Developing inhibitors of the guanosine triphosphate hydrolysis accelerating activity of Regulator of G protein Signaling-14[Figure presented]

Percy S. Agogo-Mawuli; Isra Sadiya; Tigran M. Abramyan; Dustin E. Bosch; Kyle A. Emmitte; Luis M. Colón-Pérez; Mickey Kosloff; David P. Siderovski

doi:10.1016/j.jbc.2025.110611

Developing inhibitors of the guanosine triphosphate hydrolysis accelerating activity of Regulator of G protein Signaling-14[Figure presented]

Percy S. Agogo-Mawuli
, Isra Sadiya
, Tigran M. Abramyan
, Dustin E. Bosch
, Kyle A. Emmitte
, Luis M. Colón-Pérez
, Mickey Kosloff
, David P. Siderovski

Department of Human Biology

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

Abstract

Regulator of G protein Signaling-14 (RGS14), an intracellular inactivator of G protein-coupled receptor (GPCR) signaling, is considered an undruggable protein, given its shallow and relatively featureless protein-protein interaction interface combined with a distal allosteric site prone to nonspecific inhibition by thiol-reactive compounds. Here, we identify and validate a tractable chemotype that selectively and non-covalently inhibits RGS14 GTPase-accelerating protein (GAP) activity. Combining structure-guided virtual screening, ligand docking across multiple receptor conformers, and enrichment validation, we progressed from a first-generation active, Z90276197, to over 40 second-generation analogs with improved potency. These inhibitors are predicted to engage the solvent-exposed “canyon” in the RGS14 RGS-box that interacts with the Gα switch I region. Binding pose predictions underscored the importance of non-polar interactions and shape complementarity over polar interactions in engaging this Gα-binding canyon and revealed an “ambidextrous” pattern of R1-and R2-group orientations. GAP inhibition was confirmed in fluorescence-based and gold-standard radioactive GTP hydrolysis assays. Two second-generation analogs, Z55660043 and Z55627844, inhibited RGS14 GAP activity in both assays and without measurable cytotoxicity. Deep learning-based scoring of predicted docking poses further supported observed affinity gains from R3-group additions. One analog demonstrated favorable in vivo pharmacokinetics and CNS penetration. Collectively, our findings establish tractable, non-covalent, small molecule inhibition of a G protein regulatory interface and illustrate how machine learning-enhanced docking can guide ligand optimization for shallow protein surfaces. This work opens the door to future development of RGS14 inhibitors as potential therapeutics for central nervous system and metabolic disorders.

Original language	English
Article number	110611
Journal	Journal of Biological Chemistry
Volume	301
Issue number	10
Early online date	21 Aug 2025
DOIs	https://doi.org/10.1016/j.jbc.2025.110611
State	Published - Oct 2025

Bibliographical note

Publisher Copyright:
© 2025 The Authors

Keywords

CNS-penetrant compounds
G protein-coupled receptor signaling
GAP activity inhibition
RGS14
deep learning docking
protein-protein interaction
regulator of G protein signaling
small-molecule inhibitor
structure-guided drug design
triazolothiadiazine
virtual screening

ASJC Scopus subject areas

Biochemistry
Molecular Biology
Cell Biology

UN SDGs

This output contributes to the following UN Sustainable Development Goals (SDGs)

Access to Document

10.1016/j.jbc.2025.110611

Cite this

Agogo-Mawuli, P. S., Sadiya, I., Abramyan, T. M., Bosch, D. E., Emmitte, K. A., Colón-Pérez, L. M., Kosloff, M., & Siderovski, D. P. (2025). Developing inhibitors of the guanosine triphosphate hydrolysis accelerating activity of Regulator of G protein Signaling-14[Figure presented]. Journal of Biological Chemistry, 301(10), Article 110611. https://doi.org/10.1016/j.jbc.2025.110611

@article{bc110e7a3db542ff8bacaa232206daaa,

title = "Developing inhibitors of the guanosine triphosphate hydrolysis accelerating activity of Regulator of G protein Signaling-14[Figure presented]",

abstract = "Regulator of G protein Signaling-14 (RGS14), an intracellular inactivator of G protein-coupled receptor (GPCR) signaling, is considered an undruggable protein, given its shallow and relatively featureless protein-protein interaction interface combined with a distal allosteric site prone to nonspecific inhibition by thiol-reactive compounds. Here, we identify and validate a tractable chemotype that selectively and non-covalently inhibits RGS14 GTPase-accelerating protein (GAP) activity. Combining structure-guided virtual screening, ligand docking across multiple receptor conformers, and enrichment validation, we progressed from a first-generation active, Z90276197, to over 40 second-generation analogs with improved potency. These inhibitors are predicted to engage the solvent-exposed “canyon” in the RGS14 RGS-box that interacts with the Gα switch I region. Binding pose predictions underscored the importance of non-polar interactions and shape complementarity over polar interactions in engaging this Gα-binding canyon and revealed an “ambidextrous” pattern of R1-and R2-group orientations. GAP inhibition was confirmed in fluorescence-based and gold-standard radioactive GTP hydrolysis assays. Two second-generation analogs, Z55660043 and Z55627844, inhibited RGS14 GAP activity in both assays and without measurable cytotoxicity. Deep learning-based scoring of predicted docking poses further supported observed affinity gains from R3-group additions. One analog demonstrated favorable in vivo pharmacokinetics and CNS penetration. Collectively, our findings establish tractable, non-covalent, small molecule inhibition of a G protein regulatory interface and illustrate how machine learning-enhanced docking can guide ligand optimization for shallow protein surfaces. This work opens the door to future development of RGS14 inhibitors as potential therapeutics for central nervous system and metabolic disorders.",

