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绵羊和麋鹿朊病毒蛋白中蛋氨酸 216 的氧化高度依赖于 218 位的氨基酸,但对朊病毒的传播不重要。

Oxidation of methionine 216 in sheep and elk prion protein is highly dependent upon the amino acid at position 218 but is not important for prion propagation.

机构信息

Western Regional Research Center, United States Department of Agriculture , Albany, California 94710, United States.

出版信息

Biochemistry. 2013 Mar 26;52(12):2139-47. doi: 10.1021/bi3016795. Epub 2013 Mar 15.

Abstract

We employed a sensitive mass spectrometry-based method to deconstruct, confirm, and quantitate the prions present in elk naturally infected with chronic wasting disease and sheep naturally infected with scrapie. We used this approach to study the oxidation of a methionine at position 216 (Met216), because this oxidation (MetSO216) has been implicated in prion formation. Three polymorphisms (Ile218, Val218, and Thr218) of sheep recombinant prion protein were prepared. Our analysis showed the novel result that the proportion of MetSO216 was highly dependent upon the amino acid residue at position 218 (I > V > T), indicating that Ile218 in sheep and elk prion protein (PrP) renders the Met216 intrinsically more susceptible to oxidation than the Val218 or Thr218 analogue. We were able to quantitate the prions in the attomole range. The presence of prions was verified by the detection of two confirmatory peptides: GENFTETDIK (sheep and elk) and ESQAYYQR (sheep) or ESEAYYQR (elk). This approach required much smaller amounts of tissue (600 μg) than traditional methods of detection (enzyme-linked immunosorbent assay, Western blot, and immunohistochemical analysis) (60 mg). In sheep and elk, a normal cellular prion protein containing MetSO216 is not actively recruited and converted to prions, although we observed that this Met216 is intrinsically more susceptible to oxidation.

摘要

我们采用了一种基于灵敏质谱的方法来解构、确认和定量分析天然感染慢性消耗病的麋鹿和天然感染羊瘙痒病的绵羊中的朊病毒。我们使用这种方法来研究位于 216 位的蛋氨酸(Met216)的氧化,因为这种氧化(MetSO216)与朊病毒的形成有关。我们制备了三种绵羊重组朊病毒蛋白的多态性(Ile218、Val218 和 Thr218)。我们的分析结果表明,MetSO216 的比例高度依赖于 218 位的氨基酸残基(I > V > T),这表明绵羊和麋鹿朊病毒蛋白(PrP)中的 Ile218 使 Met216 比 Val218 或 Thr218 类似物更容易发生氧化。我们能够在皮摩尔范围内定量检测朊病毒。通过检测两个确认性肽:GENFTETDIK(绵羊和麋鹿)和 ESQAYYQR(绵羊)或 ESEAYYQR(麋鹿),可以验证朊病毒的存在。与传统的检测方法(酶联免疫吸附试验、免疫印迹和免疫组织化学分析)相比,这种方法所需的组织量要少得多(600μg)(60mg)。在绵羊和麋鹿中,虽然我们观察到这种 Met216 更容易发生氧化,但含有 MetSO216 的正常细胞朊病毒蛋白并没有被主动募集并转化为朊病毒。

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