Riley-Lovingshimer Michelle R, Ronning Donald R, Sacchettini James C, Reinhart Gregory D
Department of Biochemistry and Biophysics and Center for Advanced Biomolecular Research, Texas A&M University, 2128 TAMU, College Station, Texas 77843-2128, USA.
Biochemistry. 2002 Oct 29;41(43):12967-74. doi: 10.1021/bi0263412.
The biophysical properties of a tryptophan-shifted mutant of phosphofructokinase from Bacillus stearothermophilus (BsPFK) have been examined. The mutant, designated W179Y/Y164W, has kinetic and thermodynamic properties similar to the wild-type enzyme. A 2-fold decrease in kcat is observed, and the mutant displays a 3-fold smaller K(0.5) for the substrate, fructose-6-phosphate (Fru-6-P), as compared to the wild-type enzyme. The dissociation constant for the inhibitor, phospho(enol)pyruvate (PEP), increases 2-fold, and the coupling parameter, Q(ay), decreases 2-fold. This suggests that while the mutant displays a slightly decreased affinity for PEP, PEP is still an effective inhibitor once bound. The new position of the tryptophan in W179Y/Y164W is approximately 6 A from the Fru-6-P portion of the active site. A 25% decrease in fluorescence intensity is observed upon Fru-6-P binding, and an 80% decrease in fluorescence intensity is observed with PEP binding. In addition, the intrinsic fluorescence polarization increases from 0.327 +/- 0.001 to 0.353 +/- 0.001 upon Fru-6-P binding, but decreases to 0.290 +/- 0.001 when PEP binds. Most notably, the presence of PEP induces dissociation of the tetramer. Dissociation of the tetramer into dimers occurs along the active site interface and can be monitored by the loss in activity or the loss in tryptophan fluorescence that is observed when the enzyme is titrated with PEP. Activity can be protected or recovered by incubating the enzyme with Fru-6-P. Recovery of activity is enzyme concentration dependent, and the rate constant for association is 6.2 +/- 0.3 M(-1) x s(-1). Ultracentrifugation experiments revealed that in the absence of PEP the mutant enzyme exists in an equilibrium between the dimer and tetramer forms with a dissociation constant of 11.8 +/- 0.5 microM, while in the presence of PEP the enzyme exists in equilibrium between the dimer and monomer forms with a dissociation constant of 7.5 +/- 0.02 microM. A 3.1 A crystal structure of the mutant enzyme suggests that the amino acid substitutions have not dramatically altered the tertiary structure of the enzyme. While it is clear that wild-type BsPFK exists as a tetramer under these same conditions, these results suggest that quaternary structural changes probably play an important role in allosteric communication.
对嗜热脂肪芽孢杆菌磷酸果糖激酶(BsPFK)色氨酸移位突变体的生物物理性质进行了研究。该突变体命名为W179Y/Y164W,其动力学和热力学性质与野生型酶相似。观察到催化常数kcat降低了2倍,与野生型酶相比,该突变体对底物6-磷酸果糖(Fru-6-P)的K(0.5)小3倍。抑制剂磷酸烯醇丙酮酸(PEP)的解离常数增加了2倍,偶联参数Q(ay)降低了2倍。这表明,虽然该突变体对PEP的亲和力略有降低,但PEP一旦结合仍是一种有效的抑制剂。W179Y/Y164W中色氨酸的新位置距离活性位点的Fru-6-P部分约6 Å。Fru-6-P结合后荧光强度降低25%,PEP结合后荧光强度降低80%。此外,Fru-6-P结合后固有荧光偏振从0.327±0.001增加到0.353±0.001,但PEP结合时降低到0.290±0.001。最值得注意的是,PEP的存在诱导了四聚体的解离。四聚体解离为二聚体沿着活性位点界面发生,并且可以通过活性丧失或用PEP滴定酶时观察到的色氨酸荧光丧失来监测。用Fru-6-P孵育酶可以保护或恢复活性。活性恢复依赖于酶浓度,缔合速率常数为6.2±0.3 M(-1)×s(-1)。超速离心实验表明,在没有PEP的情况下,突变体酶以二聚体和四聚体形式存在平衡,解离常数为11.8±0.5 μM,而在有PEP的情况下,酶以二聚体和单体形式存在平衡,解离常数为7.5±0.02 μM。突变体酶的3.1 Å晶体结构表明,氨基酸取代并没有显著改变酶的三级结构。虽然很明显野生型BsPFK在这些相同条件下以四聚体形式存在,但这些结果表明四级结构变化可能在变构通讯中起重要作用。
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