dye reagent solution Search Results


carboxyphenol ba  (Chem Impex International)
94
Chem Impex International carboxyphenol ba
Carboxyphenol Ba, supplied by Chem Impex International, used in various techniques. Bioz Stars score: 94/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/carboxyphenol ba/product/Chem Impex International
Average 94 stars, based on 1 article reviews
carboxyphenol ba - by Bioz Stars, 2026-03
94/100 stars
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core solution  (Chem Impex International)
95
Chem Impex International core solution
Core Solution, supplied by Chem Impex International, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/core solution/product/Chem Impex International
Average 95 stars, based on 1 article reviews
core solution - by Bioz Stars, 2026-03
95/100 stars
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thallos ion channel reagent (am) dye loading solution  (TEFLabs Inc)
90
TEFLabs Inc thallos ion channel reagent (am) dye loading solution
Identification of TREK-2 bioactive lipid activators with a thallium flux assay. (A) <t>Thallos</t> fluorescence monitored before and after addition of Tl+ (arrow) to T-REx-TREK-2 cells induced with tetracycline (1 µg/mL, blue traces) or not induced (red traces). Inset is a Western blot run with T-REx-TREK-2 cell lysates with (+) or without (−) tetracycline induction and probed with a TREK-2 antibody. (B) Bioactive lipids that activate TREK-2 channels when preincubated with T-REx-TREK-2 cells for 5 min at a 10 µM concentration. (C) Tl+ flux (arrow) into thallos loaded TREK-2 expressing cells with (blue) or without (red) pretreatment with 11-deoxy prostaglandin F2α ± SEM (p < 0.001 after 300 s). (D) Dose–response curve for TREK-2 activation with 11-deoxy prostaglandin F2α ± S.E.M.; fitting determined an EC50 value of 0.294 µM. (E) Calculation of the Z′ using the slope of Tl+ influx for each well of a 384 well plate containing TREK-2 expressing cells treated with 11-deoxy prostaglandin F2α (top) or vehicle (bottom, Z′ of 0.752).
Thallos Ion Channel Reagent (Am) Dye Loading Solution, supplied by TEFLabs Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/thallos ion channel reagent (am) dye loading solution/product/TEFLabs Inc
Average 90 stars, based on 1 article reviews
thallos ion channel reagent (am) dye loading solution - by Bioz Stars, 2026-03
90/100 stars
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2% basic fuchsine dye solution  (Carlo Erba Reagents)
90
Carlo Erba Reagents 2% basic fuchsine dye solution
Identification of TREK-2 bioactive lipid activators with a thallium flux assay. (A) <t>Thallos</t> fluorescence monitored before and after addition of Tl+ (arrow) to T-REx-TREK-2 cells induced with tetracycline (1 µg/mL, blue traces) or not induced (red traces). Inset is a Western blot run with T-REx-TREK-2 cell lysates with (+) or without (−) tetracycline induction and probed with a TREK-2 antibody. (B) Bioactive lipids that activate TREK-2 channels when preincubated with T-REx-TREK-2 cells for 5 min at a 10 µM concentration. (C) Tl+ flux (arrow) into thallos loaded TREK-2 expressing cells with (blue) or without (red) pretreatment with 11-deoxy prostaglandin F2α ± SEM (p < 0.001 after 300 s). (D) Dose–response curve for TREK-2 activation with 11-deoxy prostaglandin F2α ± S.E.M.; fitting determined an EC50 value of 0.294 µM. (E) Calculation of the Z′ using the slope of Tl+ influx for each well of a 384 well plate containing TREK-2 expressing cells treated with 11-deoxy prostaglandin F2α (top) or vehicle (bottom, Z′ of 0.752).
