Hoggett J G, Kellett G L
Eur J Biochem. 1976 Jun 15;66(1):65-77. doi: 10.1111/j.1432-1033.1976.tb10426.x.
A method is described for the purification of native hexokinases P-I and P-II from yeast using preparative isoelectric focussing to separate the isozymes. The binding of glucose to hexokinase P-II, and the effect of this on the monomer--dimer association--dissociation reaction have been investigated quantitatively by a combination of titrations of intrinsic protein fluorescence and equilibrium ultracentrifugation. Association constants for the monomer-dimer reaction decreased with increasing pH, ionic strength and concentration of glucose. Saturating concentrations of glucose did not bring about complete dissociation of the enzyme showing that both sites were occupired in the dimer. At pH 8.0 and high ionic strength, where the enzyme existed as monomer, the dissociation constant of the enzyme-glucose complex was 3 X 10(-4) mol 1(-1) and was independent of the concentration of enzyme. Binding to the dimeric form at low pH and ionic strength (I=0.02 mol 1(-1), pH less than 7.5) was also independent of enzyme concentration (in the range 10-1000 mug ml-1) but was much weaker. The process could be described by a single dissociation constant, showing that the two available sites on the dimer were equivalent and non-cooperative; values of the intrinsic dissociation constant varied from 2.5 X 10(-3) mol 1(-1) at pH 7.0 to 6 X 10(-3) at pH 6.5. Under intermediate conditions (pH 7.0, ionic strength=0.15 mol 1(-1)), where monomer and dimer coexisted, the binding of glucose showed weak positive cooperatively (Hill coefficient 1.2); in addition, the binding was dependent upon the concentration of enzyme in the direction of stronger binding at lower concentrations. The results show that the phenomenon of half-sites reactivity observed in the binding of glucose to crystalline hexokinase P-II does not occur in solution; the simplest explanation of our finding the two sites to be equivalent is that the dimer results from the homologous association of two identical subunits.
本文描述了一种从酵母中纯化天然己糖激酶P-I和P-II的方法,该方法利用制备性等电聚焦来分离同工酶。通过结合蛋白质固有荧光滴定和平衡超速离心,对葡萄糖与己糖激酶P-II的结合及其对单体-二聚体缔合-解离反应的影响进行了定量研究。单体-二聚体反应的缔合常数随pH值、离子强度和葡萄糖浓度的增加而降低。饱和浓度的葡萄糖不会导致酶完全解离,这表明二聚体中的两个位点都被占据。在pH 8.0和高离子强度下,酶以单体形式存在,酶-葡萄糖复合物的解离常数为3×10⁻⁴mol·L⁻¹,且与酶浓度无关。在低pH值和离子强度(I = 0.02 mol·L⁻¹,pH小于7.5)下与二聚体形式的结合也与酶浓度无关(在10 - 1000μg·ml⁻¹范围内),但结合力较弱。该过程可用单一解离常数来描述,表明二聚体上的两个可用位点是等效且非协同的;固有解离常数的值在pH 7.0时为2.5×10⁻³mol·L⁻¹,在pH 6.5时为6×10⁻³。在单体和二聚体共存的中间条件下(pH 7.0,离子强度 = 0.15 mol·L⁻¹),葡萄糖的结合表现出弱正协同性(希尔系数1.2);此外,结合依赖于酶浓度,在较低浓度下结合更强。结果表明,在溶液中葡萄糖与结晶己糖激酶P-II结合时观察到的半位点反应性现象并不存在;我们发现两个位点等效的最简单解释是二聚体是由两个相同亚基的同源缔合形成的。
Zotero 插件