Live-cell microscopy or fluorescence anisotropy with budded baculoviruses—which way to go with measuring ligand binding to M
            <sub>4</sub>
            muscarinic receptors?

Tahk, Maris‐Johanna; Torp, Jane; Ali, Mohammed A. S.; Fishman, Dmytro; Parts, Leopold; Grätz, Lukas; Müller, Christoph E.; Keller, Max; Veikšina, Santa; Laasfeld, Tõnis; Rinken, Ago

doi:10.1098/rsob.220019

Cited by 7 publications

(12 citation statements)

References 95 publications

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“…In the field of muscarinergic ligands, only very few conjugates to fluorescent dyes have so far been described (Figure ). − The conjugate 1 recently reported by Keller et al is based on a dibenzodiazepinone pharmacophore (blue) and comprises a Cy5-type dye (red) with two sulfonate groups for increased solubility in water. As conjugate 1 and its derivatives show strong preference for binding to the M 2 receptor over M 3 (10–500-fold), they are primarily suited as tools for investigations of the M 2 subtype.…”

Section: Introductionmentioning

confidence: 99%

Synthesis, Characterization, and Application of Muscarinergic M₃ Receptor Ligands Linked to Fluorescent Dyes

et al. 2022

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Through the linkage of two muscarinergic M 3 receptor ligands to fluorescent tetramethylrhodamine-and cyanine-5-type dyes, two novel tool compounds, OFH5503 and OFH611, have been developed. Based on the suitable binding properties and kinetics related to the M 3 subtype, both ligand-dye conjugates were found to be useful tools to determine binding affinities via flow cytometric measurements. In addition, confocal microscopy underlined the comparably low unspecific binding and the applicability for studying M 3 receptor expression in cells. Along with the proven usefulness regarding studies on the M 3 subtype, the conjugates OFH5503 and OFH611 could, due to their high affinity to the M 1 receptor, evolve as even more versatile tools in the field of research on muscarinergic receptors.

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Section: Introductionmentioning

confidence: 99%

Synthesis, Characterization, and Application of Muscarinergic M₃ Receptor Ligands Linked to Fluorescent Dyes

et al. 2022

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“…For fine-tuning the U-Net cell segmentation model for HEK293 cells, the fluorescence ground-truth masks were generated as described in ( Tahk et al, 2022 ). Briefly, HEK293-D3R cells were seeded with a density of 20,000 cells/well into a µ-Plate 96 well Black well plate (Ibidi, Gräfelfing, Germany) and incubated for 2.5 h. One mM DiI (Invitrogen, Eugene, Oregon, United States) in DMSO kept at -20°C was thawed and, to disrupt aggregates, kept in an ultrasound bath for 5 min.…”

Section: Methodsmentioning

confidence: 99%

“…Image analysis was performed as described in ( Tahk et al, 2022 ) with some modifications. For training the final U-Net2D image segmentation model in the ZeroCostDL4Mic ( Ronneberger et al, 2015 ; von Chamier et al, 2021 ) environment, U-Net2D notebook with minor modifications was used to allow compatibility with Aparecium and Matlab Keras framework model import.…”

Section: Methodsmentioning

confidence: 99%

“…Therefore, fluorescence polarization assays and other fluorescence based methods allowing kinetic measurements help reduce this fundamental knowledge gap. Fluorescence anisotropy (FA) assay has been used to study the ligand binding kinetics of many GPCRs - 5-HT 1A ( Tõntson et al, 2014 ), melanocortin MC 4 ( Link et al, 2017 ), dopamine D 1 ( Allikalt et al, 2018 ), neuropeptide Y Y 1 ( Müller et al, 2022 ), muscarinic acetylcholine M 2 ( Grätz et al, 2021 ) and M 4 ( Tahk et al, 2022 ) receptors. FA is based on measuring the change in rotational freedom of the fluorescent label upon receptor binding and, therefore, does not require the physical separation of the bound and free ligand ( Rinken et al, 2018 ).…”

