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Refolding of G protein alpha subunits from inclusion bodies expressed in Escherichia coli
Authors:McCusker Emily  Robinson Anne Skaja
Affiliation:aDepartment of Chemistry and Biochemistry, University of Delaware, Newark, DE 19716, United States;bDepartment of Chemical Engineering, University of Delaware, 150 Academy Street, Newark, DE 19716, United States
Abstract:Heterotrimeric G proteins relay signals from G protein-coupled receptors (GPCRs) to the interior of the cell. The signaling cascades induced by G protein activation control a wide range of cellular processes. The α subunit is believed to determine which G protein couples to each GPCR, and is the primary determinant of the type of signal transmitted. Several members of the Gα family have been expressed in active form in Escherichia coli. However, production levels of these proteins are limited: in most cases only not, vert, similar10% of total Gα protein expressed is active; the rest accumulates in inclusion bodies. Although G has been readily expressed in soluble form (to 10 mg/L), other α subunits are minimally soluble, and many are exclusively expressed to inclusion bodies. Previous efforts to solubilize and refold Gα from inclusion bodies have not been successful. Here we did a thorough study of the characteristics of Gα subunits (human Giα(1), human Gsα(short), human G11α and human Gtα(cone)), solubilized and purified from inclusion bodies. We find that we can obtain soluble protein both by on-column and rapid-dilution techniques. Comparison to native, soluble G expressed from E. coli showed that although the refolded Gα subunits were soluble and retained partial α-helicity characteristic of the native, folded Gα subunit, they did not bind GDP or GTP as effectively as native protein. We conclude that the refolded G protein has a native-like secondary structure, but is predominately in a molten globular state.
Keywords:GTP-binding proteins   G-protein coupled receptor   Aluminium fluoride assay   Transduction   BODYIPY-FL-GTP
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