Copik Alicja J, Swierczek Sabina I, Lowther W Todd, D'souza Ventris M, Matthews Brian W, Holz Richard C
Department of Chemistry and Biochemistry, Utah State University, Logan 84322-0300, USA.
Biochemistry. 2003 May 27;42(20):6283-92. doi: 10.1021/bi027327s.
To gain insight into the role of the strictly conserved histidine residue, H178, in the reaction mechanism of the methionyl aminopeptidase from Escherichia coli (EcMetAP-I), the H178A mutant enzyme was prepared. Metal-reconstituted H178A binds only one equivalent of Co(II) or Fe(II) tightly with affinities that are identical to the WT enzyme based on kinetic and isothermal titration calorimetry (ITC) data. Electronic absorption spectra of Co(II)-loaded H178A EcMetAP-I indicate that the active site divalent metal ion is pentacoordinate, identical to the WT enzyme. These data indicate that the metal binding site has not been affected by altering H178. The effect of altering H178 on activity is, in general, due to a decrease in k(cat). The k(cat) value for Co(II)-loaded H178A decreased 70-fold toward MGMM and 290-fold toward MP-p-NA compared to the WT enzyme, while k(cat) decreased 50-fold toward MGMM for the Fe(II)-loaded H178A enzyme and 140-fold toward MP-p-NA. The K(m) values for MGMM remained unaffected, while those for MP-p-NA increased approximately 2-fold for Co(II)- and Fe(II)-loaded H178A. The k(cat)/K(m) values for both Co(II)- and Fe(II)-loaded H178A toward both substrates ranged from approximately 50- to 580-fold reduction. The pH dependence of log K(m), log k(cat), and log(k(cat)/K(m)) of both WT and H178A EcMetAP-I were also obtained and are identical, within error, for H178A and WT EcMetAP-I. Therefore, H178A is catalytically important but is not required for catalysis. Assignment of one of the observed pK(a) values at 8.1 for WT EcMetAP-I was obtained from plots of molar absorptivity at lambda(max(640)) vs pH for both WT and H178A EcMetAP-I. Apparent pK(a) values of 8.1 and 7.6 were obtained for WT and H178A EcMetAP-I, respectively, and were assigned to the deprotonation of a metal-bound water molecule. The data reported herein provide support for the key elements of the previously proposed mechanism and suggest that a similar mechanism can apply to the enzyme with a single metal in the active site.
为深入了解严格保守的组氨酸残基H178在大肠杆菌甲硫氨酰氨肽酶(EcMetAP-I)反应机制中的作用,制备了H178A突变酶。基于动力学和等温滴定量热法(ITC)数据,金属重构的H178A仅紧密结合一当量的Co(II)或Fe(II),其亲和力与野生型酶相同。负载Co(II)的H178A EcMetAP-I的电子吸收光谱表明,活性位点二价金属离子为五配位,与野生型酶相同。这些数据表明,金属结合位点未受H178改变的影响。一般来说,改变H178对活性的影响是由于k(cat)降低。与野生型酶相比,负载Co(II)的H178A对MGMM的k(cat)值降低了70倍,对MP-p-NA降低了290倍,而负载Fe(II)的H178A酶对MGMM的k(cat)降低了50倍,对MP-p-NA降低了140倍。MGMM的K(m)值未受影响,而负载Co(II)和Fe(II)的H178A对MP-p-NA的K(m)值增加了约2倍。负载Co(II)和Fe(II)的H178A对两种底物的k(cat)/K(m)值降低了约50至580倍。还获得了野生型和H178A EcMetAP-I的log K(m)、log k(cat)和log(k(cat)/K(m))的pH依赖性,并且在误差范围内,H178A和野生型EcMetAP-I的结果相同。因此,H178A具有催化重要性,但不是催化所必需的。野生型EcMetAP-I在8.1处观察到的一个pK(a)值是通过绘制野生型和H178A EcMetAP-I在λ(max(640))处的摩尔吸光率与pH的关系图得到的。野生型和H178A EcMetAP-I的表观pK(a)值分别为8.1和7.6,并归因于金属结合水分子的去质子化。本文报道的数据为先前提出的机制的关键要素提供了支持,并表明类似的机制可适用于活性位点含有单一金属的酶。
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