Wang Y, Darnay B G, Rodwell V W
Department of Biochemistry, Purdue University, West Lafayette, Indiana 47907.
J Biol Chem. 1990 Dec 15;265(35):21634-41.
Kinetic analysis of 3-hydroxy-3-methylglutaryl coenzyme A (HMG-CoA) reductase has implicated a glutamate or aspartate residue in (i) formation of mevaldate thiohemiacetal by proton transfer to the carbonyl oxygen of mevaldate and (ii) enhanced ionization of CoASH by the resulting enzyme carboxylate anion, facilitating attack by CoAS- on the carbonyl carbon of mevaldate (Veloso, D., Cleland, W. W., and Porter, J. W. (1981) Biochemistry 81, 887-894). Although neither the identity of this acidic residue nor its location is known, the catalytic domains of 11 sequenced HMG-CoA reductases contain only 3 conserved acidic residues. For HMG-CoA reductase of Pseudomonas mevalonii, these residues are Glu52, Glu83, and Asp183. To identify the acidic residue that functions in catalysis, we generated mutants having alterations in these residues. The mutant proteins were expressed, purified, and characterized. Mutational alteration of residues Glu52 or Asp183 of P. mevalonii HMG-CoA reductase yielded enzymes with significant, but in some cases reduced, activity (Vmax = 100% Asp183----Ala, 65% Asp183----Asn, and 15% Glu52----Gln of wild-type activity, respectively). Although the activity of mutant enzymes Glu52----Gln and Asp183----Ala was undetectable under standard assay conditions, their Km values for substrates were 4-300-fold higher than those for wild-type enzyme. Km values for wild-type enzyme and for mutant enzymes Glu52----Gln and Asp183----Ala were, respectively: 0.41, 73, and 120 mM [R,S)-mevalonate); 0.080, 4.4, and 2.0 mM (coenzyme A); and 0.26, 4.4, and 1.0 mM (NAD+). By these criteria, neither Glu52 nor Asp183 is the acidic catalytic residue although each may function in substrate recognition. During chromatography on coenzyme A agarose or HMG-CoA agarose, mutant enzymes Asp183----Asn and Glu83----Gln behaved like wild-type enzyme. By contrast, and in support of a role for these residues in substrate recognition, mutant enzymes Glu52----Gln and Asp183----Ala exhibited impaired ability to bind to either support. Despite displaying Km values for substrates and chromatographic behavior on substrate affinity supports comparable to wild-type enzyme, only mutant enzyme Glu83----Gln was essentially inactive under all conditions studied (Vmax = 0.2% that of wild-type enzyme). Glutamate residue 83 of P. mevalonii HMG-CoA reductase, and consequently the glutamate of the consensus Pro-Met-Ala-Thr-Thr-Glu-Gly-Cys-Leu-Val-Ala motif of the catalytic domains of eukaryotic HMG-CoA reductases, is judged to be the acidic residue functional in catalysis.
3-羟基-3-甲基戊二酰辅酶A(HMG-CoA)还原酶的动力学分析表明,一个谷氨酸或天冬氨酸残基参与了以下过程:(i)通过将质子转移至甲羟戊酸的羰基氧形成甲羟戊酸硫代半缩醛;(ii)由此产生的酶羧基阴离子增强了辅酶A(CoASH)的电离,促进CoAS-对甲羟戊酸羰基碳的攻击(维洛索,D.,克莱兰,W.W.,以及波特,J.W.(1981年)《生物化学》81,887 - 894)。尽管这个酸性残基的身份及其位置均未知,但11种已测序的HMG-CoA还原酶的催化结构域仅包含3个保守的酸性残基。对于甲基营养型假单胞菌的HMG-CoA还原酶而言,这些残基是Glu52、Glu83和Asp183。为了鉴定在催化中起作用的酸性残基,我们构建了这些残基发生改变的突变体。突变蛋白得以表达、纯化并进行了特性分析。甲基营养型假单胞菌HMG-CoA还原酶的Glu52或Asp183残基的突变改变产生了具有显著活性但在某些情况下活性降低的酶(Vmax分别为野生型活性的100%(Asp183→Ala)、65%(Asp183→Asn)和15%(Glu52→Gln))。尽管在标准测定条件下未检测到突变酶Glu52→Gln和Asp183→Ala的活性,但其底物的Km值比野生型酶高4 - 300倍。野生型酶以及突变酶Glu52→Gln和Asp183→Ala的Km值分别为:0.
