首页> 美国卫生研究院文献>Biochemical Journal >Hydroxylation of salicylate by microsomal fractions and cytochrome P-450. Lack of production of 23-dihydroxybenzoate unless hydroxyl radical formation is permitted.
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Hydroxylation of salicylate by microsomal fractions and cytochrome P-450. Lack of production of 23-dihydroxybenzoate unless hydroxyl radical formation is permitted.

机译:水杨酸酯通过微粒体级分和细胞色素P-450的羟化作用。除非允许形成羟基自由基否则不生产23-二羟基苯甲酸酯。

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摘要

Attack by hydroxyl radicals (.OH) upon salicylate (2-hydroxybenzoate) leads to formation of both 2,3-dihydroxybenzoate (2,3-DHB) and 2,5-dihydroxybenzoate (gentisate, 2,5-DHB). It has been suggested that formation of 2,3-DHB from salicylate is a means of monitoring .OH formation. Production of 2,3-DHB and 2,5-DHB by liver microsomal fractions and isoforms of cytochrome P-450 was investigated. Liver microsomes prepared from variously treated rats and rabbits catalysed the formation of 2,5-DHB but not 2,3-DHB. Formation of 2,5-DHB was inhibited by CO, metyrapone and SKF-525A, but not by the .OH scavengers mannitol and formate or by the iron chelator desferrioxamine. Purified P-450s IIE1, IIB4 or IA2 from rabbit liver microsomes, reconstituted together with NADPH-cytochrome P-450 reductase, led to formation of equal amounts of 2,3-DHB and 2,5-DHB in reactions that were almost completely inhibited by mannitol or formate. Addition of Fe3+/EDTA either to microsomes or to membranes containing reconstituted P-450 caused formation of approximately equal amounts of 2,3-DHB and 2,5-DHB, consistent with an .OH-dependent attack on salicylate. The data indicate that the microsomal P-450 system catalyses hydroxylation of salicylate to 2,5-DHB, but not formation of 2,3-DHB. Hence measurement of 2,3-DHB might provide a means of monitoring .OH formation. Care must be taken in studies of substrate hydroxylation by microsomes or reconstituted P-450 systems to avoid artefacts resulting from .OH generation.
机译:羟基自由基(.OH)对水杨酸酯(2-羟基苯甲酸酯)的攻击导致形成2,3-二羟基苯甲酸酯(2,3-DHB)和2,5-二羟基苯甲酸酯(龙胆酸酯,2,5-DHB)。已经提出,由水杨酸酯形成2,3-DHB是监测.OH形成的手段。研究了肝微粒体组分和细胞色素P-450的同工型产生的2,3-DHB和2,5-DHB。由不同处理的大鼠和兔子制备的肝微粒体催化2,5-DHB的形成,但不催化2,3-DHB的形成。 2,5-DHB的形成受CO,甲吡酮和SKF-525A抑制,但不受.OH清除剂甘露醇和甲酸盐或铁螯合剂去铁胺的抑制。从兔肝微粒体中纯化的P-450 IIE1,IIB4或IA2与NADPH-细胞色素P-450还原酶一起重建,导致几乎完全被抑制的反应中形成相等量的2,3-DHB和2,5-DHB甘露醇或甲酸盐。将Fe3 + / EDTA加到微粒体或含有重构的P-450的膜中会导致形成大约相等量的2,3-DHB和2,5-DHB,这与对水杨酸酯的.OH依赖性攻击相一致。数据表明,微粒体P-450系统催化水杨酸酯羟基化为2,5-DHB,但不形成2,3-DHB。因此,对2,3-DHB的测量可能提供监测.OH形成的方法。在研究微粒体或重构的P-450系统对底物羟基化的过程中,必须注意避免产生.OH造成的假象。

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