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固定于壳聚糖-[C4mim][BF4]膜中的辣根过氧化物酶的直接电化学:电极动力学参数的测定

Direct electrochemistry of horseradish peroxidase immobilized in a chitosan-[C4mim][BF4] film: determination of electrode kinetic parameters.

作者信息

Long Jenny S, Silvester Debbie S, Wildgoose Gregory G, Surkus Annette-E, Flechsig Gerd-Uwe, Compton Richard G

机构信息

Department of Chemistry, Physical and Theoretical Chemistry Laboratory, Oxford University, South Parks Road, Oxford OX1 3QZ, United Kingdom.

出版信息

Bioelectrochemistry. 2008 Nov;74(1):183-7. doi: 10.1016/j.bioelechem.2008.07.008. Epub 2008 Aug 7.

Abstract

The direct electrochemistry of a HRP-chi-[C(4)mim][BF(4)] film (where HRP = horseradish peroxidase, chi = chitosan, and [C(4)mim][BF(4)] = the room temperature ionic liquid (RTIL) 1-butyl-3-methylimidazolium tetrafluoroborate) has been studied by cyclic voltammetry on a glassy carbon electrode. The mechanism for the electrochemical reaction of HRP is suggested to be EC for the reduction, and CE for the following re-oxidation, as the oxidative peak potential remained approximately unchanged across the scan rate range. The half wave potential of HRP reduction was found to be pH dependent, suggesting that a concomitant proton and electron transfer is occurring. Using theoretical simulations of the experimentally obtained peak positions, the standard electron transfer rate constant, k(0), was found to be 98 (+/-16) s(-1) at 295 K in pH 7 phosphate buffer solution, which is very close to the value reported in the absence of ionic liquid. This suggests that the ionic liquid used here in the HRP-chi-[C(4)mim][BF(4)]/GC electrode does not enhance the rate of electron transfer. k(0) was found to increase systematically with increasing temperature and followed a linear Arrhenius relation, giving an activation energy of 14.20 kJ mol(-1). The electrode kinetics and activation energies obtained are identical to those reported for HRP films in aqueous media. This leads us to question if the use of RTIL films provide any unique benefits for enzyme/protein voltammetry. Rather the films may likely contain aqueous zones in which the enzymes are located and undergo electron transfer.

摘要

通过循环伏安法在玻碳电极上研究了HRP-壳聚糖-[C(4)mim][BF(4)]膜(其中HRP =辣根过氧化物酶,壳聚糖 =壳聚糖,[C(4)mim][BF(4)] =室温离子液体1-丁基-3-甲基咪唑四氟硼酸盐)的直接电化学。HRP电化学反应的机理被认为还原时为EC,随后的再氧化时为CE,因为氧化峰电位在扫描速率范围内大致保持不变。发现HRP还原的半波电位与pH有关,表明同时发生了质子和电子转移。通过对实验获得的峰位置进行理论模拟,发现在295K的pH 7磷酸盐缓冲溶液中,标准电子转移速率常数k(0)为98(±16)s(-1),这与在无离子液体时报道的值非常接近。这表明在HRP-壳聚糖-[C(4)mim][BF(4)]/GC电极中使用的离子液体不会提高电子转移速率。发现k(0)随温度升高而系统地增加,并遵循线性阿伦尼乌斯关系,给出的活化能为14.20kJ mol(-1)。获得的电极动力学和活化能与在水性介质中报道的HRP膜的相同。这使我们质疑使用室温离子液体膜是否为酶/蛋白质伏安法提供任何独特的优势。相反,这些膜可能包含酶所在并进行电子转移的水相区域。

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