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关于HET-s218-295朊病毒蛋白的高分辨率氢/氘交换研究。

High-resolution H/D exchange studies on the HET-s218-295 prion protein.

作者信息

Nazabal Alexis, Bonneu Marc, Saupe Sven J, Schmitter Jean-Marie

机构信息

Institut Européen de Chimie et de Biologie, UMR CNRS 5144, Pessac, France.

出版信息

J Mass Spectrom. 2005 May;40(5):580-90. doi: 10.1002/jms.819.

DOI:10.1002/jms.819
PMID:15856424
Abstract

In a search for improved resolution of hydrogen/deuterium (H/D) exchange experiments analyzed by mass spectrometry (HXMS), we evaluated two methodologies for a detailed structural study of solvent accessibility in the case of the HET-s(218-295) prion protein. For the first approach, after incubation in the deuterated solvent, aggregated HET-s(218-295) was digested with pepsin and the generated peptides were analyzed by nanospray mass spectrometry in an ion trap, with and without collision-induced dissociation (CID). We compared deuterium incorporation in peptides as determined on peptide pseudomolecular ions and on b and y fragments produced by longer peptides under CID conditions. For both b and y fragment ions, an extensive H/D scrambling phenomenon was observed, in contrast with previous studies comparing CID-MS experiments and (1)H NMR data. Thus, the spatial resolution of HXMS experiments could not be improved by means of MS/MS data generated by an ion trap mass spectrometer. In a second approach, the incorporation of deuterium was analyzed by MS for 76 peptides of the HET-s(218-289) peptide mass fingerprint, and the use of shared boundaries among peptic peptides allowed us to determine deuteration levels of small regions ranging from one to four amino acids. This methodology led to evidence of highly protected regions along the HET-s(218-295) sequence.

摘要

为了提高通过质谱分析的氢/氘(H/D)交换实验的分辨率,我们评估了两种方法,用于对HET-s(218 - 295)朊病毒蛋白的溶剂可及性进行详细的结构研究。对于第一种方法,在氘代溶剂中孵育后,将聚集的HET-s(218 - 295)用胃蛋白酶消化,然后在离子阱中通过纳喷雾质谱分析生成的肽段,分别在有无碰撞诱导解离(CID)的情况下进行。我们比较了在肽假分子离子以及在CID条件下由较长肽段产生的b和y片段上测定的肽段中氘的掺入情况。对于b和y片段离子,均观察到广泛的H/D重排现象,这与之前比较CID-MS实验和¹H NMR数据的研究结果相反。因此,离子阱质谱仪产生的MS/MS数据无法提高HXMS实验的空间分辨率。在第二种方法中,通过质谱分析了HET-s(218 - 289)肽质量指纹图谱中的76个肽段的氘掺入情况,并且利用胃蛋白酶消化产生的肽段之间的共享边界,我们能够确定一到四个氨基酸的小区域的氘化水平。这种方法揭示了HET-s(218 - 295)序列中存在高度受保护的区域。

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