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测定蛋白质中骨架氮-氮 J 相关。

Determination of backbone nitrogen-nitrogen J correlations in proteins.

机构信息

Institute of Physical Biology, Heinrich-Heine-Universität, D-40225, Düsseldorf, Germany.

出版信息

J Biomol NMR. 1997 Dec;10(4):403-8. doi: 10.1023/A:1018373601391.

Abstract

Recently, a quantitative J correlation technique has been presented which makes use of homonuclear Hartmann-Hahn cross-polarization (TOCSY) to measure (3)J(C)'(C)' in proteins isotopically enriched with (13)C [Grzesiek, S. and Bax, A. (1997) J. Biomol. NMR, 9, 207-211]. Since homonuclear Hartmann-Hahn is twice as fast as conventional COSY transfer, this method is much less sensitive to transverse relaxation, which is the principal limiting factor in achieving long-range J-coupling correlations in macromolecules. Here we describe a similar experiment which is used to measure(3) J(NN) coupling constants between sequential amide(15) N nuclei in the backbone of ubiquitin. As expected from the low magnetic moment of (15)N, the (3)J(NN) coupling constants are exceedingly small, with values between 0.14 and 0.36 Hz for residues in β-conformations and values below 0.15 Hz for residues in α-conformations. In contrast to what is expected from a Karplus-type dependence on the backbone angle ψ, large differences in the values of(3) J(NN) are observed for a number of residues with very similar backbone ψ angles. A quantitative description of statistical and systematic errors, in particular of relaxation effects during the TOCSY transfer, shows that these differences are highly significant.

摘要

最近,一种定量的 J 相关技术已经被提出,该技术利用同核 Hartmann-Hahn 交叉极化(TOCSY)来测量(13)C 同位素丰度的蛋白质中的(3)J(C)'(C)[Grzesiek,S.和 Bax,A.(1997)J. Biomol. NMR,9,207-211]。由于同核 Hartmann-Hahn 的速度是传统 COSY 转移的两倍,因此该方法对横向弛豫的敏感性要低得多,横向弛豫是在大分子中实现长程 J 耦合相关的主要限制因素。在这里,我们描述了一个类似的实验,用于测量泛素骨架中连续酰胺(15)N 核之间的(3)J(NN)偶合常数。正如(15)N 的磁矩低所预期的那样,(3)J(NN)偶合常数非常小,β构象中的残基值在 0.14 到 0.36 Hz 之间,α构象中的残基值低于 0.15 Hz。与基于主链角 ψ 的 Karplus 类型依赖性所预期的相反,对于许多主链 ψ 角非常相似的残基,(3)J(NN)的值存在很大差异。对统计和系统误差,特别是 TOCSY 转移过程中的弛豫效应的定量描述表明,这些差异具有高度显著性。

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