Engineered SUMO/protease system identifies Pdr6 as a bidirectional nuclear 
transport receptor.

Vera Rodriguez, A.; Frey, S.; Görlich, D.

doi:10.1083/jcb.201812091

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Engineered SUMO/protease system identifies Pdr6 as a bidirectional nuclear transport receptor.

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Vera Rodriguez, A.
Department of Cellular Logistics, MPI for biophysical chemistry, Max Planck Society;

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Frey, S.
Department of Cellular Logistics, MPI for biophysical chemistry, Max Planck Society;

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Görlich, D.
Department of Cellular Logistics, MPI for biophysical chemistry, Max Planck Society;

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Citation

Vera Rodriguez, A., Frey, S., & Görlich, D. (2019). Engineered SUMO/protease system identifies Pdr6 as a bidirectional nuclear transport receptor. The Journal of Cell Biology, (in press). doi:10.1083/jcb.201812091.

Cite as: https://hdl.handle.net/21.11116/0000-0003-7F59-C

Abstract

Cleavage of affinity tags by specific proteases can be exploited for highly selective affinity chromatography. The SUMO/SENP1 system is the most efficient for such application but fails in eukaryotic expression because it cross-reacts with endogenous proteases. Using a novel selection system, we have evolved the SUMOEu/SENP1Eu pair to orthogonality with the yeast and animal enzymes. SUMOEu fusions therefore remain stable in eukaryotic cells. Likewise, overexpressing a SENP1Eu protease is nontoxic in yeast. We have used the SUMOEu system in an affinity-capture-proteolytic-release approach to identify interactors of the yeast importin Pdr6/Kap122. This revealed not only further nuclear import substrates such as Ubc9, but also Pil1, Lsp1, eIF5A, and eEF2 as RanGTP-dependent binders and thus as export cargoes. We confirmed that Pdr6 functions as an exportin in vivo and depletes eIF5A and eEF2 from cell nuclei. Thus, Pdr6 is a bidirectional nuclear transport receptor (i.e., a biportin) that shuttles distinct sets of cargoes in opposite directions.