内生ochrobacum中间体CL6生成新的胞外耐热草酸氧化酶:纯化和生化表征

Kunal Kumar, P. D. Belur
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引用次数: 8

摘要

草酸氧化酶(EC 1.2.3.4)催化草酸氧化裂解为二氧化碳,并将分子氧还原为过氧化氢。草酸氧化酶在临床血、尿草酸测定中的应用。本研究描述了一种内生细菌Ochrobactrum intermedium CL6产生的草酸氧化酶的纯化和生化特性。对无细胞发酵液进行两步酶纯化,纯化率为58.74倍,回收率为83%。最终纯化酶的比活性为26.78 U mg−1蛋白。该酶的最适pH为3.8℃,最适温度为80℃,在4 ~ 80℃条件下稳定6 h。酶活性不受血清和尿液中常见的金属离子和化学试剂(K+、Na+、Zn2+、Fe3+、Mn2+、Mg2+、葡萄糖、尿素、乳酸)的影响,Cu2+除外。该酶似乎是一种受Ca2+和Fe2+刺激的金属蛋白。对草酸盐的Km和Kcat分别为0.45 mM和85 s−1。该酶是唯一已知的草酸氧化酶,在底物浓度达到50 mM时不表现出底物抑制作用。热稳定性、动力学性质和无底物抑制使该酶成为临床应用的理想候选者。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
New extracellular thermostable oxalate oxidase produced from endophytic Ochrobactrum intermedium CL6: Purification and biochemical characterization
ABSTRACT Oxalate oxidase (EC 1.2.3.4) catalyzes the oxidative cleavage of oxalate to carbon dioxide with the reduction of molecular oxygen to hydrogen peroxide. Oxalate oxidase found its application in clinical assay for oxalate in blood and urine. This study describes the purification and biochemical characterization of an oxalate oxidase produced from an endophytic bacterium, Ochrobactrum intermedium CL6. The cell-free fermentation broth was subjected to two-step enzyme purification, which resulted in a 58.74-fold purification with 83% recovery. Specific activity of the final purified enzyme was 26.78 U mg−1 protein. The enzyme displayed an optimum pH and temperature of 3.8 and 80°C, respectively, and high stability at 4–80°C for 6 h. The enzymatic activity was not influenced by metal ions and chemical agents (K+, Na+, Zn2+, Fe3+, Mn2+, Mg2+, glucose, urea, lactate) commonly found in serum and urine, with Cu2+ being the exception. The enzyme appears to be a metalloprotein stimulated by Ca2+ and Fe2+. Its Km and Kcat for oxalate were found to be 0.45 mM and 85 s−1, respectively. This enzyme is the only known oxalate oxidase which did not show substrate inhibition up to a substrate concentration of 50 mM. Thermostability, kinetic properties, and the absence of substrate inhibition make this enzyme an ideal candidate for clinical applications.
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