Section: Introductionmentioning

confidence: 99%

“…The advantage of this approach is that no additional fluorescence channels are needed for cell and cell contour detection reducing both photo and chemical toxicity while also allowing for the analysis of different areas of the cell depending on the cell type or the goal of the analysis. The method has been further developed to allow for kinetic measurements and reduced data volumes by employing deep convolutional neural networks, which regularly surpass more classical machine learning models such as random forests ( Caicedo et al, 2019 ; Tahk et al, 2022 ). Nowadays, many machine learning models can be developed in almost any available high-performance cluster or even on a reasonably powerful PC, but it is also possible to use freely available open-source cloud-based tools for the task.…”

Section: Introductionmentioning

confidence: 99%

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Fluorescence based HTS-compatible ligand binding assays for dopamine D3 receptors in baculovirus preparations and live cells

Tahk

Laasfeld

Meriste

et al. 2023

Front. Mol. Biosci.

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Dopamine receptors are G-protein-coupled receptors that are connected to severe neurological disorders. The development of new ligands targeting these receptors enables gaining a deeper insight into the receptor functioning, including binding mechanisms, kinetics and oligomerization. Novel fluorescent probes allow the development of more efficient, cheaper, reliable and scalable high-throughput screening systems, which speeds up the drug development process. In this study, we used a novel Cy3B labelled commercially available fluorescent ligand CELT-419 for developing dopamine D3 receptor-ligand binding assays with fluorescence polarization and quantitative live cell epifluorescence microscopy. The fluorescence anisotropy assay using 384-well plates achieved Z’ value of 0.71, which is suitable for high-throughput screening of ligand binding. The assay can also be used to determine the kinetics of both the fluorescent ligand as well as some reference unlabeled ligands. Furthermore, CELT-419 was also used with live HEK293-D3R cells in epifluorescence microscopy imaging for deep-learning-based ligand binding quantification. This makes CELT-419 quite a universal fluorescence probe which has the potential to be also used in more advanced microscopy techniques resulting in more comparable studies.

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Exploring Muscarinic Acetylcholine Receptor Binding Kinetics with Fluorescence Anisotropy

Laasfeld,

Tahk,

Allikalt

et al. 2024

Neuromethods

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Live-cell microscopy or fluorescence anisotropy with budded baculoviruses—which way to go with measuring ligand binding to M ₄ muscarinic receptors?

Cited by 7 publications

References 95 publications

Synthesis, Characterization, and Application of Muscarinergic M₃ Receptor Ligands Linked to Fluorescent Dyes

Synthesis, Characterization, and Application of Muscarinergic M₃ Receptor Ligands Linked to Fluorescent Dyes

Fluorescence based HTS-compatible ligand binding assays for dopamine D3 receptors in baculovirus preparations and live cells

Exploring Muscarinic Acetylcholine Receptor Binding Kinetics with Fluorescence Anisotropy

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Live-cell microscopy or fluorescence anisotropy with budded baculoviruses—which way to go with measuring ligand binding to M 4 muscarinic receptors?

Cited by 7 publications

References 95 publications

Synthesis, Characterization, and Application of Muscarinergic M3 Receptor Ligands Linked to Fluorescent Dyes

Synthesis, Characterization, and Application of Muscarinergic M3 Receptor Ligands Linked to Fluorescent Dyes

Fluorescence based HTS-compatible ligand binding assays for dopamine D3 receptors in baculovirus preparations and live cells

Exploring Muscarinic Acetylcholine Receptor Binding Kinetics with Fluorescence Anisotropy

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Product

Resources

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Live-cell microscopy or fluorescence anisotropy with budded baculoviruses—which way to go with measuring ligand binding to M ₄ muscarinic receptors?

Synthesis, Characterization, and Application of Muscarinergic M₃ Receptor Ligands Linked to Fluorescent Dyes

Synthesis, Characterization, and Application of Muscarinergic M₃ Receptor Ligands Linked to Fluorescent Dyes