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基于对强荧光靶点的扫描,通过高通量筛选系统鉴定抗朊病毒药物。

Systematic identification of antiprion drugs by high-throughput screening based on scanning for intensely fluorescent targets.

作者信息

Bertsch Uwe, Winklhofer Konstanze F, Hirschberger Thomas, Bieschke Jan, Weber Petra, Hartl F Ulrich, Tavan Paul, Tatzelt Jörg, Kretzschmar Hans A, Giese Armin

机构信息

Zentrum für Neuropathologie und Prionforschung, Ludwig Maximilians Universität, Feodor Lynen Str. 23, D-81377 München, Germany.

出版信息

J Virol. 2005 Jun;79(12):7785-91. doi: 10.1128/JVI.79.12.7785-7791.2005.

DOI:10.1128/JVI.79.12.7785-7791.2005
PMID:15919931
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1143673/
Abstract

Conformational changes and aggregation of specific proteins are hallmarks of a number of diseases, like Alzheimer's disease, Parkinson's disease, and prion diseases. In the case of prion diseases, the prion protein (PrP), a neuronal glycoprotein, undergoes a conformational change from the normal, mainly alpha-helical conformation to a disease-associated, mainly beta-sheeted scrapie isoform (PrP(Sc)), which forms amyloid aggregates. This conversion, which is crucial for disease progression, depends on direct PrP(C)/PrP(Sc) interaction. We developed a high-throughput assay based on scanning for intensely fluorescent targets (SIFT) for the identification of drugs which interfere with this interaction at the molecular level. Screening of a library of 10,000 drug-like compounds yielded 256 primary hits, 80 of which were confirmed by dose response curves with half-maximal inhibitory effects ranging from 0.3 to 60 microM. Among these, six compounds displayed an inhibitory effect on PrP(Sc) propagation in scrapie-infected N2a cells. Four of these candidate drugs share an N'-benzylidene-benzohydrazide core structure. Thus, the combination of high-throughput in vitro assay with the established cell culture system provides a rapid and efficient method to identify new antiprion drugs, which corroborates that interaction of PrP(C) and PrP(Sc) is a crucial molecular step in the propagation of prions. Moreover, SIFT-based screening may facilitate the search for drugs against other diseases linked to protein aggregation.

摘要

特定蛋白质的构象变化和聚集是许多疾病的标志,如阿尔茨海默病、帕金森病和朊病毒病。就朊病毒病而言,朊病毒蛋白(PrP)是一种神经元糖蛋白,其构象从正常的主要为α螺旋构象转变为与疾病相关的主要为β折叠的瘙痒病异构体(PrP(Sc)),后者形成淀粉样聚集体。这种转变对于疾病进展至关重要,它依赖于PrP(C)/PrP(Sc)的直接相互作用。我们开发了一种基于扫描强荧光靶点(SIFT)的高通量检测方法,用于鉴定在分子水平上干扰这种相互作用的药物。对一个包含10000种类药物化合物的文库进行筛选,得到了256个初步命中物,其中80个通过剂量反应曲线得到确认,半数最大抑制效应范围为0.3至60微摩尔。在这些命中物中,有六种化合物对瘙痒病感染的N2a细胞中PrP(Sc)的传播显示出抑制作用。其中四种候选药物具有N'-亚苄基苯甲酰肼核心结构。因此,高通量体外检测与已建立的细胞培养系统相结合,提供了一种快速有效的方法来鉴定新的抗朊病毒药物,这证实了PrP(C)和PrP(Sc)的相互作用是朊病毒传播中的一个关键分子步骤。此外,基于SIFT的筛选可能有助于寻找针对其他与蛋白质聚集相关疾病的药物。

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本文引用的文献

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Evaluation of new cell culture inhibitors of protease-resistant prion protein against scrapie infection in mice.新型抗蛋白酶朊病毒蛋白细胞培养抑制剂对小鼠羊瘙痒病感染的评估。
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