Three Mutations Convert the Selectivity of a Protein Sensor from Nicotinic Agonists to S-methadone for Use in Cells, Organelles, and Biofluids

Author:

Muthusamy Anand K.ORCID,Kim Charlene H.ORCID,Virgil Scott C.ORCID,Knox Hailey J.ORCID,Marvin Jonathan S.ORCID,Nichols Aaron L.ORCID,Cohen Bruce N.ORCID,Dougherty Dennis A.ORCID,Looger Loren L.ORCID,Lester Henry A.ORCID

Abstract

ABSTRACTWe report a reagentless, intensity-based S-methadone fluorescent sensor, iS-methadoneSnFR, consisting of a circularly permuted GFP inserted within the sequence of a mutated bacterial periplasmic binding protein (PBP). We evolved a previously reported nicotine-binding PBP to become a selective S-methadone-binding sensor, via three mutations in the PBP’s second shell and hinge regions. iS-methadoneSnFR displays the necessary sensitivity, kinetics, and selectivity – notably enantioselectivity against R-methadone – for biological applications. Robust iS-methadoneSnFR responses in human sweat and saliva and mouse serum enable diagnostic uses. Expression and imaging in mammalian cells demonstrate that S-methadone enters at least two organelles and undergoes acid trapping in the Golgi apparatus, where opioid receptors can signal. This work shows a straightforward strategy in adapting existing PBPs to serve real-time applications ranging from subcellular to personal pharmacokinetics.

Publisher

Cold Spring Harbor Laboratory

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