Shaffer Christopher L, Langer Connie S
Department of Pharmacokinetics, Pharmacodynamics and Metabolism, Pfizer Global Research and Development, Groton/New London Laboratories, Pfizer Inc., Groton, CT 06340, USA.
J Pharm Biomed Anal. 2007 Mar 12;43(4):1195-205. doi: 10.1016/j.jpba.2006.11.022. Epub 2006 Dec 5.
The metabolism of 2-{[2-(3-fluoropyrid-2-yl)-1H-imidazol-1-yl]methyl}-1-propyl-5-cyano-1H-benzimidazole (1), a potent subtype-selective GABA(A) receptor partial agonist, was investigated in rat, dog and human liver microsomes. Due to its significant metabolic cleavage at C(8) observed in preliminary biotransformation studies with non-radiolabeled 1, both [(14)C]1 and [(3)H]1 were synthesized with respective radioisotopes placed on either side of C(8) to determine if all microsomal metabolites formed after C(8)N-dealkylation of 1 (or its core-intact metabolites) could be detected and quantified adequately. Both radiolabeled forms of 1, used separately in mono-radiolabel studies in cross-species microsomes and concomitantly in dual-radiolabel studies in rat microsomes, permitted the detection and quantification of all metabolites of 1, and a combination of radioactive and mass spectral data allowed structural elucidation of its Phase I metabolites. As expected, the sum of (14)C-only metabolites equaled that of (3)H-only metabolites in all incubations. In-line radiometric analysis worked extremely well (and was very reproducible) for quantifying either (14)C- or (3)H-compounds within separate incubations when using mono-radiolabeled 1. However, although the in-line radiodetector provided a comprehensive qualitative metabolic profile using dual-radiolabled 1, its inability to exclude completely (14)C- from (3)H-generated counts caused a degree of ambiguity pertaining to metabolite quantification. Thus, off-line liquid scintillation counting of collected dual-radiolabeled incubation LC-fractions was employed to quantify both (14)C- and (3)H-metabolites simultaneously, while in-line radiodetection was only used for qualitative analyses accompanying MS and MS/MS experiments. These studies demonstrated the analytical feasibility of using a dual-radiolabel approach for subsequent in vivo ADME studies with 1.
对强效亚型选择性GABA(A)受体部分激动剂2-{[2-(3-氟吡啶-2-基)-1H-咪唑-1-基]甲基}-1-丙基-5-氰基-1H-苯并咪唑(1)在大鼠、犬和人肝微粒体中的代谢情况进行了研究。由于在对非放射性标记的1进行的初步生物转化研究中观察到其在C(8)处有显著的代谢裂解,因此合成了[(14)C]1和[(3)H]1,将各自的放射性同位素置于C(8)的两侧,以确定在1经C(8)N-脱烷基化后形成的所有微粒体代谢物(或其核心完整代谢物)是否能够被充分检测和定量。1的两种放射性标记形式,分别用于跨物种微粒体的单放射性标记研究以及大鼠微粒体的双放射性标记研究,能够检测和定量1的所有代谢物,并且放射性数据和质谱数据相结合可以阐明其I相代谢物的结构。正如预期的那样,在所有孵育实验中,仅含(14)C的代谢物总和与仅含(3)H的代谢物总和相等。当使用单放射性标记的1时,在线放射性分析在单独孵育中对(14)C-或(3)H-化合物进行定量时效果极佳(且重复性很好)。然而,尽管在线放射性检测器使用双放射性标记的1提供了全面的定性代谢图谱,但它无法完全排除(3)H产生的计数中的(14)C,这在代谢物定量方面造成了一定程度的模糊性。因此,采用离线液体闪烁计数法对收集的双放射性标记孵育液相色谱馏分进行计数,以同时定量(14)C-和(3)H-代谢物,而在线放射性检测仅用于伴随质谱和串联质谱实验的定性分析。这些研究证明了使用双放射性标记方法对1进行后续体内药物代谢动力学和药物处置研究的分析可行性。
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