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Quantitative Detection and Biological Propagation of Scrapie Seeding Activity In Vitro Facilitate Use of Prions as Model Pathogens for Disinfection

机译:Sc草种子活性的体外定量检测和生物繁殖促进了使用ions病毒作为模型病原菌进行消毒

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摘要

Prions are pathogens with an unusually high tolerance to inactivation and constitute a complex challenge to the re-processing of surgical instruments. On the other hand, however, they provide an informative paradigm which has been exploited successfully for the development of novel broad-range disinfectants simultaneously active also against bacteria, viruses and fungi. Here we report on the development of a methodological platform that further facilitates the use of scrapie prions as model pathogens for disinfection. We used specifically adapted serial protein misfolding cyclic amplification (PMCA) for the quantitative detection, on steel wires providing model carriers for decontamination, of 263K scrapie seeding activity converting normal protease-sensitive into abnormal protease-resistant prion protein. Reference steel wires carrying defined amounts of scrapie infectivity were used for assay calibration, while scrapie-contaminated test steel wires were subjected to fifteen different procedures for disinfection that yielded scrapie titre reductions of ≤101- to ≥105.5-fold. As confirmed by titration in hamsters the residual scrapie infectivity on test wires could be reliably deduced for all examined disinfection procedures, from our quantitative seeding activity assay. Furthermore, we found that scrapie seeding activity present in 263K hamster brain homogenate or multiplied by PMCA of scrapie-contaminated steel wires both triggered accumulation of protease-resistant prion protein and was further propagated in a novel cell assay for 263K scrapie prions, i.e., cerebral glial cell cultures from hamsters. The findings from our PMCA- and glial cell culture assays revealed scrapie seeding activity as a biochemically and biologically replicative principle in vitro, with the former being quantitatively linked to prion infectivity detected on steel wires in vivo. When combined, our in vitro assays provide an alternative to titrations of biological scrapie infectivity in animals that substantially facilitates the use of prions as potentially highly indicative test agents in the search for novel broad-range disinfectants.
机译:ions病毒是对灭活具有异常高耐受性的病原体,对外科器械的再加工构成了复杂的挑战。但是,另一方面,它们提供了一种信息范例,已被成功地用于开发同时对细菌,病毒和真菌也具有活性的新型大范围消毒剂。在这里,我们报告了一种方法平台的发展,该平台进一步促进了瘙痒病pr病毒作为模型病原体的消毒使用。我们使用了经过特殊调整的系列蛋白质错折叠循环扩增(PMCA),在提供去污模型载体的钢丝上对263K刮scrap种子接种活性进行了定量检测,从而将正常的蛋白酶敏感性转化为抗蛋白酶的abnormal病毒蛋白。使用带有确定量的瘙痒病感染性的参考钢丝进行测定校准,同时对被瘙痒病污染的测试钢丝进行十五种不同的消毒程序,以使瘙痒病的滴度降低≤10 1 -至≥10 5.5 倍。如通过仓鼠滴定法所证实的,从我们的定量播种活性分析中,可以可靠地推断出所有已检验的消毒程序中测试线上残留的瘙痒病传染性。此外,我们发现存在于263K仓鼠大脑匀浆中的痒病接种活性或乘以受痒病污染的钢丝的PMCA均触发了蛋白酶抗性病毒蛋白的积累,并在针对263K痒病ions病毒的新型细胞测定中进一步传播,即仓鼠的神经胶质细胞培养。我们的PMCA和神经胶质细胞培养测定法的发现表明,瘙痒病的播种活性是体外的生物化学和生物学复制原理,前者与体内在钢丝上检测到的病毒感染性存在定量联系。当结合使用时,我们的体外测定法可替代滴定动物中生物瘙痒病感染性的方法,从而极大地促进了病毒在寻找新型大范围消毒剂中作为潜在的高度指示性测试剂的使用。

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