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Comparison of the sensitivity of in vivo antibody production tests with in vitro PCR-based methods to detect infectious contamination of biological materials

机译:比较体内抗体生产测试与基于体外PCR的方法检测生物材料的传染性污染的敏感性

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摘要

Bacteria and viruses may be transmitted to laboratory rodents by contaminated biological materials such as transplantable tumours, cell lines, sera or other biological materials. Biological materials are currently being screened using the mouse or rat antibody production (MAP/RAP) test (serological testing). We decided to test and validate an alternative assay using polymerase chain reaction (PCR/realtime PCR) technology to detect viral contamination directly in biological material. The aim of this study therefore is the validation of our new PCR assays and the comparison of PCR and the MAP test. For 8/14 viruses, conventional PCR was more sensitive and more specific than the MAP test in detecting murine viruses. For 12/14 viruses, the realtime PCR was more sensitive than the MAP test. In 2/14 cases, all three detection methods had the same sensitivity. Furthermore, PCR screening clearly conforms to the principles of the 3Rs as a replacement technique because it eliminates the need for using animals to screen for murine viruses in biological material.
机译:细菌和病毒可能通过受污染的生物材料(例如可移植的肿瘤,细胞系,血清或其他生物材料)传播到实验室啮齿动物。目前正在使用小鼠或大鼠抗体产生(MAP / RAP)测试(血清学测试)来筛选生物材料。我们决定使用聚合酶链反应(PCR /实时PCR)技术测试并验证一种替代检测方法,以直接检测生物材料中的病毒污染。因此,本研究的目的是验证我们新的PCR分析方法以及PCR和MAP试验的比较。对于8/14病毒,常规PCR在检测鼠类病毒方面比MAP测试更灵敏,更特异性。对于12/14病毒,实时PCR比MAP测试更敏感。在2/14情况下,所有三种检测方法均具有相同的灵敏度。此外,PCR筛选显然符合3Rs的替代技术原理,因为它无需使用动物来筛选生物材料中的鼠病毒。

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