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A Modified Fluorimetric Method for Determination of Hydrogen Peroxide Using Homovanillic Acid Oxidation Principle

机译:高香草酸氧化原理改进的荧光法测定过氧化氢

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摘要

Hydrogen peroxide (H2O2) level in biological samples is used as an important index in various studies. Quantification of H2O2 level in tissue fractions in presence of H2O2 metabolizing enzymes may always provide an incorrect result. A modification is proposed for the spectrofluorimetric determination of H2O2 in homovanillic acid (HVA) oxidation method. The modification was included to precipitate biological samples with cold trichloroacetic acid (TCA, 5% w/v) followed by its neutralization with K2HPO4 before the fluorimetric estimation of H2O2 is performed. TCA was used to precipitate the protein portions contained in the tissue fractions. After employing the above modification, it was observed that H2O2 content in tissue samples was ≥2 fold higher than the content observed in unmodified method. Minimum 2 h incubation of samples in reaction mixture was required for completion of the reaction. The stability of the HVA dimer as reaction product was found to be >12 h. The method was validated by using known concentrations of H2O2 and catalase enzyme that quenches H2O2 as substrate. This method can be used efficiently to determine more accurate tissue H2O2 level without using internal standard and multiple samples can be processed at a time with additional low cost reagents such as TCA and K2HPO4.
机译:生物样品中的过氧化氢(H2O2)水平被用作各种研究的重要指标。在存在H2O2代谢酶的情况下,对组织部分中H2O2含量的定量可能总是会提供错误的结果。提出了一种改进方法,用于在高香草酸(HVA)氧化方法中分光荧光法测定H2O2。包括该修饰以用冷的三氯乙酸(TCA,5%w / v)沉淀生物样品,然后用K2HPO4中和,然后进行H2O2的荧光估算。 TCA用于沉淀组织级分中包含的蛋白质部分。使用上述修饰后,观察到组织样品中的H2O2含量比未修饰方法中观察到的高出2倍以上。完成反应至少需要在反应混合物中孵育2小时。发现作为反应产物的HVA二聚​​体的稳定性> 12 h。该方法通过使用已知浓度的H2O2和过氧化氢酶来淬灭H 2 O 2 作为底物进行验证。该方法可以有效地用于确定更准确的组织H 2 O 2 水平,而无需使用内标物,并且可以使用其他低成本试剂同时处理多个样品,例如TCA和K 2 HPO 4

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    Biswaranjan Paital;

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  • 年(卷),期 -1(2014),-1
  • 年度 -1
  • 页码 342958
  • 总页数 8
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