Grazi E, Trombetta G
Arch Biochem Biophys. 1984 Sep;233(2):595-602. doi: 10.1016/0003-9861(84)90484-3.
The equivalence of the four dihydroxyacetone phosphate binding sites of aldolase was abolished by lowering the temperature. At pH 6.2 and -13 degrees C, four binding sites were detected by gel filtration; two sites with a Kdiss less than or equal to 0.1 microM, and a second set of sites with a Kdiss = 4 microM. The alteration of the binding was accompanied by the alteration of the catalytic activity. The low-affinity sites were incapable of catalyzing the cleavage of the (3S) C-H bond of dihydroxyacetone phosphate, and form only the ketimine phosphate intermediate. The high-affinity sites were still able to cleave the (3S) C-H bond of dihydroxyacetone phosphate; however, the eneamine phosphate intermediate formed was almost fully converted into the eneamine-aldehyde . . . phosphate intermediate, which was the prevailing species at the equilibrium. The mechanism of the half-of-the sites reactivity of aldolase at low temperature has been explained and the nonequivalence of sites in promoting catalysis has been utilized to dissect and characterize the individual partial reactions of the enzyme. In the course of these studies it has been shown that the rate of hydration-dehydration of dihydroxyacetone phosphate at -24 degrees C was too slow to measure.
通过降低温度,醛缩酶的四个磷酸二羟丙酮结合位点的等效性被消除。在pH 6.2和-13℃条件下,通过凝胶过滤检测到四个结合位点;两个位点的解离常数Kdiss≤0.1μM,另一组位点的Kdiss = 4μM。结合的改变伴随着催化活性的改变。低亲和力位点无法催化磷酸二羟丙酮的(3S)C-H键的裂解,仅形成酮亚胺磷酸中间体。高亲和力位点仍能够裂解磷酸二羟丙酮的(3S)C-H键;然而,形成的烯胺磷酸中间体几乎完全转化为烯胺-醛……磷酸中间体,这是平衡时的主要物种。已经解释了醛缩酶在低温下半位点反应性的机制,并且利用位点在促进催化方面的不等效性来剖析和表征该酶的各个部分反应。在这些研究过程中已经表明,在-24℃下磷酸二羟丙酮的水合-脱水速率太慢而无法测量。
