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用部分纯化的底物和合成聚阴离子重建蛋白酶抗性朊病毒蛋白扩增。

Protease-resistant prion protein amplification reconstituted with partially purified substrates and synthetic polyanions.

作者信息

Deleault Nathan R, Geoghegan James C, Nishina Koren, Kascsak Richard, Williamson R Anthony, Supattapone Surachai

机构信息

Department of Biochemistry, Dartmouth Medical School, Hanover, New Hampshire 03755, USA.

出版信息

J Biol Chem. 2005 Jul 22;280(29):26873-9. doi: 10.1074/jbc.M503973200. Epub 2005 May 24.

Abstract

Little is currently known about the biochemical mechanism by which induced prion protein (PrP) conformational change occurs during mammalian prion propagation. In this study, we describe the reconstitution of PrPres amplification in vitro using partially purified and synthetic components. Overnight incubation of purified PrP27-30 and PrPC molecules at a molar ratio of 1:250 yielded approximately 2-fold baseline PrPres amplification. Addition of various polyanionic molecules increased the level of PrPres amplification to approximately 10-fold overall. Polyanionic compounds that stimulated purified PrPres amplification to varying degrees included synthetic, homopolymeric nucleic acids such as poly(A) and poly(dT), as well as non-nucleic acid polyanions, such as heparan sulfate proteoglycan. Size fractionation experiments showed that synthetic poly(A) polymers must be >0.2 kb in length to stimulate purified PrPres amplification. Thus, one possible set of minimal components for efficient conversion of PrP molecules in vitro may be surprisingly simple, consisting of PrP27-30, PrPC, and a stimulatory polyanionic compound.

摘要

目前对于哺乳动物朊病毒传播过程中诱导朊病毒蛋白(PrP)构象变化的生化机制知之甚少。在本研究中,我们描述了使用部分纯化的和合成的成分在体外重建PrPres扩增。将纯化的PrP27-30和PrPC分子以1:250的摩尔比过夜孵育,产生了约2倍的基线PrPres扩增。添加各种聚阴离子分子使PrPres扩增水平总体提高到约10倍。不同程度刺激纯化PrPres扩增的聚阴离子化合物包括合成的同聚核酸,如聚(A)和聚(dT),以及非核酸聚阴离子,如硫酸乙酰肝素蛋白聚糖。尺寸分级实验表明,合成的聚(A)聚合物长度必须>0.2 kb才能刺激纯化的PrPres扩增。因此,体外高效转化PrP分子的一组可能的最小成分可能出奇地简单,由PrP27-30、PrPC和一种刺激性聚阴离子化合物组成。

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