Stable isotope synthesis of glycine transporter 1 inhibitor Iclepertin (BI 425809) and its major metabolites

Author:

Latli Bachir1ORCID,Hrapchak Matt J.1,Chevliakov Maxim1,Samankumara Lalith P.1,Frutos Rogelio P.1,Lee Heewon1

Affiliation:

1. The Radiosynthesis Laboratory, Chemical Development Boehringer Ingelheim Pharmaceuticals, Inc. Ridgefield Connecticut USA

Abstract

Stable isotope labeled Iclepertin (BI 425809, 1) and its major metabolites are needed as internal standards in bioanalytical studies. BI 425809 consists of two main building blocks, 5‐methylsulfonyl‐2‐[(1R)‐2,2,2‐trifluoro‐1‐methyl‐ethoxy]benzoic acid (2) and 3‐[(1R,5R)‐3‐azabicyclo[3.1.0]hexan‐5‐yl]‐5‐(trifluoromethyl)isoxazole (3) linked to each other via an amide bond. We used fluoro[13C6]benzene as the starting material in the preparation of [13C6]‐2. This intermediate was then employed to access carbon 13 labeled Iclepertin ([13C6]‐1) and other metabolites. The major metabolite BI 761036 (6), which resulted from cytochrome P450 oxidation and amide hydrolysis of BI 425809, was prepared labeled with carbon 13 and nitrogen 15 via two synthetic routes. In the first route, diethyl [13C3]malonate, [13C]methyl iodide, and hydroxyl[15N]amine were used to provide [13C4,15N]‐BI 761036 ([13C4,15N]‐6a) in 13 steps in 6% overall yield, whereas in the second route, [13C3]propargyl alcohol, potassium [13C]cyanide, and [15N]ammonia were used to furnish [13C4,15N]‐BI 761036 ([13C4,15N]‐6b) in 11 steps in 1% overall yield. The detailed stable isotope synthesis of 1 and its major metabolites is described.

Publisher

Wiley

Subject

Organic Chemistry,Spectroscopy,Drug Discovery,Radiology, Nuclear Medicine and imaging,Biochemistry,Analytical Chemistry

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