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细胞色素P-450/还原酶比率对乙醇氧化及羟基自由基清除剂2-酮-4-硫代甲基丁酸(KMBA)的不同影响。

Differential effects of the cytochrome P-450/reductase ratio on the oxidation of ethanol and the hydroxyl radical scavenging agent 2-keto-4-thiomethylbutyric acid (KMBA).

作者信息

Winston G W, Cederbaum A I

出版信息

Biochem Pharmacol. 1986 Nov 15;35(22):4053-8. doi: 10.1016/0006-2952(86)90027-4.

Abstract

NADPH-cytochrome P-450 reductase catalyzes a low rate of oxidation of hydroxyl radical scavenging agents such as ethanol and 2-keto-4-thiomethylbutyric acid (KMBA), in a reaction markedly stimulated by the addition of ferric-EDTA. The effect of various ratios of cytochrome P-450 (phenobarbital-inducible isozyme)/reductase on the oxidation of ethanol and KMBA was determined: There was essentially no increase in KMBA oxidation over the range of ratios from 0.5 to 5 as compared to the reductase-catalyzed rate. High ratios actually caused some decrease in KMBA oxidation, which was especially notable under conditions of increased rates of hydroxyl radical generation (presence of increasing amounts of ferric-EDTA). This decrease at high P-450/reductase ratios could reflect tight coupling of reductase to P-450-PB, therefore decreasing electron transfer from reductase to ferric-EDTA, or could involve non-specific scavenging of .OH by P-450-PB. Indeed, native, but not boiled, P-450 inhibited KMBA oxidation by the xanthine oxidase system. By contrast, the oxidation of ethanol was stimulated at all concentrations of P-450-PB, and this increase was not sensitive to desferrioxamine. However, under conditions of high rates of .OH production, the ethanol oxidation profile tended to resemble the KMBA oxidation profile with respect to the effect of P-450-PB, whereas the two profiles were different under conditions of low rates of .OH production. These results suggest that P-450-PB does not catalyze the oxidation of .OH scavengers or promote the production of .OH, even at ratios of P-450/reductase approaching those found with intact microsomes and even in the presence of excess iron-EDTA, whereas ethanol is directly oxidized by P-450-PB, as are typical drug substrates. However, the P-450-PB-dependent oxidation of ethanol can be masked under conditions in which .OH production is increased.

摘要

NADPH-细胞色素P-450还原酶催化乙醇和2-酮-4-硫代甲基丁酸(KMBA)等羟基自由基清除剂的氧化速率较低,在添加铁-EDTA的反应中,该反应受到显著刺激。测定了细胞色素P-450(苯巴比妥诱导同工酶)/还原酶的不同比例对乙醇和KMBA氧化的影响:与还原酶催化的速率相比,在0.5至5的比例范围内,KMBA氧化基本没有增加。高比例实际上导致KMBA氧化有所下降,在羟基自由基生成速率增加的条件下(铁-EDTA含量增加)尤其明显。在高P-450/还原酶比例下的这种下降可能反映了还原酶与P-450-PB的紧密偶联,因此减少了从还原酶到铁-EDTA的电子转移,或者可能涉及P-450-PB对·OH的非特异性清除。事实上,天然的而非煮沸的P-450抑制了黄嘌呤氧化酶系统对KMBA的氧化。相比之下,在所有浓度的P-450-PB下,乙醇的氧化都受到刺激,并且这种增加对去铁胺不敏感。然而,在高·OH产生速率的条件下,就P-450-PB的影响而言,乙醇氧化曲线倾向于类似于KMBA氧化曲线,而在低·OH产生速率的条件下,这两条曲线是不同的。这些结果表明,即使在P-450/还原酶比例接近完整微粒体中的比例且存在过量铁-EDTA的情况下,P-450-PB也不催化羟基自由基清除剂的氧化或促进·OH的产生,而乙醇则像典型的药物底物一样被P-450-PB直接氧化。然而,在·OH产生增加的条件下,P-450-PB依赖的乙醇氧化可能会被掩盖。

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