Miyamoto S, Kollman P A
Department of Pharmaceutical Chemistry, University of California, San Francisco 94143.
Proteins. 1993 Jul;16(3):226-45. doi: 10.1002/prot.340160303.
We present calculations of the absolute and relative binding free energies of complexation of streptavidin with biotin and its analogs by means of a thermodynamic free energy perturbation method implemented with molecular dynamics. Using the recently solved crystal structure of the streptavidin-biotin complex, biotin was mutated into a dummy molecule as well as thiobiotin and iminobiotin both in the protein and in solution. The calculated absolute binding free energy was dependent on the simulation model used. Encouragingly, the "best models" provided a reasonable semiquantitative reproduction (-20 to -22 kcal/mol) of the experimental free energy (-18.3 kcal/mol). Furthermore, the calculated results give clear insights into the binding nature of the protein-ligand complex, showing that the van der Waals energy dominates the electrostatic and hydrogen bonding energies in the binding of biotin by streptavidin. Specifically, the mutation of biotin into a dummy molecule in solution has a delta G (van der Waals) approximately -4 kcal/mol, due to the cancellation of dispersion and repulsion "cavity" effects. On the other hand, in the protein, a very small free energy price must be paid to create a cavity since one already exists and the mutation of biotin into a dummy molecule has a delta G (van der Waals) approximately 15 kcal/mol. These results are also consistent with the interpretation that the entropy increase to be expected from hydrophobic interactions from desolvation of biotin is counterbalanced by a decrease in entropy accompanying the formation of buried hydrogen bonds, which have been derived from the apparently conflicting experimental data. They provide an alternative interpretation of the reason for the extremely high affinity of the biotin-streptavidin interaction than that recently proposed by Weber et al. (J. Am. Chem. Soc. 114:3197, 1992). In the case of the relative binding free energies, the calculated values of 3.8 +/- 0.6 and 7.2 +/- 0.6 kcal/mol compare well with the experimental values of 3.6 and 6.2 kcal/mol for the perturbation of biotin to thiobiotin and iminobiotin, respectively in the related protein avidin. The calculations indicate that desolvation of the ligand is important in understanding the relative affinity of the ligands with the protein. The above successful simulations suggest that the molecular dynamics/free energy perturbation method is useful for understanding the energetic features affecting the binding between proteins and ligands, since it is generally difficult to determine these factors unambiguously by experiment.(ABSTRACT TRUNCATED AT 400 WORDS)
我们通过分子动力学实现的热力学自由能微扰方法,给出了链霉亲和素与生物素及其类似物络合的绝对和相对结合自由能的计算结果。利用最近解析的链霉亲和素 - 生物素复合物晶体结构,在蛋白质和溶液中,将生物素突变为虚拟分子以及硫代生物素和亚氨基生物素。计算得到的绝对结合自由能取决于所使用的模拟模型。令人鼓舞的是,“最佳模型”对实验自由能(-18.3 kcal/mol)给出了合理的半定量再现(-20至-22 kcal/mol)。此外,计算结果清晰地揭示了蛋白质 - 配体复合物的结合本质,表明在链霉亲和素结合生物素的过程中,范德华能在静电能和氢键能中占主导地位。具体而言,在溶液中将生物素突变为虚拟分子时,由于色散和排斥“空穴”效应的抵消,其ΔG(范德华)约为 -4 kcal/mol。另一方面,在蛋白质中,由于已经存在一个空穴,将生物素突变为虚拟分子时只需付出非常小的自由能代价,其ΔG(范德华)约为15 kcal/mol。这些结果也与以下解释一致:生物素去溶剂化产生的疏水相互作用预期的熵增加,被埋藏氢键形成伴随的熵减少所抵消,这一解释源于明显相互矛盾的实验数据。它们为生物素 - 链霉亲和素相互作用具有极高亲和力的原因提供了一种与Weber等人(《美国化学会志》114:3197, 1992)最近提出的不同的解释。在相对结合自由能的情况下,对于在相关蛋白质抗生物素蛋白中生物素到硫代生物素和亚氨基生物素的微扰,计算值3.8±0.6和7.2±0.6 kcal/mol与实验值3.6和6.2 kcal/mol比较吻合。计算表明,配体的去溶剂化对于理解配体与蛋白质的相对亲和力很重要。上述成功模拟表明,分子动力学/自由能微扰方法对于理解影响蛋白质与配体结合的能量特征很有用,因为通常很难通过实验明确确定这些因素。(摘要截断于400字)
