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Identification of the residue in human CYP3A4 that is covalently modified by bergamottin and the reactive intermediate that contributes to the grapefruit juice effect

机译:鉴定人类CYP3A4中被佛手柑共价修饰的残基和有助于柚子汁作用的反应性中间体

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Previous studies have demonstrated that bergamottin (BG), a component of grapefruit juice, is a mechanism-based inactivator of CYP3A4 and contributes, in part, to the grapefruit juice-drug interaction. Although the covalent binding of [ 14C]BG to the CYP3A4 apoprotein has been demonstrated by SDS-polyacrylamide gel electrophoresis, the identity of the modified amino acid residue and the reactive intermediate species of BG responsible for the inactivation have not been reported. In the present study, we show that inactivation of CYP3A4 by BG results in formation of a modified apoprotein-3A4 and a GSH conjugate, both exhibiting mass increases of 388 Da, which corresponds to the mass of 6′,7′-dihydroxybergamottin (DHBG), a metabolite of BG, plus one oxygen atom. To identify the adducted residue, BG-inactivated 3A4 was digested with trypsin, and the digests were then analyzed by liquid chromatography-tandem mass spectrometry (MS/MS). A mass shift of 388 Da was used for the SEQUEST database search, which revealed a mass increase of 388 Da for the peptide with the sequence 272LQLMIDSQNSK 282, and MS/MS analysis of the adducted peptide demonstrated that Gln273 is the residue modified. Mutagenesis studies showed that the Gln273 to Val mutant was resistant to inactivation by BG and DHBG and did not generate two of the major metabolites of BG formed by 3A4 wild type. In conclusion, we have determined that the reactive intermediate, oxygenated DHBG, covalently binds to Gln273 and thereby contributes to the mechanism-based inactivation of CYP3A4 by BG.
机译:先前的研究表明,葡萄柚汁的成分佛手柑(BG)是CYP3A4的一种基于机制的灭活剂,部分地促进了葡萄柚汁与药物的相互作用。尽管[14 C] BG与CYP3A4载脂蛋白的共价结合已通过SDS-聚丙烯酰胺凝胶电泳证明,但尚未报道修饰的氨基酸残基的身份和负责失活的BG的反应性中间物种。在本研究中,我们显示CYP3A4被BG灭活会导致形成修饰的载脂蛋白3A4和GSH缀合物,两者均显示388 Da的质量增加,这对应于6',7'-二羟基bergamottin(DHBG ),是BG的代谢产物,外加一个氧原子。为了鉴定加成残基,用胰蛋白酶消化BG灭活的3A4,然后通过液相色谱-串联质谱(MS / MS)分析消化物。在SEQUEST数据库搜索中使用了388 Da的质量位移,该序列显示序列272LQLMIDSQNSK 282的肽的质量增加了388 Da,并且对加成肽的MS / MS分析表明Gln273是残基修饰的。诱变研究表明,Gln273 to Val突变体对BG和DHBG的失活具有抗性,并且不产生3A4野生型形成的BG的两个主要代谢产物。综上所述,我们确定了反应性中间体氧化的DHBG与Gln273共价结合,从而促进了BG对CYP3A4的基于机制的失活。

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