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PMCA 证明了在可重复使用医疗器械上朊病毒失活方法的有效性:替代动物生物检测的相关方法。

PMCA to demonstrate the efficacy of prion inactivation methods on reusable medical devices: a relevant alternative to animal bioassays.

机构信息

Molecular Virology Immunology Unit, Université Paris-Saclay, INRAE, UVSQ, Jouy-en-Josas, France.

Advanced Sterilization Products, Irvine, CA, USA.

出版信息

J Hosp Infect. 2024 Dec;154:60-63. doi: 10.1016/j.jhin.2024.07.020. Epub 2024 Sep 30.

DOI:10.1016/j.jhin.2024.07.020
PMID:39357541
Abstract

Validation of prion inactivation processes for medical devices relies on in-vivo experimental protocols. However, bioassays are costly, long (1-2 years) and ethically disputable. Additionally, results obtained with one prion strain - for example, 263K (hamster-adapted strain originating from sheep scrapie) - cannot be easily extrapolated to relevant human prion strains, further questioning the utility of bioassays. Over the past two decades, cell-free prion amplification assays have emerged as potential alternatives to bioassays. Rather than measuring prion infectivity, they quantify prion seeding activity (i.e. the capacity to convert the normal prion protein into the disease-associated isoform). The results obtained from an optimized cell-free assay termed 'miniaturized-bead protein misfolding cyclic amplification' (mb-PMCA) with four processes using three different prion strains - 263K and two human prions derived from variant and sporadic Creutzfeldt-Jakob disease - were compared with published bioassays using the same three strains and processes, when available. Tests performed on reference processes (steam, sodium hydroxide, sodium hypochlorite) and low temperature HO sterilization (STERRAD NX Advanced cycle) showed perfect alignment between mb-PMCA and available bioassays. STERRAD NX Advanced cycle was efficacious against all three prion strains. These data confirm that PMCA, particularly mb-PMCA, is a relevant alternative to animal bioassays for the assessment of prion inactivation processes, and highlight the interest of some low temperature HO sterilization cycles.

摘要

医疗器械中朊病毒灭活过程的验证依赖于体内实验方案。然而,生物测定法既昂贵又耗时(1-2 年),且在伦理上存在争议。此外,用一种朊病毒株(例如 263K(源自绵羊瘙痒病的仓鼠适应株))获得的结果不能轻易外推到相关的人类朊病毒株,这进一步质疑了生物测定法的实用性。在过去的二十年中,无细胞朊病毒扩增测定法已成为生物测定法的潜在替代方法。它们不是测量朊病毒感染性,而是量化朊病毒接种活性(即将正常朊病毒蛋白转化为疾病相关异构体的能力)。用优化的无细胞测定法“微型化珠蛋白错误折叠循环扩增”(mb-PMCA)获得的结果,该测定法使用三种不同的朊病毒株(263K 和两种源自变异型和散发性克雅氏病的人类朊病毒)进行了四个过程,与使用相同三种菌株和过程的已发表生物测定法进行了比较,在可用的情况下。对参考过程(蒸汽、氢氧化钠、次氯酸钠)和低温 HO 灭菌(STERRAD NX 高级循环)进行的测试表明,mb-PMCA 与可用的生物测定法完全一致。STERRAD NX 高级循环对所有三种朊病毒株均有效。这些数据证实 PMCA,特别是 mb-PMCA,是评估朊病毒灭活过程的动物生物测定法的一种相关替代方法,并强调了一些低温 HO 灭菌循环的重要性。

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