AI Article Synopsis

  • A new method for evolving integral membrane proteins in E. coli is presented, resulting in significantly enhanced functional expression of a mammalian G protein-coupled receptor while maintaining its original biochemical properties.
  • The improved variant demonstrates increased expression in other organisms like Pichia pastoris and HEK293T cells, and shows better stability during purification, suggesting effective evolutionary selection.
  • Additionally, a specific amino acid change was identified that eliminates antagonist binding but keeps agonist binding intact, which can help resolve challenges in structural studies by providing stable protein variants.

Article Abstract

We outline a powerful method for the directed evolution of integral membrane proteins in the inner membrane of Escherichia coli. For a mammalian G protein-coupled receptor, we arrived at a sequence with an order-of-magnitude increase in functional expression that still retains the biochemical properties of wild type. This mutant also shows enhanced heterologous expression in eukaryotes (12-fold in Pichia pastoris and 3-fold in HEK293T cells) and greater stability when solubilized and purified, indicating that the biophysical properties of the protein had been under the pressure of selection. These improvements arise from multiple small contributions, which would be difficult to assemble by rational design. In a second screen, we rapidly pinpointed a single amino acid substitution in wild type that abolishes antagonist binding while retaining agonist-binding affinity. These approaches may alleviate existing bottlenecks in structural studies of these targets by providing sufficient quantities of stable variants in defined conformational states.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC2567449PMC
http://dx.doi.org/10.1073/pnas.0803103105DOI Listing

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