A novel fusion tool to enable G protein-coupled receptor structure determination

Shah, N.R.; Oosterlaken, M.; Bisson, C.; Bertinelli, M.; Churchill-Angus, A.M.; Hutchin, A.; Kopec, J.; Kotov, V.; McFarlane, C.R.; Griss Pascualli, E.; Pavic, A.; Zebisch, M.; Fiez-Vandal, C.; Fabini, E.; Duclos, S.

doi:10.1107/S2059798326003785

Acta Crystallographica Section D
Acta Crystallographica
Section D STRUCTURAL BIOLOGY

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Figure 1
Assessment of A_2AR with different fusion tags inserted into ICL3 from small-scale affinity pull-down experiments. (a) SDS–PAGE and (b) Western blot analysis of solubilized (S) and affinity pull-down elution (E) samples of A_2AR fusion constructs (numbers correspond to the fusion constructs listed in Supplementary Table S1). M, molecular-weight standards in kDa; C, Western blot anti-FLAG control; NI, non-infected cell control; F, A_2AR-bRIL fusion control. (c) fSEC analysis of A_2AR with two β-lactamase fusions (Fusion 5, β-lactamase_Bli, and Fusion 6, β-lactamase_Ban) inserted into ICL3, with A_2AR-bRIL fusion control [F (bRIL)] and molecular-weight standards (Std), at 670, 158, 44, 17 and 1.35 kDa. fSEC readings were collected with an excitation wavelength of 488 nm and an emission wavelength of 512 nm; the molecular-weight standards readings (Std) are from the A₂₈₀ signal.

STRUCTURAL
BIOLOGY

ISSN: 2059-7983

Volume 82| Part 6| June 2026| Pages 655-663

https://doi.org/10.1107/S2059798326003785

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