首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Processing and microfiltration of mosquitoes for malaria antigen detection in a rapid dot immunobinding assay.
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Processing and microfiltration of mosquitoes for malaria antigen detection in a rapid dot immunobinding assay.

机译:蚊子的处理和微滤用于快速点免疫结合测定中的疟疾抗原检测。

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摘要

Data on a technique for the detection of antigen from arthropod vectors in a dot immunobinding assay are presented. In this system, antigen present in the vector was first solubilized in sodium dodecyl sulfate. The homogenate from this process was microfiltered through a two-membrane sandwich; target antigen molecules passed through the first membrane and were immobilized on the second one. The first membrane was nonbinding and served to impinge debris. The second membrane was a high-protein-binding-capacity hydrophobic polyvinylidene difluoride membrane. High signal-to-noise ratios were produced by this method, which is readily adaptable for field use. This assay was used for malaria sporozoites, but it can serve as a general technique that is applicable to other arthropod vectors and etiologic agents.
机译:提出了关于在点免疫结合测定中从节肢动物载体中检测抗原的技术的数据。在该系统中,首先将存在于载体中的抗原溶解在十二烷基硫酸钠中。该过程的匀浆通过两层膜三明治微滤;靶抗原分子穿过第一个膜并固定在第二个膜上。第一膜是不结合的并且用于撞击碎屑。第二膜是高蛋白结合能力的疏水性聚偏二氟乙烯膜。通过这种方法产生了很高的信噪比,很容易适应现场使用。该测定法用于疟疾子孢子,但是它可以作为适用于其他节肢动物载体和病原体的通用技术。

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