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用于质谱处理的高滴度朊病毒会使朊病毒感染性失活。

Processing of high-titer prions for mass spectrometry inactivates prion infectivity.

机构信息

Rocky Mountain Laboratories, Laboratory of Persistent Viral Disease, National Institute of Allergy & Infectious Diseases, National Institutes of Health, Hamilton, MT, USA.

Rocky Mountain Laboratories, Laboratory of Persistent Viral Disease, National Institute of Allergy & Infectious Diseases, National Institutes of Health, Hamilton, MT, USA.

出版信息

Biochim Biophys Acta Proteins Proteom. 2018 Nov;1866(11):1174-1180. doi: 10.1016/j.bbapap.2018.08.004. Epub 2018 Aug 20.

Abstract

Prions represent a class of universally fatal and transmissible neurodegenerative disorders that affect humans and other mammals. The prion agent contains a pathologically aggregated form of the host prion protein that can transmit infectivity without any bacterial or viral component and is thus difficult to inactivate using disinfection protocols designed for infectious microorganisms. Methods for prion inactivation include treatment with acids, bases, detergents, bleach, prolonged autoclaving and incineration. During these procedures, the sample is often either destroyed or damaged such that further analysis for research purposes is compromised. In this study we show that a straightforward denaturation and in-gel protease digestion protocol used to prepare prion-infected samples for mass spectroscopy leads to the loss of at least 7 logs of prion infectivity, yielding a final product that fails to transmit prion disease in vivo. We further show that the resultant sample remains suitable for mass spectrometry-based protein identifications. Thus, the procedure described can be used to prepare prion-infected samples for mass spectrometry analysis with greatly reduced biosafety concerns.

摘要

朊病毒代表了一类普遍致命且可传播的神经退行性疾病,可影响人类和其他哺乳动物。朊病毒制剂包含一种病理性聚集的宿主朊病毒蛋白,它可以在没有任何细菌或病毒成分的情况下传播感染性,因此很难使用针对传染性微生物设计的消毒方案来灭活。朊病毒的灭活方法包括用酸、碱、去污剂、漂白剂、长时间高压灭菌和焚烧处理。在此过程中,样品通常会被破坏或损坏,从而影响进一步的研究分析。在这项研究中,我们表明,一种简单的变性和胶内蛋白酶消化方案,用于准备用于质谱分析的朊病毒感染样品,会导致朊病毒感染性至少降低 7 个对数级,从而产生最终产物,该产物无法在体内传播朊病毒疾病。我们进一步表明,所得样品仍然适用于基于质谱的蛋白质鉴定。因此,所描述的方法可用于准备用于质谱分析的朊病毒感染样品,而大大降低生物安全风险。

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