keywords = "CNS-penetrant compounds, G protein-coupled receptor signaling, GAP activity inhibition, RGS14, deep learning docking, protein-protein interaction, regulator of G protein signaling, small-molecule inhibitor, structure-guided drug design, triazolothiadiazine, virtual screening",

author = "Agogo-Mawuli, \{Percy S.\} and Isra Sadiya and Abramyan, \{Tigran M.\} and Bosch, \{Dustin E.\} and Emmitte, \{Kyle A.\} and Col{\'o}n-P{\'e}rez, \{Luis M.\} and Mickey Kosloff and Siderovski, \{David P.\}",

note = "Publisher Copyright: {\textcopyright} 2025 The Authors",

year = "2025",

month = oct,

doi = "10.1016/j.jbc.2025.110611",

language = "English",

volume = "301",

journal = "Journal of Biological Chemistry",

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T1 - Developing inhibitors of the guanosine triphosphate hydrolysis accelerating activity of Regulator of G protein Signaling-14[Figure presented]

AU - Agogo-Mawuli, Percy S.

AU - Sadiya, Isra

AU - Abramyan, Tigran M.

AU - Bosch, Dustin E.

AU - Emmitte, Kyle A.

AU - Colón-Pérez, Luis M.

AU - Kosloff, Mickey

AU - Siderovski, David P.

PY - 2025/10

Y1 - 2025/10

N2 - Regulator of G protein Signaling-14 (RGS14), an intracellular inactivator of G protein-coupled receptor (GPCR) signaling, is considered an undruggable protein, given its shallow and relatively featureless protein-protein interaction interface combined with a distal allosteric site prone to nonspecific inhibition by thiol-reactive compounds. Here, we identify and validate a tractable chemotype that selectively and non-covalently inhibits RGS14 GTPase-accelerating protein (GAP) activity. Combining structure-guided virtual screening, ligand docking across multiple receptor conformers, and enrichment validation, we progressed from a first-generation active, Z90276197, to over 40 second-generation analogs with improved potency. These inhibitors are predicted to engage the solvent-exposed “canyon” in the RGS14 RGS-box that interacts with the Gα switch I region. Binding pose predictions underscored the importance of non-polar interactions and shape complementarity over polar interactions in engaging this Gα-binding canyon and revealed an “ambidextrous” pattern of R1-and R2-group orientations. GAP inhibition was confirmed in fluorescence-based and gold-standard radioactive GTP hydrolysis assays. Two second-generation analogs, Z55660043 and Z55627844, inhibited RGS14 GAP activity in both assays and without measurable cytotoxicity. Deep learning-based scoring of predicted docking poses further supported observed affinity gains from R3-group additions. One analog demonstrated favorable in vivo pharmacokinetics and CNS penetration. Collectively, our findings establish tractable, non-covalent, small molecule inhibition of a G protein regulatory interface and illustrate how machine learning-enhanced docking can guide ligand optimization for shallow protein surfaces. This work opens the door to future development of RGS14 inhibitors as potential therapeutics for central nervous system and metabolic disorders.

AB - Regulator of G protein Signaling-14 (RGS14), an intracellular inactivator of G protein-coupled receptor (GPCR) signaling, is considered an undruggable protein, given its shallow and relatively featureless protein-protein interaction interface combined with a distal allosteric site prone to nonspecific inhibition by thiol-reactive compounds. Here, we identify and validate a tractable chemotype that selectively and non-covalently inhibits RGS14 GTPase-accelerating protein (GAP) activity. Combining structure-guided virtual screening, ligand docking across multiple receptor conformers, and enrichment validation, we progressed from a first-generation active, Z90276197, to over 40 second-generation analogs with improved potency. These inhibitors are predicted to engage the solvent-exposed “canyon” in the RGS14 RGS-box that interacts with the Gα switch I region. Binding pose predictions underscored the importance of non-polar interactions and shape complementarity over polar interactions in engaging this Gα-binding canyon and revealed an “ambidextrous” pattern of R1-and R2-group orientations. GAP inhibition was confirmed in fluorescence-based and gold-standard radioactive GTP hydrolysis assays. Two second-generation analogs, Z55660043 and Z55627844, inhibited RGS14 GAP activity in both assays and without measurable cytotoxicity. Deep learning-based scoring of predicted docking poses further supported observed affinity gains from R3-group additions. One analog demonstrated favorable in vivo pharmacokinetics and CNS penetration. Collectively, our findings establish tractable, non-covalent, small molecule inhibition of a G protein regulatory interface and illustrate how machine learning-enhanced docking can guide ligand optimization for shallow protein surfaces. This work opens the door to future development of RGS14 inhibitors as potential therapeutics for central nervous system and metabolic disorders.

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KW - protein-protein interaction

KW - regulator of G protein signaling

KW - small-molecule inhibitor

KW - structure-guided drug design

KW - triazolothiadiazine

KW - virtual screening

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DO - 10.1016/j.jbc.2025.110611

M3 - Article

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AN - SCOPUS:105016308172

SN - 0021-9258

VL - 301

JO - Journal of Biological Chemistry

JF - Journal of Biological Chemistry

IS - 10

M1 - 110611

ER -

Developing inhibitors of the guanosine triphosphate hydrolysis accelerating activity of Regulator of G protein Signaling-14[Figure presented]

Abstract

Bibliographical note

Keywords

ASJC Scopus subject areas

UN SDGs

Access to Document

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