A dual-light reporter system to determine the efficiency of protein-protein interactions in mammalian cells

doi:10.1093/nar/gni066

Nucleic Acids Research 2005 33(7):e66; doi:10.1093/nar/gni066

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Published online 11 April 2005

© The Author 2005. Published by Oxford University Press. All rights reserved
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A dual-light reporter system to determine the efficiency of protein–protein interactions in mammalian cells

M. T. Nasim^* and R. C. Trembath

Department of Genetics, University of Leicester Leicester LE1 7RH, UK

^*To whom correspondence should be addressed. Tel: +44 116 223 1262; Fax: +44 116 223 1779; Email: mtn4{at}le.ac.uk

Received January 11, 2005. Revised March 24, 2005. Accepted March 24, 2005.

Methods for determining protein–protein interactions inmammalian cells typically rely on single reporter functionsand are susceptible to variations between samples particularlyin regard to levels of transcription, processing and translation.A method has been developed for determining protein–proteininteractions in mammalian cells, which bypasses these variablesconfounding single reporter assays. The approach utilizes twounits of gene expression linked to reporter functions that areinterposed by a deactivation–activation unit in such away that the downstream expression unit is switched off. Henceupstream expression occurs regardless of protein–proteininteraction, leading to the production of the upstream reporter.In the event of protein–protein interactions, the downstreamexpression unit is switched on leading to dual reporter readouts. Thus, the ratio of the two reporter activities providesa measure to determine the efficiency of protein–proteininteractions. To access the system we screened a mutant of BMPR2where the interaction between BMPR-II and LIMK is abrogated.BMPR-II is a type II receptor of the TGFß superfamilyand plays a key role in the pathogenesis of familial pulmonaryarterial hypertension. This system has potential for high-throughputscreening of libraries (peptide, chemical, cDNA, etc.) to isolateagents that are capable of interfering with highly selectiveprotein–protein interaction.

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