Folkers P J, Clore G M, Driscoll P C, Dodt J, Köhler S, Gronenborn A M
Laboratory of Chemical Physics, National Institute of Diabetes and Digestive and Kidney Diseases, Bethesda, Maryland 20892.
Biochemistry. 1989 Mar 21;28(6):2601-17. doi: 10.1021/bi00432a038.
The solution structure of recombinant wild-type hirudin and of the putative active site mutant Lys-47----Glu has been investigated by nuclear magnetic resonance (NMR) spectroscopy at 600 MHz. The 1H NMR spectra of the two hirudin variants are assigned in a sequential manner with a combination of two-dimensional NMR techniques. Some assignments made in our previous paper [Sukumaran, D. K., Clore, G. M., Preuss, A., Zarbock, J., & Gronenborn, A. M. (1987) Biochemistry 26, 333-338] were found to be incorrect and are now corrected. Analysis of the NOE data indicates that hirudin consists of an N-terminal compact domain (residues 1-49) held together by three disulfide linkages and a disordered C-terminal tail (residues 50-65) which does not fold back on the rest of the protein. This last observation corrects conclusions drawn by us previously on hirudin extracted from its natural source, the leech Hirudo medicinalis. The improved sensitivity of the 600-MHz spectrometer relative to that of our old 500-MHz spectrometer, the availability of two variants with slightly different chemical shifts, and the additional information arising from stereospecific assignments of methylene beta-protons and methyl protons of valine have permitted the determination of the solution structure of hirudin with much greater precision than before. Structure calculations on the N-terminal domain using the hybrid distance geometry-dynamical simulated annealing method were based on 685 and 661 approximate interproton distance restraints derived from nuclear Overhauser enhancement (NOE) data for the wild-type and mutant hirudin, respectively, together with 16 distance restraints for 8 backbone hydrogen bonds identified on the basis of NOE and amide NH exchange data and 26 phi backbone and 18 chi 1 side-chain torsion angle restraints derived from NOE and three-bond coupling constant data. A total of 32 structures were computed for both the wild-type and mutant hirudin. The structure of residues 2-30 and 37-48 which form the core of the N-terminal domain is well determined in both cases with an average atomic rms difference between the individual structures and the respective mean structures of approximately 0.7 A for the backbone atoms and approximately 1 A for all atoms. As found previously, the orientation of the exposed finger of antiparallel beta-sheet (residues 31-36) with respect to the core could not be determined on the basis of the present data due to the absence of any long-range NOEs between the exposed finger and the core.(ABSTRACT TRUNCATED AT 250 WORDS)
利用600兆赫的核磁共振(NMR)光谱研究了重组野生型水蛭素及其假定的活性位点突变体Lys-47----Glu的溶液结构。采用二维NMR技术相结合的方法,按顺序对两种水蛭素变体的1H NMR光谱进行了归属。我们之前论文[Sukumaran, D. K., Clore, G. M., Preuss, A., Zarbock, J., & Gronenborn, A. M. (1987) Biochemistry 26, 333 - 338]中所做的一些归属被发现是错误的,现已修正。对核Overhauser效应(NOE)数据的分析表明,水蛭素由一个通过三个二硫键维系在一起的N端紧密结构域(残基1 - 49)和一个无序的C端尾巴(残基50 - 65)组成,该C端尾巴不会折叠回到蛋白质的其余部分。这一最新发现修正了我们之前对从天然来源医用水蛭中提取的水蛭素所得出的结论。与我们旧的500兆赫光谱仪相比,600兆赫光谱仪灵敏度的提高、两种化学位移略有不同的变体的可得性以及缬氨酸亚甲基β-质子和甲基质子的立体专一性归属所产生的额外信息,使得能够比以前更精确地测定水蛭素的溶液结构。使用混合距离几何 - 动力学模拟退火方法对N端结构域进行结构计算,分别基于野生型和突变型水蛭素的核Overhauser增强(NOE)数据得出的685个和661个近似质子间距离约束,以及基于NOE和酰胺NH交换数据确定的8个主链氢键的16个距离约束,还有基于NOE和三键耦合常数数据得出的26个主链φ角和18个侧链χ1扭转角约束。对野生型和突变型水蛭素均计算了总共32个结构。在这两种情况下,形成N端结构域核心的残基2 - 30和37 - 48的结构都得到了很好的确定,各个结构与相应平均结构之间的平均原子均方根差值,主链原子约为0.7埃,所有原子约为1埃。如之前所发现的,由于暴露的反平行β-折叠指状结构(残基31 - 36)与核心之间不存在任何长程NOE,基于目前的数据无法确定其相对于核心的取向。(摘要截取自250词)
