Simple procedures for purification and stabilization of human serum paraoxonase-1

Journal of biochemical and biophysical methods Pub Date : 2008-04-24 DOI:10.1016/j.jbbm.2007.09.003

Leila Golmanesh , Hossein Mehrani , Mohammad Tabei

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引用次数: 31

Abstract

Human paraoxonases-1 is one of the most important detoxifying enzymes. In this study using simple chromatographic procedures human paraoxonases-1 was purified from human pooled plasma. The enzyme was purified using DEAE Sephadex an anion exchanger and G-200 a gel filtration chromatographic media. Results showed a single band of approximately 43 KD proteins in SDS–PAGE, corresponding to the human PON1. Using paraoxon as the substrate the activity was related to the concentration of calcium and sodium ions (K_m = 1.2 ± 0.2 mM). Phenyl acetate hydrolyzing activity was independent of sodium and calcium ions (K_m = 0.78 ± 0.08 mM). Keeping at 25 °C for 20 days 75% of the enzyme original activity was restored in 20% (v/v) glycerol. EDTA and zinc chloride both inhibited the enzyme activity. In conclusion the applied procedures can be used for large scale purification. It would greatly facilitate their structural and functional characterization and permit examination of their weak, yet potentially most biologically relevant activities, in the complete absence of other serum proteins.

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人血清对氧磷酶-1的纯化和稳定的简单方法

对氧磷酶-1是人体最重要的解毒酶之一。本研究采用简单色谱法从人血浆中纯化人对氧磷酶-1。采用DEAE Sephadex阴离子交换剂和G-200凝胶过滤层析介质纯化酶。结果显示，SDS-PAGE中存在约43个KD蛋白单带，与人类PON1相对应。以对氧磷为底物，其活性与钙离子和钠离子浓度有关(Km = 1.2±0.2 mM)。乙酸苯酯水解活性与钠离子和钙离子无关(Km = 0.78±0.08 mM)。在25℃下保存20天，20% (v/v)甘油中酶活性恢复75%。EDTA和氯化锌均能抑制酶活性。综上所述，该方法可用于大规模提纯。这将极大地促进其结构和功能表征，并允许在完全没有其他血清蛋白的情况下检查其微弱但可能最具生物学相关性的活性。

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Journal of biochemical and biophysical methods

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