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Prions affect the appearance of other prions: the story of [PIN(+)].朊病毒会影响其他朊病毒的表现:[PIN(+)]的故事。
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本文引用的文献

1
Selfish prion of Rnq1 mutant in yeast.酵母中 Rnq1 突变体的自私朊病毒。
Genes Cells. 2009 May;14(5):659-68. doi: 10.1111/j.1365-2443.2009.01297.x. Epub 2009 Apr 15.
2
Heterologous prion interactions are altered by mutations in the prion protein Rnq1p.朊病毒蛋白Rnq1p中的突变会改变异源朊病毒的相互作用。
J Mol Biol. 2009 May 8;388(3):583-96. doi: 10.1016/j.jmb.2009.03.036. Epub 2009 Mar 24.
3
Chaperone-dependent amyloid assembly protects cells from prion toxicity.伴侣蛋白依赖性淀粉样蛋白组装可保护细胞免受朊病毒毒性的影响。
Proc Natl Acad Sci U S A. 2008 May 20;105(20):7206-11. doi: 10.1073/pnas.0802593105. Epub 2008 May 14.
4
A regulatory role of the Rnq1 nonprion domain for prion propagation and polyglutamine aggregates.Rnq1非朊病毒结构域对朊病毒传播和聚谷氨酰胺聚集体的调控作用。
Mol Cell Biol. 2008 May;28(10):3313-23. doi: 10.1128/MCB.01900-07. Epub 2008 Mar 10.
5
J-protein co-chaperone Sis1 required for generation of [RNQ+] seeds necessary for prion propagation.J蛋白共伴侣Sis1是朊病毒传播所需的[RNQ+]种子生成所必需的。
EMBO J. 2007 Aug 22;26(16):3794-803. doi: 10.1038/sj.emboj.7601811. Epub 2007 Aug 2.
6
Propagation of the [PIN+] prion by fragments of Rnq1 fused to GFP.与绿色荧光蛋白(GFP)融合的Rnq1片段介导的[PIN+]朊病毒传播。
Curr Genet. 2007 May;51(5):309-19. doi: 10.1007/s00294-007-0127-0. Epub 2007 Apr 6.
7
Channel mutations in Hsp104 hexamer distinctively affect thermotolerance and prion-specific propagation.热休克蛋白104六聚体中的通道突变对耐热性和朊病毒特异性增殖有显著影响。
Mol Microbiol. 2007 Mar;63(6):1669-83. doi: 10.1111/j.1365-2958.2007.05629.x.
8
Visualization of aggregation of the Rnq1 prion domain and cross-seeding interactions with Sup35NM.Rnq1朊病毒结构域聚集以及与Sup35NM交叉播种相互作用的可视化
J Biol Chem. 2007 Jan 19;282(3):1779-87. doi: 10.1074/jbc.M609269200. Epub 2006 Nov 22.
9
"Prion-proof" for [PIN+]: infection with in vitro-made amyloid aggregates of Rnq1p-(132-405) induces [PIN+].针对[PIN+]的“抗朊病毒”特性:用体外制备的Rnq1p-(132 - 405)淀粉样聚集体感染可诱导[PIN+]。
J Mol Biol. 2007 Jan 19;365(3):773-82. doi: 10.1016/j.jmb.2006.10.069. Epub 2006 Oct 25.
10
Biochemical and genetic methods for characterization of [PIN+] prions in yeast.用于表征酵母中[PIN+]朊病毒的生化和遗传方法。
Methods. 2006 May;39(1):23-34. doi: 10.1016/j.ymeth.2006.04.010.

酵母细胞中 Rnq1 N 端非朊病毒结构域中朊病毒不稳定突变的定位。

Localization of prion-destabilizing mutations in the N-terminal non-prion domain of Rnq1 in Saccharomyces cerevisiae.

机构信息

Department of Basic Medical Sciences, Institute of Medical Science, University of Tokyo, Minato-ku, Tokyo, Japan.

出版信息

Prion. 2009 Oct-Dec;3(4):250-8. doi: 10.4161/pri.3.4.10388. Epub 2009 Oct 20.

DOI:10.4161/pri.3.4.10388
PMID:20009538
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2807699/
Abstract

[PIN(+)] is the prion form of Rnq1 in Saccharomyces cerevisiae and is necessary for the de novo induction of a second prion, [PSI(+)]. The function of Rnq1, however, is little understood. The limited availability of defective rnq1 alleles impedes the study of its structure-function relationship by genetic analysis. In this study, we isolated rnq1 mutants that are defective in the stable maintenance of the [PIN(+)] prion. Since there is no rnq1 phenotype available that is applicable to a direct selection or screening for loss-of-function rnq1 mutants, we took advantage of a prion inhibitory agent, Rnq1Delta100, to develop a color-based genetic screen. Rnq1Delta100 eliminates the [PSI(+)] prion in the [PIN(+)] state but not in the [pin(-)] state. This allows us to find loss-of-[PIN(+)] rnq1 mutants as white [PSI(+)] colonies. Nine rnq1 mutants with single-amino-acid substitutions were defined. These mutations impaired the stable maintenance of [PIN(+)] and, as a consequence, were also partially defective in the de novo induction of [PSI(+)]. Interestingly, eight of the nine alleles were mapped to the N-terminal region of Rnq1, which is known as the non-prion domain preceding the asparagine and glutamine rich prion domain of Rnq1. Notably, overexpression of these rnq1 mutant proteins restored [PIN(+)] prion activity, suggesting that each of the rnq1 mutants was not completely inactive. These findings indicate that the N-terminal non-prion domain of Rnq1 harbors a potent activity to regulate the maintenance of the [PIN(+)] prion.

摘要

[PIN(+)] 是酿酒酵母中 Rnq1 的朊病毒形式,是从头诱导第二种朊病毒 [PSI(+)] 所必需的。然而,Rnq1 的功能知之甚少。有限的有缺陷 rnq1 等位基因的可用性阻碍了通过遗传分析研究其结构-功能关系。在这项研究中,我们分离了 rnq1 突变体,这些突变体在 [PIN(+)] 朊病毒的稳定维持方面存在缺陷。由于没有适用于功能丧失 rnq1 突变体的直接选择或筛选的 rnq1 表型,我们利用一种朊病毒抑制剂 Rnq1Delta100 开发了一种基于颜色的遗传筛选。Rnq1Delta100 消除了 [PSI(+)] 朊病毒在 [PIN(+)] 状态下,但不在 [pin(-)] 状态下。这使我们能够找到失去 [PIN(+)] 的 rnq1 突变体作为白色 [PSI(+)] 菌落。定义了九个具有单个氨基酸取代的 rnq1 突变体。这些突变破坏了 [PIN(+)] 的稳定维持,因此在从头诱导 [PSI(+)] 方面也部分缺陷。有趣的是,九个等位基因中有八个被映射到 Rnq1 的 N 端区域,该区域被称为 Rnq1 的天门冬酰胺和谷氨酸丰富的朊病毒结构域之前的非朊病毒结构域。值得注意的是,这些 rnq1 突变蛋白的过表达恢复了 [PIN(+)] 朊病毒活性,这表明每个 rnq1 突变体都不是完全无活性的。这些发现表明,Rnq1 的 N 端非朊病毒结构域具有调节 [PIN(+)] 朊病毒维持的强大活性。