Screening of HIV-1 Protease Using a Combination of an Ultra-High-Throughput Fluorescent-Based Assay and RapidFire Mass Spectrometry

Author:

Meng Juncai1,Lai Ming-Tain2,Munshi Vandna2,Grobler Jay2,McCauley John3,Zuck Paul1,Johnson Eric N.14,Uebele Victor N.1,Hermes Jeffrey D.1,Adam Gregory C.1

Affiliation:

1. Screening and Protein Sciences, Merck Research Labs, North Wales, PA, USA

2. Department of Infectious Disease, Merck Research Labs, West Point, PA, USA

3. Medicinal Chemistry, Merck Research Labs, West Point, PA, USA

4. Wuxi Apptech

Abstract

HIV-1 protease (PR) represents one of the primary targets for developing antiviral agents for the treatment of HIV-infected patients. To identify novel PR inhibitors, a label-free, high-throughput mass spectrometry (HTMS) assay was developed using the RapidFire platform and applied as an orthogonal assay to confirm hits identified in a fluorescence resonance energy transfer (FRET)–based primary screen of > 1 million compounds. For substrate selection, a panel of peptide substrates derived from natural processing sites for PR was evaluated on the RapidFire platform. As a result, KVSLNFPIL, a new substrate measured to have a ~ 20- and 60-fold improvement in kcat/ Km over the frequently used sequences SQNYPIVQ and SQNYPIV, respectively, was identified for the HTMS screen. About 17% of hits from the FRET-based primary screen were confirmed in the HTMS confirmatory assay including all 304 known PR inhibitors in the set, demonstrating that the HTMS assay is effective at triaging false-positives while capturing true hits. Hence, with a sampling rate of ~7 s per well, the RapidFire HTMS assay enables the high-throughput evaluation of peptide substrates and functions as an efficient tool for hits triage in the discovery of novel PR inhibitors.

Publisher

Elsevier BV

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