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2,5-二氯-1,4-苯醌对刀豆脲酶活性的影响。抑制作用、总还原能力及DPPH自由基清除活性。

Influence of 2,5-dichloro-1,4-benzoquinone on jack bean urease activity. Inhibitory effect, total reducing capacity and DPPH radical scavenging activity.

作者信息

Kot Mirosława, Olech Zofia

机构信息

Jagiellonian University, Kraków, Poland.

出版信息

Acta Biochim Pol. 2011;58(4):627-33. Epub 2011 Dec 15.

Abstract

Inhibition of jack bean activity by 2,5-dichloro-1,4-benzoquinone (DCBQ) was studied in phosphate buffer, pH 7.0. It was found that DCBQ acted as a strong, time and concentration dependent inactivator of urease. Under the experimental conditions obeyed the terms of pseudo-first-order reaction, urease was totally inactivated. Application of Wilson-Kitz method proved that the urease-DCBQ interaction followed a simple bimolecular process and the presence of intermediate complex was undetectable. The determined second order rate constant of the inactivation was 0.053 (μM min)(-1). Thiols such as l-cysteine, glutathione and dithiothreitol (DTT) protected urease from inhibition by DCBQ but DCBQ-modified urease did not regain its activity after DTT application. The thiol protective studies indicated an essential role of urease thiol(s) in the inhibition. The irreversibility of the inactivation showed that the process was a result of a direct modification of urease thiol(s) by DCBQ (DCBQ chlorine(s) substitution). The decomposition of DCBQ in aqueous solution at natural light exposure was monitored by visible spectrophotometry, determination of the total reducing capacity (Folin-Ciocalteu method) and DPPH (2,2-diphenyl-1-picrylhydrazyl) radical scavenging ability. The DCBQ conversion resulted in a decrease of the inhibition power and was well correlated with the increase of the total reducing capacity and DPPH scavenging ability. These findings were attributed to DCBQ transformation by photolysis and the hydrolysis effect was found to be negligible.

摘要

在pH 7.0的磷酸盐缓冲液中研究了2,5-二氯-1,4-苯醌(DCBQ)对刀豆脲酶活性的抑制作用。发现DCBQ是一种强效的、时间和浓度依赖性的脲酶失活剂。在符合准一级反应条件的实验条件下,脲酶完全失活。应用Wilson-Kitz方法证明脲酶与DCBQ的相互作用遵循简单的双分子过程,且未检测到中间复合物。测定的失活二级速率常数为0.053(μM·min)⁻¹。硫醇如L-半胱氨酸、谷胱甘肽和二硫苏糖醇(DTT)可保护脲酶免受DCBQ的抑制,但DCBQ修饰后的脲酶在应用DTT后不能恢复其活性。硫醇保护研究表明脲酶中的硫醇在抑制过程中起重要作用。失活的不可逆性表明该过程是DCBQ对脲酶硫醇直接修饰(DCBQ氯取代)的结果。通过可见分光光度法、总还原能力测定(Folin-Ciocalteu法)和DPPH(2,2-二苯基-1-苦基肼)自由基清除能力监测自然光照射下水溶液中DCBQ的分解。DCBQ的转化导致抑制能力下降,且与总还原能力和DPPH清除能力的增加密切相关。这些发现归因于DCBQ的光解转化,且发现水解作用可忽略不计。

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