Hawkes T R, Thomas P G, Edwards L S, Rayner S J, Wilkinson K W, Rice D W
Department of Exploratory Plant Sciences, Zeneca Agrochemicals, Bracknell, Berkshire, U.K.
Biochem J. 1995 Mar 1;306 ( Pt 2)(Pt 2):385-97. doi: 10.1042/bj3060385.
The HIS3+ gene of Saccharomyces cerevisiae was overexpressed in Escherichia coli and the recombinant imidazoleglycerol-phosphate dehydratase (IGPD) purified to homogeneity. Laser-desorption and electrospray m.s. indicated a molecular ion within 2 units of that expected (23833.3) on the basis of the protein sequence, with about half of the polypeptide lacking the N-terminal formylmethionine residue. IGPD initially purified as an apoprotein was catalytically inactive and mainly a trimer of M(r) 70,000. Addition of Mn2+ (but not Mg2+) caused this to assemble to an active (40 units/mg) enzyme (Mn-IGPD) comprising of 24 subunits (M(r) 573,000) and containing 1.35 +/- 0.1 Mn atoms/polypeptide subunit. An enzyme with an identical activity and metal content was also obtained when the fermenter growth medium of recombinant Escherichia coli was supplemented with MnCl2, and IGPD was purified through as Mn-IGPD rather than as the apoenzyme and assembled in vitro. Inhibition by EDTA indicated that the intrinsic Mn2+ was essential for activity. The retention of activity over time after dilution to very low concentrations of enzyme (< 20 nM) indicated that the metal remained in tight association with the protein. A novel continuous assay method was developed to facilitate the kinetic characterization of Mn-IGPD. At pH 7.0, the Km for IGP was 0.10 +/- 0.02 mM and the Ki value for inhibition by 1,2,4-triazole, 0.12 +/- 0.02 mM. In contrast with other reports, thiols had no influence on catalytic activity. The activity of Mn-IGPD varied with enzyme concentration in such a way as to suggest that it dissociates to a less active form at very low concentrations. Significant inhibition by the product, imidazole acetol phosphate, was inferred from the shape of the progress curve. Titration with, the potent competitive inhibitor, 2-hydroxy-3-(1,2,4-triazol-1-yl)propyl phosphonate indicated that Mn-IGPD contained 0.9 +/- 0.1 catalytic sites/protomer. The activity nearly doubled in the presence of high concentrations of Mn2+; the apparent Ks for stimulation was 20 microM. The basis of this effect was obscure, since there was no corresponding increase in the titre of active sites. Neither was there a discernable shift in the values of Km or Ki (above), although exogenous Mn2+ did reduce the optimum pH for kcat, from 7.2 to 6.8. On the basis of a single site/subunit, the maximum rate of catalytic turnover at 30 degrees C was 32 s-1.
酿酒酵母的HIS3+基因在大肠杆菌中过表达,重组咪唑甘油磷酸脱水酶(IGPD)被纯化至同质。激光解吸和电喷雾质谱表明,基于蛋白质序列,分子离子在预期值(23833.3)的2个单位范围内,约一半的多肽缺乏N端甲酰甲硫氨酸残基。最初作为脱辅基蛋白纯化的IGPD无催化活性,主要是Mr为70,000的三聚体。添加Mn2+(而非Mg2+)导致其组装成一种活性酶(40单位/毫克),即Mn-IGPD,由24个亚基组成(Mr为573,000),每个多肽亚基含有1.35±0.1个Mn原子。当重组大肠杆菌的发酵罐生长培养基补充MnCl2时,也获得了具有相同活性和金属含量的酶,IGPD通过Mn-IGPD而非脱辅基酶进行纯化并在体外组装。EDTA抑制表明内在的Mn2+对活性至关重要。在稀释至极低酶浓度(<20 nM)后活性随时间的保持表明金属与蛋白质紧密结合。开发了一种新型连续测定方法以促进Mn-IGPD的动力学表征。在pH 7.0时,IGP的Km为0.10±0.02 mM,1,2,4-三唑抑制的Ki值为0.12±0.02 mM。与其他报道相反,硫醇对催化活性没有影响。Mn-IGPD的活性随酶浓度变化,表明在极低浓度下它会解离为活性较低的形式。从进程曲线的形状推断,产物咪唑丙酮磷酸有显著抑制作用。用强效竞争性抑制剂2-羟基-3-(1,2,4-三唑-1-基)丙基膦酸滴定表明Mn-IGPD每个原体含有0.9±0.1个催化位点。在高浓度Mn2+存在下活性几乎翻倍;刺激的表观Ks为20 μM。这种效应的基础尚不清楚,因为活性位点的滴定没有相应增加。Km或Ki值(见上文)也没有明显变化,尽管外源Mn2+确实将kcat的最适pH从7.2降至6.8。基于每个亚基一个位点,在30℃时催化周转的最大速率为32 s-1。
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