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Low Density Subcellular Fractions Enhance Disease-specific Prion Protein Misfolding

机译:低密度亚细胞部分增强疾病特异性Disease蛋白错折叠

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摘要

The production of prion particles in vitro by amplification with or without exogenous seed typically results in infectivity titers less than those associated with PrPSc isolated ex vivo and highlights the potential role of co-factors that can catalyze disease-specific prion protein misfolding in vivo. We used a cell-free conversion assay previously shown to replicate many aspects of transmissible spongiform encephalopathy disease to investigate the cellular location of disease-specific co-factors using fractions derived from gradient centrifugation of a scrapie-susceptible cell line. Fractions from the low density region of the gradient doubled the efficiency of conversion of recombinant PrP. These fractions contain plasma membrane and cytoplasmic proteins, and conversion enhancement can be achieved using PrPSc derived from two different strains of mouse-passaged scrapie as seed. Equivalent fractions from a second scrapie-susceptible cell line also stimulate conversion. We also show that subcellular fractions enhancing disease-specific prion protein conversion prevent in vitro fibrillization of recombinant prion protein, suggesting the existence of separate, competing mechanisms of disease-specific and nonspecific misfolding in vivo.
机译:通过在有或没有外源种子的情况下进行扩增而在体外产生pr病毒颗粒时,其感染力滴度通常低于离体离体的PrP Sc 所产生的滴度,并突显了可催化疾病的辅因子的潜在作用。体内特异性病毒蛋白错误折叠。我们使用无细胞转化试验,先前证实可复制可传播性海绵状脑病的许多方面,以使用对瘙痒病敏感细胞系进行梯度离心的馏分研究疾病特异性辅因子的细胞位置。来自梯度低密度区域的馏分使重组PrP的转化效率提高了一倍。这些级分包含质膜和细胞质蛋白,并且可以使用来源于两种不同的小鼠传代瘙痒病菌株的PrP Sc 作为种子来实现转化增强。来自第二瘙痒病易感细胞系的等价馏分也刺激转化。我们还显示,增强疾病特异性病毒蛋白转化的亚细胞级分可阻止重组病毒蛋白的体外原纤维化,提示存在疾病特异性和非特异性错折叠的独立,竞争机制。

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