Fluorescent ligands: Bringing light to emerging GPCR paradigms

Soave, Mark; Briddon, Stephen J.; Hill, Stephen J.; Stoddart, Leigh A.

doi:10.1111/bph.14953

Cited by 66 publications

(70 citation statements)

References 114 publications

(170 reference statements)

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“…fully used to determine the real-time kinetics of ligand binding to GPCRs [23][24][25] . Here, we investigated the ability of the selective A 3 R antagonists MRS 1220, K17 or K18 to inhibit specific binding of the fluorescent A 3 R antagonist CA200645 to Nluc-A 3 R 26,27 .…”

Section: Kinetics Of a 3 R Antagonists Determined Through Bret Nanobmentioning

confidence: 99%

Pharmacological characterisation of novel adenosine A3 receptor antagonists

Barkan

Lagarias

Stampelou

et al. 2020

Sci Rep

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The adenosine A3 receptor (A3R) belongs to a family of four adenosine receptor (AR) subtypes which all play distinct roles throughout the body. A3R antagonists have been described as potential treatments for numerous diseases including asthma. Given the similarity between (adenosine receptors) orthosteric binding sites, obtaining highly selective antagonists is a challenging but critical task. Here we screen 39 potential A3R, antagonists using agonist-induced inhibition of cAMP. Positive hits were assessed for AR subtype selectivity through cAMP accumulation assays. The antagonist affinity was determined using Schild analysis (pA2 values) and fluorescent ligand binding. Structure–activity relationship investigations revealed that loss of the 3-(dichlorophenyl)-isoxazolyl moiety or the aromatic nitrogen heterocycle with nitrogen at α-position to the carbon of carboximidamide group significantly attenuated K18 antagonistic potency. Mutagenic studies supported by molecular dynamic simulations combined with Molecular Mechanics—Poisson Boltzmann Surface Area calculations identified the residues important for binding in the A3R orthosteric site. We demonstrate that K18, which contains a 3-(dichlorophenyl)-isoxazole group connected through carbonyloxycarboximidamide fragment with a 1,3-thiazole ring, is a specific A3R (< 1 µM) competitive antagonist. Finally, we introduce a model that enables estimates of the equilibrium binding affinity for rapidly disassociating compounds from real-time fluorescent ligand-binding studies. These results demonstrate the pharmacological characterisation of a selective competitive A3R antagonist and the description of its orthosteric binding mode. Our findings may provide new insights for drug discovery.

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Section: Kinetics Of a 3 R Antagonists Determined Through Bret Nanobmentioning

confidence: 99%

Pharmacological characterisation of novel adenosine A3 receptor antagonists

Barkan

Lagarias

Stampelou

et al. 2020

Sci Rep

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“…In contrast, NanoBRET binding assays 11 make use of a small and bright luciferase variant (Nluc) 19 , that is fused to the extracellular part of the investigated GPCR. In both cases, binding of the fluorescent ligand is detected based on RET between the receptor as light emitting donor and the fluorescent ligand serving as the acceptor 10 . Both RET-assays have been proven extremely useful for the characterization of ligand binding at GPCRs, especially if high affinity radioligands are not available or if binding kinetics 10 , 23 , 24 are central to the investigated research question.…”

Section: Discussionmentioning

confidence: 99%

“…In both cases, binding of the fluorescent ligand is detected based on RET between the receptor as light emitting donor and the fluorescent ligand serving as the acceptor 10 . Both RET-assays have been proven extremely useful for the characterization of ligand binding at GPCRs, especially if high affinity radioligands are not available or if binding kinetics 10 , 23 , 24 are central to the investigated research question. Typical saturation hyperbolas were obtained for all three ligands when we performed NanoBRET assays with living HEK293T cells expressing an Nluc-D 3 R fusion protein.…”

Section: Discussionmentioning

confidence: 99%

“…Over recent years, fluorescence-based technologies have emerged as exciting alternative to study ligand affinity 10 – 12 . Similar to radioactive probes, fluorescent molecules can be detected at very low concentration with high specificity.…”

