两类不同脱氢奎尼酸酶的酶学性质与生物物理性质比较
A comparison of the enzymological and biophysical properties of two distinct classes of dehydroquinase enzymes.
作者信息
Kleanthous C, Deka R, Davis K, Kelly S M, Cooper A, Harding S E, Price N C, Hawkins A R, Coggins J R
机构信息
Department of Biochemistry, University of Glasgow, U.K.
出版信息
Biochem J. 1992 Mar 15;282 ( Pt 3)(Pt 3):687-95. doi: 10.1042/bj2820687.
This paper compares the biophysical and mechanistic properties of a typical type I dehydroquinase (DHQase), from the biosynthetic shikimate pathway of Escherichia coli, and a typical type II DHQase, from the quinate pathway of Aspergillus nidulans. C.d. shows that the two proteins have different secondary-structure compositions; the type I enzyme contains approx. 50% alpha-helix while the type II enzyme contains approx. 75% alpha-helix. The stability of the two types of DHQase was compared by denaturant-induced unfolding, as monitored by c.d., and by differential scanning calorimetry. The type II enzyme unfolds at concentrations of denaturant 4-fold greater than the type I and through a series of discrete transitions, while the type I enzyme unfolds in a single transition. These differences in conformational stability were also evident from the calorimetric experiments which show that type I DHQase unfolds as a single co-operative dimer at 57 degrees C whereas the type II enzyme unfolds above 82 degrees C and through a series of transitions suggesting higher orders of structure than that seen for the type I enzyme. Sedimentation and Mr analysis of both proteins by analytical ultracentrifugation is consistent with the unfolding data. The type I DHQase exists predominantly as a dimer with Mr = 46,000 +/- 2000 (a weighted average affected by the presence of monomer) and has a sedimentation coefficient s0(20,w) = 4.12 (+/- 0.08) S whereas the type II enzyme is a dodecamer, weight-average Mr = 190,000 +/- 10,000 and has a sedimentation coefficient, s0(20,w) = 9.96 (+/- 0.21) S. Although both enzymes have reactive histidine residues in the active site and can be inactivated by diethyl pyrocarbonate, the possibility that these structurally dissimilar enzymes catalyse the same dehydration reaction by the same catalytic mechanism is deemed unlikely by three criteria: (1) they have very different pH/log kcat. profiles and pH optima; (2) imine intermediates, which are known to play a central role in the mechanism of type I enzymes, could not be detected (by borohydride reduction) in the type II enzyme; (3) unlike Schiff's base-forming type I enzymes, there are no conserved lysine residues in type II amino acid sequences.
本文比较了来自大肠杆菌生物合成莽草酸途径的典型I型脱氢奎尼酸酶(DHQase)和来自构巢曲霉奎尼酸途径的典型II型DHQase的生物物理和作用机制特性。圆二色光谱显示这两种蛋白质具有不同的二级结构组成;I型酶含有约50%的α-螺旋,而II型酶含有约75%的α-螺旋。通过变性剂诱导的解折叠对两种类型的DHQase的稳定性进行了比较,通过圆二色光谱监测,并采用差示扫描量热法。II型酶在变性剂浓度比I型酶高4倍时解折叠,且通过一系列离散转变,而I型酶以单一转变解折叠。这些构象稳定性的差异在量热实验中也很明显,实验表明I型DHQase在57℃时作为单一协同二聚体解折叠,而II型酶在82℃以上解折叠,并通过一系列转变,表明其结构比I型酶具有更高的有序性。通过分析超速离心对两种蛋白质进行沉降和相对分子质量分析,结果与解折叠数据一致。I型DHQase主要以二聚体形式存在,相对分子质量为46,000±2000(受单体存在影响的加权平均值),沉降系数s0(20,w)=4.12(±0.08)S,而II型酶是十二聚体,重均相对分子质量为190,000±10,000,沉降系数s0(20,w)=9.96(±0.21)S。尽管两种酶在活性位点都有反应性组氨酸残基,并且都可被焦碳酸二乙酯灭活,但根据三个标准,认为这些结构不同的酶通过相同催化机制催化相同脱水反应的可能性不大:(1)它们具有非常不同的pH/log kcat曲线和最适pH;(2)在II型酶中未检测到(通过硼氢化钠还原)在I型酶机制中起核心作用的亚胺中间体;(3)与形成席夫碱的I型酶不同,II型氨基酸序列中没有保守的赖氨酸残基。
Zotero 插件