Validation of a Fluorescent Imaging Plate Reader Membrane Potential Assay for High-Throughput Screening of Glycine Transporter Modulators

Author:

Benjamin Elfrida R.1,Skelton Joanne2,Hanway Denise,Olanrewaju Shakira,Pruthi Farhana,Ilyin Victor I.1,Lavery Daniel3,Victory Sam F.4,Valenzano Kenneth J.1

Affiliation:

1. Purdue Pharma Discovery Research, Cranbury, New Jersey

2. Veridex, Warren, New Jersey

3. Chromocell Corporation, North Brunswick, New Jersey

4. TransTech Pharma, High Point, North Carolina

Abstract

A fluorescent imaging plate reader (FLIPR) membrane potential (Vm) assay was evaluated for pharmacological characterization and high-throughput screening (HTS) of rat glycine transporter type 2 (rGlyT2) in a stable rGlyT2-HEK cell line. Data show that glycine activation of rGlyT2consistently results in a concentration-dependent Vmresponse on the FLIPR that is blocked by the potent and selective GlyT2antagonist 4-benzyloxy-3,5-dimethoxy-N-[1-dimethylamino-cyclopentyl)methyl]-benz-amide (Org-25543). Agonist and antagonist pharmacologies match those reported using conventional [3H]glycine uptake assays and electrophysiology. The glycine response is dependent on buffer ionic composition consistent with GlyT2physiology. Assay signal-to-background and coefficient of variation meets sufficient statistical criteria to conduct HTS. The results of a screen of the chemical inventory demonstrate that the assay is able to successfully identify and confirm GlyT2inhibitors. The advantages of this assay are its homogeneity, compatibility with both 96- and 384-well formats, and lack of radioactivity usage. Thus, the authors conclude that a fluorescence-based Vmassay on FLIPR is a viable approach for identification and pharmacological profiling of small molecule modulators of the electrogenic transporter rGlyT2.

Publisher

Elsevier BV

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