Michał Szczepańczyk, Lea Paul, T. Ruzgas, Sebastian Björklund
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引用次数: 0
Abstract
Catalase is a key antioxidative enzyme, and a deficiency or malfunction of catalase is hypothesized to be related to various diseases. To investigate catalase activity, it is important to use reliable methods and experimental protocols enabling consistent fallouts. One major problem, however, is that the activity values obtained with different techniques and procedures can vary to a large extent. The aim of this work was to identify experimental conditions that provide similar catalase activity values with two different methods based on either spectrophotometry or chronoamperometry. The investigated parameters include the concentration of catalase and its substrate (H2O2), as well as the effect of deoxygenation of the catalase medium by nitrogen (N2). Within the frame of investigated conditions, we show that spectrophotometry is strongly affected by the catalase concentration, whereas chronoamperometry is shown to be more dependent on the substrate concentration. Deoxygenation leads to elevated catalase activity values in the case of chronoamperometry, whereas it shows no influence on the results obtained with spectrophotometry. In particular, in the case of low substrate concentrations (i.e., low catalase reaction rates), higher and more accurate results are obtained with deoxygenation in the case of chronoamperometry measurements due to minimized oxygen escape. The effect of deoxygenation, giving rise to elevated catalase activity values, however, is not statistically significant at high substrate concentrations, implying that the protocol can be simplified by excluding this step as long as the other parameters are optimized. Finally, by comparing the two methods at different experimental conditions, we identified protocols resulting in similar results, i.e., 10 mM H2O2 and catalase activity of 4–5 U/mL. Based on this work, improved consistency of catalase activity data obtained with different methodologies and in different labs is expected.
过氧化氢酶是一种关键的抗氧化酶,过氧化氢酶的缺乏或功能障碍被认为与各种疾病有关。为了研究过氧化氢酶活性,重要的是使用可靠的方法和实验方案来实现一致的下降。然而,一个主要问题是,用不同的技术和程序获得的活性值可能在很大程度上变化。这项工作的目的是通过基于分光光度法或计时电流法的两种不同方法来确定提供相似过氧化氢酶活性值的实验条件。研究的参数包括过氧化氢酶及其底物(H2O2)的浓度,以及氮(N2)对过氧化氢酶培养基的脱氧作用。在所研究的条件范围内,我们发现分光光度法受到过氧化氢酶浓度的强烈影响,而计时电流法则更依赖于底物浓度。在计时电流法的情况下,脱氧会导致过氧化氢酶活性值升高,而它对分光光度法获得的结果没有影响。特别地,在低底物浓度(即,低过氧化氢酶反应速率)的情况下,在计时电流法测量的情况下通过脱氧获得更高和更准确的结果,这是由于氧气逸出最小化。然而,脱氧作用导致过氧化氢酶活性值升高,在高底物浓度下没有统计学意义,这意味着只要优化其他参数,就可以通过排除这一步骤来简化方案。最后,通过在不同实验条件下比较这两种方法,我们确定了产生类似结果的方案,即10 mM H2O2和4–5 U/mL的过氧化氢酶活性。基于这项工作,预计在不同的方法和实验室中获得的过氧化氢酶活性数据的一致性会得到提高。
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