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通过二维傅里叶变换核磁共振方法的系统应用对核糖体蛋白E-L30的1H核磁共振谱中的共振进行残基特异性归属。

Residue-specific assignments of resonances in the 1H nuclear magnetic resonance spectrum of ribosomal protein E-L30 by systematic application of two-dimensional Fourier transform nuclear magnetic resonance methods.

作者信息

van de Ven F J, Hilbers C W

出版信息

J Mol Biol. 1986 Nov 20;192(2):389-417. doi: 10.1016/0022-2836(86)90372-4.

Abstract

A two-dimensional Fourier transform nuclear magnetic resonance study of the ribosomal protein E-L30 is reported. Five two-dimensional techniques, namely: nuclear magnetic resonance J-resolved spectroscopy, correlated spectroscopy, double quantum spectroscopy, relayed coherence transfer and nuclear Overhauser enhancement spectroscopy were used. Qualitative inspection of the spectra obtained by these techniques provided evidence that the E-L30 molecule has a well-defined structure in solution. This analysis indicated that, despite the fact that the protein is stable only at moderate temperatures and neutral pH, a structural analysis of the molecule would be feasible. A detailed analysis of the spectra permitted unambiguous discrimination between the spin systems of different amino acids, resulting in residue-specific resonance assignments. We were able to assign all resonances of all six threonine, four valine, five alanine, two histidine, two serine, one phenylalanine, one asparagine and one aspartic acid residue of E-L30. Complete resonance assignment was obtained for two glycine residues. Partial assignments became available for all six isoleucine, three glycine and one glutamine residue. These results form a sound basis for the structure determination of the protein described in the accompanying paper.

摘要

报道了核糖体蛋白E-L30的二维傅里叶变换核磁共振研究。使用了五种二维技术,即:核磁共振J分辨谱、相关谱、双量子谱、接力相干转移谱和核Overhauser增强谱。对通过这些技术获得的谱进行定性检查,提供了证据表明E-L30分子在溶液中具有明确的结构。该分析表明,尽管该蛋白质仅在中等温度和中性pH下稳定,但对该分子进行结构分析是可行的。对谱的详细分析允许明确区分不同氨基酸的自旋系统,从而得到残基特异性的共振归属。我们能够归属E-L30的所有六个苏氨酸、四个缬氨酸、五个丙氨酸、两个组氨酸、两个丝氨酸、一个苯丙氨酸、一个天冬酰胺和一个天冬氨酸残基的所有共振。获得了两个甘氨酸残基的完整共振归属。对所有六个异亮氨酸、三个甘氨酸和一个谷氨酰胺残基进行了部分归属。这些结果为随附论文中所述蛋白质的结构测定奠定了坚实的基础。

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