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来自苯巴比妥和β-萘黄酮诱导动物的小鼠肝脏S9组分微粒体单加氧酶在各种长期储存条件下的稳定性。

Stability of microsomal monooxygenases in murine liver S9 fractions derived from phenobarbital and beta-naphthoflavone induced animals under various long-term conditions of storage.

作者信息

Bauer C, Corsi C, Paolini M

机构信息

Dipartimento di Fisiologia e Biochimica, Laboratori di Biochimica, Pisa, Italy.

出版信息

Teratog Carcinog Mutagen. 1994;14(1):13-22. doi: 10.1002/tcm.1770140103.

DOI:10.1002/tcm.1770140103
PMID:7910416
Abstract

The aim of this study was to define the long-term stability of metabolizing enzymes in activating preparations for short-term genotoxicity bioassays under various storage conditions. Expressions of cytochrome P450 content, NADPH-cytochrome (P450) c-reductase activity, and of the several monooxygenases, such as aminopyrine N-demethylase (class IIIA P450), p-nitroanisole O-demethylase (mixed), dinemorphan N-demethylase (IIB1), ethoxyresorufin O-deethylase (IA1), ethoxycoumarin O-deethylase (mixed), and pentoxyresorufin O-dealkylase (IIB1), were examined in S9 fractions derived from Na-phenobarbital (PB) plus beta-naphthoflavone (beta-NF) induced male and female mice, stored at -80 degrees C, or lyophilized and stored at -20 degrees C. Lipid peroxidation was also determined. Cytochrome P450 and the associated activities were decreased by 30-82% within 9 months of storage. The pattern and degree of relative stabilities were different for the various isoforms. The IA1-like activity, for example, was much more stable (approximately 49% loss) than IIB1-like activities (up to 82% loss). In general, lyophilized enzymes were less stable than directly frozen preparations. In addition, immediately after freeze-drying (lyophilization), a marked decrease in activity of up to 35% was observed. On the contrary, demethylation of aminopyrine and p-nitroanisole remains almost constant over 6 months storage at -196 degrees C. The results obtained indicate that either fresh, daily made S9 fractions or, alternatively, fractions stored in liquid nitrogen (up to 6 months) are recommended for mutagenesis studies.

摘要

本研究的目的是确定在各种储存条件下,用于短期遗传毒性生物测定的活化制剂中代谢酶的长期稳定性。检测了细胞色素P450含量、NADPH-细胞色素(P450)c-还原酶活性以及几种单加氧酶的表达,这些单加氧酶包括氨基比林N-脱甲基酶(ⅢA类P450)、对硝基苯甲醚O-脱甲基酶(混合)、地尼吗啡N-脱甲基酶(ⅡB1)、乙氧异黄酮O-脱乙基酶(ⅠA1)、乙氧香豆素O-脱乙基酶(混合)和戊氧异黄酮O-脱烷基酶(ⅡB1),它们来自于经苯巴比妥钠(PB)加β-萘黄酮(β-NF)诱导的雄性和雌性小鼠的S9组分,这些组分储存在-80℃或冻干后储存在-20℃。还测定了脂质过氧化情况。细胞色素P450及其相关活性在储存9个月内下降了30%-82%。不同同工型的相对稳定性模式和程度有所不同。例如,ⅠA1样活性比ⅡB1样活性稳定得多(损失约49%)(损失高达82%)。一般来说,冻干酶比直接冷冻的制剂稳定性差。此外,在冻干后立即观察到活性显著下降高达35%。相反,氨基比林和对硝基苯甲醚的脱甲基在-196℃储存6个月期间几乎保持不变。所得结果表明,诱变研究推荐使用新鲜的、每日制备的S9组分,或者储存在液氮中的组分(长达6个月)。

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