Department of Chemistry, Graduate School of Science, Nagoya University, Nagoya, 464-8602, Japan.
Dalton Trans. 2010 Mar 28;39(12):3105-14. doi: 10.1039/b924365h. Epub 2010 Feb 2.
In a previous study, we constructed a prototype thermally tolerant artificial peroxidase from an electron transfer protein, cytochrome c(552) from Thermus thermophilus, and demonstrated that engineering of proteins from thermophiles could be a promising methodology to produce artificial enzymes for practical use. In the present study, further improvement of the prototype (the V49D/M69A mutant) in enzymatic activity and thermal tolerance has been achieved by successive modifications based on detailed analyses of an active intermediate formed in the peroxidase reaction. Spectroscopic studies revealed that the major active intermediate of V49D/M69A was an oxo-ferryl heme with a protein radical predominantly localized on Tyr45. The magnetic power saturation measurement in EPR studies showed little magnetic coupling between the oxo-ferryl heme and the tyrosyl radical. This result indicated that the oxo-ferryl heme and the tyrosyl radical served as isolated oxidants. Kinetics studies indicated that the isolated oxo-ferryl heme component in the active intermediate could be a precursor to heme degradation by the reaction with H(2)O(2). Replacement of Tyr45 with phenylalanine on V49D/M69A resulted in delocalization of the radical over the protein and increased magnetic coupling between the oxo-ferryl heme and the protein radical in the intermediate. The stronger magnetic coupling between the oxo-ferryl heme and the radical was achieved by replacement of Tyr45 with tryptophan, which was similar to a tryptophanyl radical found in active intermediates of some catalase-peroxidases. The protein radical intermediates of the Tyr45 mutants exhibited relatively higher reactivity to an organic substrate than H(2)O(2) in comparison to the basal mutant, V49D/M69A, which was preferable to suppress the heme degradation process. This was reflected in the improved enzymatic activity and thermal tolerance observed for the Tyr45 mutants in the peroxidase reaction.
在之前的研究中,我们构建了一个原型热耐受人工过氧化物酶,该酶来自嗜热菌 Thermus thermophilus 的电子传递蛋白细胞色素 c(552),并证明了对来自嗜热菌的蛋白质进行工程改造可能是一种很有前途的方法,可以生产出用于实际应用的人工酶。在本研究中,通过对过氧化物酶反应中形成的活性中间体进行详细分析,对原型(V49D/M69A 突变体)的酶活性和热耐受性进行了进一步的改进。光谱研究表明,V49D/M69A 的主要活性中间体是具有蛋白自由基的氧合铁血红素,该自由基主要定位于 Tyr45。EPR 研究中的磁功率饱和测量表明,氧合铁血红素和酪氨酸自由基之间的磁偶合很小。这一结果表明,氧合铁血红素和酪氨酸自由基充当了分离的氧化剂。动力学研究表明,活性中间体中分离的氧合铁血红素组分可能是与 H(2)O(2)反应导致血红素降解的前体。在 V49D/M69A 上用苯丙氨酸替换 Tyr45 会导致自由基在蛋白质上离域,并增加中间物中氧合铁血红素和蛋白质自由基之间的磁偶合。用色氨酸替换 Tyr45 可以实现氧合铁血红素和自由基之间更强的磁偶合,这类似于一些过氧化氢酶过氧化物酶的活性中间体中的色氨酸自由基。与基础突变体 V49D/M69A 相比,Tyr45 突变体的蛋白质自由基中间体对有机底物的反应性相对较高,而不是 H(2)O(2),这有利于抑制血红素降解过程。这反映在过氧化物酶反应中观察到 Tyr45 突变体的酶活性和热耐受性得到了提高。
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