首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Resonance Raman evidence for oxygen exchange between the FeIV = O heme and bulk water during enzymic catalysis of horseradish peroxidase and its relation with the heme-linked ionization.
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Resonance Raman evidence for oxygen exchange between the FeIV = O heme and bulk water during enzymic catalysis of horseradish peroxidase and its relation with the heme-linked ionization.

机译:辣根过氧化物酶的酶催化过程中FeIV = O血红素与大量水之间的氧交换的共振拉曼证据及其与血红素连接的电离的关系。

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摘要

Raman spectroscopic studies of compound II of horseradish peroxidase show that the oxygen atom in the FeIV = O group of the heme is rapidly exchanged in H2O at pH 7.0 but not in an alkaline solution (pH 11.0). This conclusion is based on studies of shift in the FeIV = O stretching mode of compound II in H2(18)O; further studies show that the FeIV = O heme is hydrogen-bonded to an amino acid residue of the protein in neutral solutions but not in the alkaline solution. Deprotonation of this residue takes place with the midpoint pH at 8.8 and accordingly corresponds to the so-called heme-linked ionization. It is concluded that this hydrogen-bonded proton plays an important part in the oxygen exchange mechanism. From this it seems clear that this hydrogen-bonded proton has an essential role in the acid/base catalysis of this enzyme and that alkaline deactivation of this enzyme can be attributed to the lack of a hydrogen-bonded proton at high pH.
机译:辣根过氧化物酶化合物II的拉曼光谱研究表明,血红素FeIV = O基团中的氧原子在pH 7.0的H2O中迅速交换,而在碱性溶液(pH 11.0)中则不交换。该结论基于对化合物II在H2(18)O中FeIV = O拉伸模式的转变的研究。进一步的研究表明,FeIV = O血红素在中性溶液中氢键合到蛋白质的氨基酸残基上,而不在碱性溶液中。该残留物的去质子化在中点pH为8.8时发生,因此对应于所谓的血红素连接电离。结论是该氢键质子在氧交换机理中起重要作用。由此看来,显然氢键合的质子在该酶的酸/碱催化中具有重要作用,并且该酶的碱失活可以归因于在高pH下缺乏氢键合的质子。

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