首页> 外文期刊>Toxicology: An International Journal Concerned with the Effects of Chemicals on Living Systems >Cytochrome P450 reductase-mediated anaerobic biotransformation of ethanol to 1-hydroxyethyl-free radicals and acetaldehyde.
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Cytochrome P450 reductase-mediated anaerobic biotransformation of ethanol to 1-hydroxyethyl-free radicals and acetaldehyde.

机译:细胞色素P450还原酶介导的乙醇厌氧生物转化为1-羟乙基自由基和乙醛。

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摘要

The ability of cytochrome P450 reductase to metabolize ethanol (EtOH) to acetaldehyde (AC) and 1-hydroxyethyl free radicals (1HEt) in anaerobic media was studied. Determination of AC was made by GC-FID analysis of the head space of incubation mixtures. The formation of 1HEt was established by GC-MS analysis of the adduct formed between the radical and the spin trap PBN. Results showed that pure human P450 reductase is able to biotransform EtOH to AC and 1HEt in a NADPH-dependent process under an oxygen-free nitrogen atmosphere. Pure FAD in the presence of NADPH was also able to generate AC and 1HEt from the alcohol. Anaerobic incubation mixtures containing either rat liver microsomes or pure nuclei were also able to biotransform EtOH to AC and 1HEt in the presence of NADPH. These processes were inhibited by antibody against rat liver microsomal P450 reductase. Results suggest that semiquinone forms of the flavin in P450 reductase may biotransform EtOH. These reactions might be of some significance in tissues where the P450 reductase is present in the absence of specific forms of cytochrome P450 known to be involved in EtOH metabolism (e.g. CYP2E1). However the toxicological significance of this enzymatic process remains to be established.
机译:研究了细胞色素P450还原酶在厌氧培养基中将乙醇(EtOH)代谢为乙醛(AC)和1-羟乙基自由基(1HEt)的能力。通过GC-FID分析孵育混合物的顶部空间来测定AC。通过GC-MS分析自由基和自旋阱PBN之间形成的加合物,确定了1HEt的形成。结果表明,纯人P450还原酶能够在NADPH依赖性过程中在无氧的氮气气氛下将EtOH生物转化为AC和1HEt。在NADPH存在下,纯FAD也能够从酒精中生成AC和1HEt。在NADPH存在下,含有大鼠肝微粒体或纯核的厌氧培养混合物也能够将EtOH生物转化为AC和1HEt。这些过程被抗大鼠肝微粒体P450还原酶的抗体抑制。结果表明,P450还原酶中黄素的半醌形式可能会生物转化EtOH。这些反应在没有已知参与EtOH代谢的特定形式的细胞色素P450的特定形式(例如CYP2E1)的情况下在存在P450还原酶的组织中可能具有某些意义。然而,该酶促过程的毒理学意义尚待确定。

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