Kristensen S M, Siegal G, Sankar A, Driscoll P C
Department of Chemistry, University of Copenhagen, Universitetsparken 5, Kobenhavn O, DK-2100, Denmark.
J Mol Biol. 2000 Jun 9;299(3):771-88. doi: 10.1006/jmbi.2000.3760.
The backbone dynamics of the C-terminal SH2 domain from the regulatory subunit p85alpha (p85alpha C-SH2) of phosphoinositide 3-kinase has been investigated in the absence of, and in complex with, a high-affinity phosphotyrosine-containing peptide ligand derived from the platelet-derived growth-factor receptor. (15)N R(1) and R(2) relaxation rates and steady-state [(1)H]-(15)N NOE values were measured by means of (1)H-(15)N correlated two-dimensional methods and were analyzed within the framework of the model-free formalism. Several residues in the BC loop and in the neighbouring secondary structural elements display fast local dynamics in the absence of phosphotyrosine peptide ligand as evidenced by below-average [(1)H]-(15)N NOE values. Furthermore, residue Gln41 (BC3) displays conformational exchange phenomena as indicated by an above-average R(2) relaxation rate. Upon binding of the phosphotyrosine peptide, the NOE values increase to values observed for regular secondary structure and the exchange contribution to the R(2) relaxation rate for Gln41 (BC3) vanishes. These observations indicate a loss of backbone flexibility upon ligand binding. Substantial exchange contributions for His56 (betaD4) and Cys57 (betaD5), which are known to make important interactions with the ligand, are attenuated upon ligand binding. Several residues in the betaD'-FB region and the BG loop, which contribute to the ligand binding surface of the protein, exhibit exchange terms which are reduced or vanish when the ligand is bound. Together, these observations suggest that ligand binding is accompanied by a loss of conformational flexibility on the ligand binding face of the protein. However, comparison with other SH2 domains reveals an apparent lack of consensus in the changes in dynamics induced by ligand binding. Exchange rates for individual residues were quantified in peptide-complexed p85alpha C-SH2 from the dependence of the exchange contributions on the CPMG delay in an R(2) series and show that peptide-complexed p85alpha C-SH2 is affected by multiple conformational exchange processes with exchange rate constants from 10(2) s(-1) to 7.10(3) s(-1). Mapping of the exchange-rate constants on the protein surface show a clustering of residues with similar exchange-rate constants and suggests that clustered residues are affected by a common predominant exchange process.
在不存在磷酸酪氨酸肽配体以及与源自血小板衍生生长因子受体的高亲和力含磷酸酪氨酸肽配体形成复合物的情况下,对磷脂酰肌醇3激酶调节亚基p85α的C末端SH2结构域(p85α C-SH2)的主链动力学进行了研究。通过1H-15N相关二维方法测量了15N R1和R2弛豫率以及稳态[1H]-15N NOE值,并在无模型形式体系的框架内进行了分析。BC环和相邻二级结构元件中的几个残基在不存在磷酸酪氨酸肽配体时表现出快速的局部动力学,这由低于平均水平的[1H]-15N NOE值证明。此外,残基Gln41(BC3)表现出构象交换现象,这由高于平均水平的R2弛豫率表明。在结合磷酸酪氨酸肽后,NOE值增加到规则二级结构所观察到的值,并且Gln41(BC3)对R2弛豫率的交换贡献消失。这些观察结果表明配体结合后主链灵活性丧失。已知与配体进行重要相互作用的His56(βD4)和Cys57(βD5)的大量交换贡献在配体结合后减弱。βD'-FB区域和BG环中对蛋白质配体结合表面有贡献的几个残基,在结合配体时表现出减少或消失的交换项。总之,这些观察结果表明配体结合伴随着蛋白质配体结合面上构象灵活性的丧失。然而,与其他SH2结构域的比较揭示了配体结合诱导的动力学变化明显缺乏一致性。根据R2系列中交换贡献对CPMG延迟的依赖性,对肽复合的p85α C-SH2中各个残基的交换率进行了量化,结果表明肽复合的p85α C-SH2受到多个构象交换过程的影响,交换速率常数从102 s-1到7.1×103 s-1。将交换速率常数映射到蛋白质表面显示具有相似交换速率常数的残基聚集在一起,这表明聚集的残基受到共同的主要交换过程的影响。
