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利用一株识别由鼠 PrP 的 aa119-127 组成的区域的 mAb 来描绘朊病毒感染细胞中 PrP(Sc)的细胞内定位。

Characterization of intracellular localization of PrP(Sc) in prion-infected cells using a mAb that recognizes the region consisting of aa 119-127 of mouse PrP.

机构信息

Laboratory of Veterinary Hygiene, Graduate School of Veterinary Medicine, Hokkaido University, Kita 18, Nishi 9, Kita-ku, Sapporo 060-0818, Japan.

Department of Molecular Infectiology, Graduate School of Medicine, Chiba University, 1-8-1 Inohana, Chiba 260-8670, Japan.

出版信息

J Gen Virol. 2012 Mar;93(Pt 3):668-680. doi: 10.1099/vir.0.037101-0. Epub 2011 Nov 16.

Abstract

Generation of an abnormal isoform of the prion protein (PrP(Sc)) is a key aspect of the propagation of prions. Elucidation of the intracellular localization of PrP(Sc) in prion-infected cells facilitates the understanding of the cellular mechanism of prion propagation. However, technical improvement in PrP(Sc)-specific detection is required for precise analysis. Here, we show that the mAb 132, which recognizes the region adjacent to the most amyloidogenic region of PrP, is useful for PrP(Sc)-specific detection by immunofluorescence assay in cells pre-treated with guanidine thiocyanate. Extensive analysis of the intracellular localization of PrP(Sc) in prion-infected cells using mAb 132 revealed the presence of PrP(Sc) throughout endocytic compartments. In particular, some of the granular PrP(Sc) signals that were clustered at peri-nuclear regions appeared to be localized in an endocytic recycling compartment through which exogenously loaded transferrin, shiga and cholera toxin B subunits were transported. The granular PrP(Sc) signals at peri-nuclear regions were dispersed to the peripheral regions including the plasma membrane during incubation at 20 °C, at which temperature transport from the plasma membrane to peri-nuclear regions was impaired. Conversely, dispersed PrP(Sc) signals appeared to return to peri-nuclear regions within 30 min during subsequent incubation at 37 °C, following which PrP(Sc) at peri-nuclear regions appeared to redisperse again to peripheral regions over the next 30 min incubation. These results suggest that PrP(Sc) is dynamically transported along with the membrane trafficking machinery of cells and that at least some PrP(Sc) circulates between peri-nuclear and peripheral regions including the plasma membrane via an endocytic recycling pathway.

摘要

异常朊病毒蛋白 (PrP(Sc)) 的产生是朊病毒传播的关键方面。阐明朊病毒感染细胞中 PrP(Sc) 的细胞内定位有助于理解朊病毒传播的细胞机制。然而,需要改进 PrP(Sc) 特异性检测技术,以进行精确分析。在这里,我们展示了 mAb 132,它识别靠近 PrP 最淀粉样变性区域的区域,通过用硫氰酸胍预处理的细胞中的免疫荧光测定法,对于 PrP(Sc) 特异性检测非常有用。使用 mAb 132 对朊病毒感染细胞中 PrP(Sc) 的细胞内定位进行了广泛分析,结果表明 PrP(Sc) 存在于整个内吞体隔室中。特别是,一些聚集在核周区域的颗粒状 PrP(Sc) 信号似乎定位于通过外源性加载转铁蛋白、志贺毒素和霍乱毒素 B 亚基的内吞体再循环隔室中。在 20°C 孵育期间,核周区域的颗粒状 PrP(Sc) 信号分散到包括质膜在内的外周区域,在该温度下,从质膜到核周区域的运输受到损害。相反,在随后在 37°C 下孵育 30 分钟期间,分散的 PrP(Sc) 信号似乎返回核周区域,随后核周区域的 PrP(Sc) 似乎再次在接下来的 30 分钟孵育期间重新分散到外周区域。这些结果表明,PrP(Sc) 与细胞的膜运输机制一起动态运输,并且至少一些 PrP(Sc) 通过内吞体再循环途径在核周和包括质膜在内的外周区域之间循环。

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