Vögeli Beat, Yao Lishan
Laboratory of Physical Chemistry, Swiss Federal Institute of Technology, ETH-Honggerberg, CH-8093 Zurich, Switzerland.
J Am Chem Soc. 2009 Mar 18;131(10):3668-78. doi: 10.1021/ja808616v.
Although collective dynamics of atom groups steer many biologically relevant processes in biomacromolecules, most atomic resolution motional studies focus on isolated bonds. In this study, a new method is introduced to assess correlated dynamics between bond vectors by cross relaxation nuclear magnetic resonance (NMR). Dipole-dipole cross correlated relaxation rates between intra- and inter-residual H(N)-N and H(alpha)-C(alpha) in the 56 residue protein GB3 are measured with high accuracy. It is demonstrated that the assumption of anisotropic molecular tumbling is necessary to evaluate rates accurately and predictions from the static structure using effective bond lengths of 1.041 and 1.117 A for H(N)-N and H(alpha)-C(alpha) are within 3% of both experimental intra- and inter-residual rates. Deviations are matched to models of different degrees of motional correlation. These models are based on previously determined orientations and motional amplitudes from residual dipolar couplings with high accuracy and precision. Clear evidence of correlated motion in the loops comprising residues 10-14, 20-22, and 47-50 and anticorrelated motion in the alpha helix comprising 23-38 is presented. Somewhat weaker correlation is observed in the beta strands 2-4, which have previously been shown to exhibit slow correlated motional modes.
尽管原子基团的集体动力学主导着生物大分子中许多与生物学相关的过程,但大多数原子分辨率的运动研究都集中在孤立的键上。在本研究中,引入了一种新方法,通过交叉弛豫核磁共振(NMR)来评估键向量之间的相关动力学。高精度测量了56个残基的蛋白质GB3中残基内和残基间H(N)-N以及H(α)-C(α)之间的偶极-偶极交叉相关弛豫率。结果表明,各向异性分子翻滚的假设对于准确评估速率是必要的,并且使用1.041和1.117 Å的有效键长从静态结构进行的预测与实验测得的残基内和残基间速率的偏差均在3%以内。偏差与不同程度运动相关性的模型相匹配。这些模型基于先前通过残余偶极耦合以高精度和高精确度确定的取向和运动幅度。给出了包含残基10 - 14、20 - 22和47 - 50的环中相关运动以及包含23 - 38的α螺旋中反相关运动的明确证据。在β链2 - 4中观察到的相关性稍弱,之前已表明其表现出缓慢的相关运动模式。