A High-Throughput Splicing Assay Identifies New Classes of Inhibitors of Human and Yeast Spliceosomes

Author:

Effenberger Kerstin A.12,Perriman Rhonda J.12,Bray Walter M.3,Lokey R. Scott3,Ares Manuel12,Jurica Melissa S.12

Affiliation:

1. Department of Molecular Cell and Developmental Biology, University of California Santa Cruz, Santa Cruz, CA, USA

2. Center for Molecular Biology of RNA, University of California Santa Cruz, Santa Cruz, CA, USA

3. Department of Chemistry and Biochemistry, University of California Santa Cruz, Santa Cruz, CA, USA

Abstract

The spliceosome is the macromolecular machine responsible for pre-mRNA splicing, an essential step in eukaryotic gene expression. During splicing, myriad subunits join and leave the spliceosome as it works on the pre-mRNA substrate. Strikingly, there are very few small molecules known to interact with the spliceosome. Splicing inhibitors are needed to capture transient spliceosome conformations and probe important functional components. Such compounds may also have chemotherapeutic applications, as links between splicing and cancer are increasingly uncovered. To identify new splicing inhibitors, we developed a high-throughput assay for in vitro splicing using a reverse transcription followed by quantitative PCR readout. In a pilot screen of 3080 compounds, we identified three small molecules that inhibit splicing in HeLa extract by interfering with different stages of human spliceosome assembly. Two of the compounds similarly affect spliceosomes in yeast extracts, suggesting selective targeting of conserved components. By examining related molecules, we identified chemical features required for the activity of two of the splicing inhibitors. In addition to verifying our assay procedure and paving the way to larger screens, these studies establish new compounds as chemical probes for investigating the splicing machinery.

Publisher

Elsevier BV

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