以检测和区分 Babesia gibsoni (亚洲基因型) B。犬子亚种。 vogeli B。犬子亚种。 canis B。犬子亚种。犬血液样本中的 rossi DNA。设计了一个外引物对,以扩增来自 B的18S rRNA基因的〜340 bp片段。 gibsoni (亚洲基因型), B。犬子亚种。 vogeli B。犬子亚种。 rossi B。犬子亚种。 canis ,但不是哺乳动物的DNA。设计了正向引物,可以在半巢式PCR中特异性扩增每个生物体的较小片段。实际检测极限是50个生物体/毫升模拟感染的EDTA抗凝全血。引物对还扩增了 B的〜370-bp片段。 gibsoni (美国/加利福尼亚的基因型),来自实验感染的狗中寄生虫率高的狗血液中的18S rRNA基因。当从寄生虫率低的自然感染 Theanna annae 的狗的血液中提取的DNA扩增时,未扩增出扩增子。由于灵敏度有限,因此不建议将该测试用于 B的常规诊断。 gibsoni (美国/加利福尼亚的基因型)或 T。安娜。 PCR测试未扩增弓形虫新孢子虫婴儿利什曼原虫隐孢子虫或犬DNA任何测试条件。半嵌套式PCR测试能够检测和区分B。 gibsoni (亚洲基因型), B。犬子亚种。 vogeli B。犬子亚种。 canis B。犬子亚种。感染犬血液样本中的 rossi DNA。

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