Falconi M, Stroppolo M E, Cioni P, Strambini G, Sergi A, Ferrario M, Desideri A
INFM and Department of Biology, University of Rome Tor Vergata, Via della Ricerca Scientifica, 00133, Rome, Italy.
Biophys J. 2001 Jun;80(6):2556-67. doi: 10.1016/S0006-3495(01)76227-3.
A single mutation (Val29-->Gly) at the subunit interface of a Cu, Zn superoxide dismutase dimer leads to a twofold increase in the second order catalytic rate, when compared to the native enzyme, without causing any modification of the structure or the electric field distribution. To check the role of dynamic processes in this catalytic enhancement, the flexibility of the dimeric protein at the subunit interface region has been probed by the phosphorescence and fluorescence properties of the unique tryptophan residue. Multiple spectroscopic data indicate that Trp83 experiences a very similar, and relatively hydrophobic, environment in both wild-type and mutant protein, whereas its mobility is distinctly more restrained in the latter. Molecular dynamics simulation confirms this result, and provides, at the molecular level, details of the dynamic change felt by tryptophan. Moreover, the simulation shows that the loops surrounding the active site are more flexible in the mutant than in the native enzyme, making the copper more accessible to the incoming substrate, and being thus responsible for the catalytic rate enhancement. Evidence for increased, dynamic copper accessibility also comes from faster copper removal in the mutant by a metal chelator. These results indicate that differences in dynamic, rather than structural, features of the two enzymes are responsible for the observed functional change.
与天然酶相比,铜锌超氧化物歧化酶二聚体亚基界面处的单个突变(Val29→Gly)使二级催化速率提高了两倍,且未引起结构或电场分布的任何改变。为了检验动态过程在这种催化增强中的作用,通过独特色氨酸残基的磷光和荧光特性探测了二聚体蛋白在亚基界面区域的柔韧性。多个光谱数据表明,在野生型和突变型蛋白中,Trp83所处的环境非常相似且相对疏水,而在后者中其流动性明显受到更大限制。分子动力学模拟证实了这一结果,并在分子水平上提供了色氨酸所感受的动态变化细节。此外,模拟表明,突变体中围绕活性位点的环比天然酶中的更灵活,使得铜对进入的底物更易接近,从而导致催化速率提高。金属螯合剂在突变体中更快地去除铜也证明了动态的、更易接近的铜的存在。这些结果表明,两种酶在动态而非结构特征上的差异是观察到的功能变化的原因。