Effect of Ligands and Transducers on the Neurotensin Receptor 1 Conformational Ensemble

Austin D. Dixon; Asuka Inoue; Scott A. Robson; Kelly J. Culhane; Jonathan C. Trinidad; Sivaraj Sivaramakrishnan; Fabian Bumbak; Joshua J. Ziarek

doi:10.1021/jacs.2c00828

Effect of Ligands and Transducers on the Neurotensin Receptor 1 Conformational Ensemble

Austin D. Dixon, Asuka Inoue, Scott A. Robson, Kelly J. Culhane, Jonathan C. Trinidad, Sivaraj Sivaramakrishnan, Fabian Bumbak, Joshua J. Ziarek^*

^*Corresponding author for this work

Pharmacology

Research output: Contribution to journal › Article › peer-review

12 Scopus citations

Abstract

Using a discrete, intracellular ¹⁹F nuclear magnetic resonance (NMR) probe on transmembrane helix 6 of the neurotensin receptor 1 (NTS1), we aim to understand how ligands and transducers modulate the receptor's structural ensemble in a solution. For apo NTS1, ¹⁹F NMR spectra reveal an ensemble of at least three conformational substates (one inactive and two active-like) in equilibrium that exchange on the millisecond to second timescale. Dynamic NMR experiments reveal that these substates follow a linear three-site exchange process that is both thermodynamically and kinetically remodeled by orthosteric ligands. As previously observed in other G protein-coupled receptors (GPCRs), the full agonist is insufficient to completely stabilize the active-like state. The inactive substate is abolished upon coupling to β-arrestin-1 (βArr1) or the C-terminal helix of Gα_q, which comprises ≳60% of the GPCR/G protein interface surface area. Whereas βArr1 exclusively selects for pre-existing active-like substates, the Gα_qpeptide induces a new substate. Both transducer molecules promote substantial line broadening of active-like states, suggesting contributions from additional microsecond to millisecond exchange processes. Together, our study suggests that (i) the NTS1 allosteric activation mechanism may be alternatively dominated by induced fit or conformational selection depending on the coupled transducer, and (ii) the available static structures do not represent the entire conformational ensemble observed in a solution.

Original language	English (US)
Pages (from-to)	10241-10250
Number of pages	10
Journal	Journal of the American Chemical Society
Volume	144
Issue number	23
DOIs	https://doi.org/10.1021/jacs.2c00828
State	Published - Jun 15 2022

Funding

We are grateful to Prof. Gregor Hagelueken at the University of Bonn for assistance with modeling using mtsslWizard software, Dr. Hongwei Wu at Indiana University for NMR instrument assistance, Dr. Ratan Rai at Indiana University School of Medicine for NMR instrument assistance, Kouki Kawakami at Tohoku University for technical assistance, Kayo Sato, Shigeko Nakano, and Ayumi Inoue at Tohoku University for their assistance in plasmid preparation and cell-based GPCR assays, Prof. Ashish Manglik at the University of California for providing the \u03B2Arr1 construct used in this study, and Prof. Daniel Scott at the Florey Institute for providing the enNTS1 plasmid used in this study. The 14.1 T spectrometers used in this study were generously supported by the Indiana University Fund. The project was funded by the following: Indiana Precision Health Initiative (JJZ); NIH grants R35GM126940 (SS), K12GM119955 (KJC), R00GM115814 (JJZ), and R35GM143054 (JJZ); KAKENHI 21H04791 (AI), 21H051130 (AI), and JPJSBP120213501 (AI) from the Japan Society for the Promotion of Science (JSPS); LEAP JP20gm0010004 (AI) and BINDS JP20am0101095 (AI) from the Japan Agency for Medical Research and Development (AMED); FOREST Program JPMJFR215T (AI); JST Moonshot Research and Development Program JPMJMS2023 (AI) from the Japan Science and Technology Agency (JST); Daiichi Sankyo Foundation of Life Science (AI); Takeda Science Foundation (AI); Ono Medical Research Foundation (AI); and Uehara Memorial Foundation (AI).

ASJC Scopus subject areas

Catalysis
General Chemistry
Biochemistry
Colloid and Surface Chemistry

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abstract = "Using a discrete, intracellular 19F nuclear magnetic resonance (NMR) probe on transmembrane helix 6 of the neurotensin receptor 1 (NTS1), we aim to understand how ligands and transducers modulate the receptor's structural ensemble in a solution. For apo NTS1, 19F NMR spectra reveal an ensemble of at least three conformational substates (one inactive and two active-like) in equilibrium that exchange on the millisecond to second timescale. Dynamic NMR experiments reveal that these substates follow a linear three-site exchange process that is both thermodynamically and kinetically remodeled by orthosteric ligands. As previously observed in other G protein-coupled receptors (GPCRs), the full agonist is insufficient to completely stabilize the active-like state. The inactive substate is abolished upon coupling to β-arrestin-1 (βArr1) or the C-terminal helix of Gαq, which comprises ≳60% of the GPCR/G protein interface surface area. Whereas βArr1 exclusively selects for pre-existing active-like substates, the Gαqpeptide induces a new substate. Both transducer molecules promote substantial line broadening of active-like states, suggesting contributions from additional microsecond to millisecond exchange processes. Together, our study suggests that (i) the NTS1 allosteric activation mechanism may be alternatively dominated by induced fit or conformational selection depending on the coupled transducer, and (ii) the available static structures do not represent the entire conformational ensemble observed in a solution.",

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Effect of Ligands and Transducers on the Neurotensin Receptor 1 Conformational Ensemble

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