Section: Introductionmentioning

confidence: 99%

“…Although the synthesis of small-molecule fluorescent ligands is far from trivial, it requires lower level regulatory and safety precautions compared to the preparation of radioligands. Moreover, several fluorescence-based technologies like resonance energy transfer (RET) and fluorescence anisotropy (also known as fluorescence polarization) do not require separation of unbound ligands and assays can thus be run in a homogenous, fast “mix-and-measure” setup 10 , 13 . In combination with sophisticated techniques like total internal reflection fluorescence (TIRF) microscopy, fluorescent ligands allow to detect and track GPCRs with single molecule resolution 14 – 16 .…”

Section: Introductionmentioning

confidence: 99%

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Fluorescent ligands for dopamine D2/D3 receptors

Allikalt

Purkayastha

Flad

et al. 2020

Sci Rep

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Fluorescent ligands are versatile tools for the study of G protein-coupled receptors. Depending on the fluorophore, they can be used for a range of different applications, including fluorescence microscopy and bioluminescence or fluorescence resonance energy transfer (BRET or FRET) assays. Starting from phenylpiperazines and indanylamines, privileged scaffolds for dopamine D2-like receptors, we developed dansyl-labeled fluorescent ligands that are well accommodated in the binding pockets of D2 and D3 receptors. These receptors are the target proteins for the therapy for several neurologic and psychiatric disorders, including Parkinson’s disease and schizophrenia. The dansyl-labeled ligands exhibit binding affinities up to 0.44 nM and 0.29 nM at D2R and D3R, respectively. When the dansyl label was exchanged for sterically more demanding xanthene or cyanine dyes, fluorescent ligands 10a-c retained excellent binding properties and, as expected from their indanylamine pharmacophore, acted as agonists at D2R. While the Cy3B-labeled ligand 10b was used to visualize D2R and D3R on the surface of living cells by total internal reflection microscopy, ligand 10a comprising a rhodamine label showed excellent properties in a NanoBRET binding assay at D3R.

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Shedding Light on the D₁‐Like Receptors: A Fluorescence‐Based Toolbox for Visualization of the D₁ and D₅ Receptors**

Rosier,

Mönnich,

Nagl

et al. 2023

ChemBioChem

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Dopamine D1‐like receptors are the most abundant type of dopamine receptors in the central nervous system and, even after decades of discovery, still highly interesting for the study of neurological diseases. We herein describe the synthesis of a new set of fluorescent ligands, structurally derived from D1R antagonist SCH‐23390 and labeled with two different fluorescent dyes, as tool compounds for the visualization of D1‐like receptors. Pharmacological characterization in radioligand binding studies identified UR‐NR435 (25) as a high‐affinity ligand for D1‐like receptors (pKi (D1R)=8.34, pKi (D5R)=7.62) with excellent selectivity towards D2‐like receptors. Compound 25 proved to be a neutral antagonist at the D1R and D5R in a Gs heterotrimer dissociation assay, an important feature to avoid receptor internalization and degradation when working with whole cells. The neutral antagonist 25 displayed rapid association and complete dissociation to the D1R in kinetic binding studies using confocal microscopy verifying its applicability for fluorescence microscopy. Moreover, molecular brightness studies determined a single‐digit nanomolar binding affinity of the ligand, which was in good agreement with radioligand binding data. For this reason, this fluorescent ligand is a useful tool for a sophisticated characterization of native D1 receptors in a variety of experimental setups.

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Fluorescent ligands: Bringing light to emerging GPCR paradigms

Cited by 66 publications

References 114 publications

Pharmacological characterisation of novel adenosine A3 receptor antagonists

Pharmacological characterisation of novel adenosine A3 receptor antagonists

Fluorescent ligands for dopamine D2/D3 receptors

Shedding Light on the D₁‐Like Receptors: A Fluorescence‐Based Toolbox for Visualization of the D₁ and D₅ Receptors**

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Fluorescent ligands: Bringing light to emerging GPCR paradigms

Cited by 66 publications

References 114 publications

Pharmacological characterisation of novel adenosine A3 receptor antagonists

Pharmacological characterisation of novel adenosine A3 receptor antagonists

Fluorescent ligands for dopamine D2/D3 receptors

Shedding Light on the D1‐Like Receptors: A Fluorescence‐Based Toolbox for Visualization of the D1 and D5 Receptors**

Contact Info

Product

Resources

About

Shedding Light on the D₁‐Like Receptors: A Fluorescence‐Based Toolbox for Visualization of the D₁ and D₅ Receptors**