Novel fluorescent antagonist as a molecular probe in A3 adenosine receptor binding assays using flow cytometry

Kozma, Eszter; Kumar, T. Santhosh; Federico, Stephanie; Phan, Khai; Balasubramanian, R.; Gao, Zhan‐Guo; Paoletta, Silvia; Moro, Stefano; Spalluto, Giampiero

doi:10.1016/j.bcp.2012.02.019

Cited by 35 publications

(62 citation statements)

References 28 publications

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“…In such way, a new fluorophore-conjugated A 3 R antagonist ( 16 ) (Table 2) was synthesized and used for cell-based applications. This compound clearly labelled the A 3 R at the plasma membrane of CHO cells expressing the receptor and by means of FCM a very high specific-to-nonspecific binding ratio was obtained (Kozma et al, 2012). Interestingly, by using this last approach an equilibrium binding constant comparable to that calculated from kinetic radioligand experiments in membranes was observed (Kozma et al, 2012).…”

Section: Uncovering the Biology Of G Protein-coupled Purinergic Rementioning

confidence: 99%

“…This compound clearly labelled the A 3 R at the plasma membrane of CHO cells expressing the receptor and by means of FCM a very high specific-to-nonspecific binding ratio was obtained (Kozma et al, 2012). Interestingly, by using this last approach an equilibrium binding constant comparable to that calculated from kinetic radioligand experiments in membranes was observed (Kozma et al, 2012). Another adenosine receptor fluorescent ligand used in FCM was compound 12 (Table 2), which consisted of an Alexa Fluor 488-conjugated A 2A R agonist.…”

Section: Uncovering the Biology Of G Protein-coupled Purinergic Rementioning

confidence: 99%

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Lighting up G protein-coupled purinergic receptors with engineered fluorescent ligands

Ciruela

Fernández-Dueñas

2015

Neuropharmacology

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The use of G protein-coupled receptors fluorescent ligands is undergoing continuous expansion. In line with this, fluorescent agonists and antagonists of high affinity for G protein-coupled adenosine and P2Y receptors have been shown to be useful pharmacological probe compounds. Fluorescent ligands for A1R, A2AR, and A3R (adenosine receptors) and P2Y2R, P2Y4R, P2Y6R, and P2Y14R (nucleotide receptors) have been reported. Such ligands have been successfully applied to drug discovery and to GPCR characterization by flow cytometry, fluorescence correlation spectroscopy, fluorescence microscopy, fluorescence polarization, fluorescence resonance energy transfer and scanning confocal microscopy. Here we summarize recently reported and readily available representative fluorescent ligands of purinergic receptors. In addition, we pay special attention on the use of this family of fluorescent ligands revealing two main aspects of purinergic receptor biology, namely ligand binding and receptor oligomerization.

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Section: Uncovering the Biology Of G Protein-coupled Purinergic Rementioning

confidence: 99%

Section: Uncovering the Biology Of G Protein-coupled Purinergic Rementioning

confidence: 99%

Lighting up G protein-coupled purinergic receptors with engineered fluorescent ligands

Ciruela

Fernández-Dueñas

2015

Neuropharmacology

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“…However, the approach has also been used for ligands for adenosine [85, 86], adrenergic [87, 88], cannabinoid [89], chemokine [90, 91], galanin [92], long chain fatty acid [93], neuropeptide Y [94], somatostatin [95, 96], urotensin [97], vasopressin [98]and yeast α-factor [82, 99–102] receptors.…”

Section: Fluorescent Ligandsmentioning

confidence: 99%

Fluorescent approaches for understanding interactions of ligands with G protein coupled receptors

Sridharan

Zuber

Connelly

et al. 2014

Biochimica et Biophysica Acta (BBA) - Biomembranes

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G Protein Coupled Receptors (GPCRs) are responsible for a wide variety of signaling responses in diverse cell types. Despite major advances in the determination of structures of this class of receptors, the underlying mechanisms by which binding of different types of ligands specifically elicits particular signaling responses remains unclear. The use of fluorescence spectroscopy can provide important information about the process of ligand binding and ligand dependent conformational changes in receptors, especially kinetic aspects of these processes, that can be difficult to extract from x-ray structures. We present an overview of the extensive array of fluorescent ligands that have been used in studies of GPCRs and describe spectroscopic approaches for assaying binding and probing the environment of receptor-bound ligands with particular attention to examples involving yeast pheromone receptors. In addition, we discuss the use of fluorescence spectroscopy for detecting and characterizing conformational changes in receptors induced by the binding of ligands. Such studies have provided strong evidence for diversity of receptor conformations elicited by different ligands, consistent with the idea that GPCRs are not simple on and off switches. This diversity of states constitutes an underlying mechanistic basis for biased agonism, the observation that different stimuli can produce different responses from a single receptor. It is likely that continued technical advances will allow fluorescence spectroscopy to play an important role in continued probing of structural transitions in GPCRs.

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“…In order to overcome this problem, two differing methods were recently introduced: one on membrane fragments 7 and another on intact cells. 6 Kecskès et al used an Alexa Fluor 488-tagged A 2A AR antagonist MRS5346 ( 53 ) in a newly developed ligand binding assay that uses fluorescence polarization (FP) with A 2A -HEK293 cell membranes. 7,41 The same study also reported a TAMRA derivative MRS5347 ( 55 ) and a BODIPY 650/665-X derivative MRS5418 ( 54 ) synthesized by Kumar et al 41 Conjugates 54 and 55 were designed for FM, and the structure was based on a pyrazolo[4,3- e ][1,2,4]triazolo[1,5- c ]pyrimidine-5-amine (PTP) scaffold that promotes high affinity and selectivity as antagonists for the A 2A AR.…”

Section: Fluorescent Ar Ligands As Tracers In Ligand Binding Assaysmentioning

confidence: 99%

“…6,7 Recently, the expense, health risks, and disposal issues that radioligands pose have increased the need to develop more efficient techniques. Fluorescent methods solve many of these issues associated with radioactivity, in addition to providing other advantages.…”

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confidence: 99%

Fluorescent ligands for adenosine receptors

Kozma¹,

Jayasekara²,

Squarcialupi³

et al. 2013

Bioorganic & Medicinal Chemistry Letters

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Interest is increasing in developing fluorescent ligands for characterization of adenosine receptors (ARs), which hold a promise of usefulness in the drug discovery process. The size of a strategically labeled AR ligand can be greatly increased after the attachment of a fluorophore. The choice of dye moiety (e.g. Alexa Fluor 488), attachment point and linker length can alter the selectivity and potency of the parent molecule. Fluorescent derivatives of adenosine agonists and antagonists (e.g. XAC and other heterocyclic antagonist scaffolds) have been synthesized and characterized pharmacologically. Some are useful AR probes for flow cytometry, fluorescence correlation spectroscopy, fluorescence microscopy, fluorescence polarization, fluorescence resonance energy transfer, and scanning confocal microscopy. Thus, the approach of fluorescent labeled GPCR ligands, including those for ARs, is a growing dynamic research field.

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Novel fluorescent antagonist as a molecular probe in A3 adenosine receptor binding assays using flow cytometry

Cited by 35 publications

References 28 publications

Lighting up G protein-coupled purinergic receptors with engineered fluorescent ligands

Lighting up G protein-coupled purinergic receptors with engineered fluorescent ligands

Fluorescent approaches for understanding interactions of ligands with G protein coupled receptors

Fluorescent ligands for adenosine receptors

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