2% Basic Fuchsine Dye Solution, supplied by Carlo Erba Reagents, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/2% basic fuchsine dye solution/product/Carlo Erba Reagents
Average 90 stars, based on 1 article reviews
2% basic fuchsine dye solution - by Bioz Stars, 2026-03
90/100 stars
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mtt dye uptake method cell titer 96 aqueous one solution reagent  (Promega)
90
Promega mtt dye uptake method cell titer 96 aqueous one solution reagent
Identification of TREK-2 bioactive lipid activators with a thallium flux assay. (A) <t>Thallos</t> fluorescence monitored before and after addition of Tl+ (arrow) to T-REx-TREK-2 cells induced with tetracycline (1 µg/mL, blue traces) or not induced (red traces). Inset is a Western blot run with T-REx-TREK-2 cell lysates with (+) or without (−) tetracycline induction and probed with a TREK-2 antibody. (B) Bioactive lipids that activate TREK-2 channels when preincubated with T-REx-TREK-2 cells for 5 min at a 10 µM concentration. (C) Tl+ flux (arrow) into thallos loaded TREK-2 expressing cells with (blue) or without (red) pretreatment with 11-deoxy prostaglandin F2α ± SEM (p < 0.001 after 300 s). (D) Dose–response curve for TREK-2 activation with 11-deoxy prostaglandin F2α ± S.E.M.; fitting determined an EC50 value of 0.294 µM. (E) Calculation of the Z′ using the slope of Tl+ influx for each well of a 384 well plate containing TREK-2 expressing cells treated with 11-deoxy prostaglandin F2α (top) or vehicle (bottom, Z′ of 0.752).
Mtt Dye Uptake Method Cell Titer 96 Aqueous One Solution Reagent, supplied by Promega, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/mtt dye uptake method cell titer 96 aqueous one solution reagent/product/Promega
Average 90 stars, based on 1 article reviews
mtt dye uptake method cell titer 96 aqueous one solution reagent - by Bioz Stars, 2026-03
90/100 stars
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colorimetric vital dye celltiter 96 aqueous one solution reagent  (Promega)
90
Promega colorimetric vital dye celltiter 96 aqueous one solution reagent
Identification of TREK-2 bioactive lipid activators with a thallium flux assay. (A) <t>Thallos</t> fluorescence monitored before and after addition of Tl+ (arrow) to T-REx-TREK-2 cells induced with tetracycline (1 µg/mL, blue traces) or not induced (red traces). Inset is a Western blot run with T-REx-TREK-2 cell lysates with (+) or without (−) tetracycline induction and probed with a TREK-2 antibody. (B) Bioactive lipids that activate TREK-2 channels when preincubated with T-REx-TREK-2 cells for 5 min at a 10 µM concentration. (C) Tl+ flux (arrow) into thallos loaded TREK-2 expressing cells with (blue) or without (red) pretreatment with 11-deoxy prostaglandin F2α ± SEM (p < 0.001 after 300 s). (D) Dose–response curve for TREK-2 activation with 11-deoxy prostaglandin F2α ± S.E.M.; fitting determined an EC50 value of 0.294 µM. (E) Calculation of the Z′ using the slope of Tl+ influx for each well of a 384 well plate containing TREK-2 expressing cells treated with 11-deoxy prostaglandin F2α (top) or vehicle (bottom, Z′ of 0.752).
Colorimetric Vital Dye Celltiter 96 Aqueous One Solution Reagent, supplied by Promega, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/colorimetric vital dye celltiter 96 aqueous one solution reagent/product/Promega
Average 90 stars, based on 1 article reviews
colorimetric vital dye celltiter 96 aqueous one solution reagent - by Bioz Stars, 2026-03
90/100 stars
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150 ll of abf dye reagent working solution  (Promega)
90
Promega 150 ll of abf dye reagent working solution
Identification of TREK-2 bioactive lipid activators with a thallium flux assay. (A) <t>Thallos</t> fluorescence monitored before and after addition of Tl+ (arrow) to T-REx-TREK-2 cells induced with tetracycline (1 µg/mL, blue traces) or not induced (red traces). Inset is a Western blot run with T-REx-TREK-2 cell lysates with (+) or without (−) tetracycline induction and probed with a TREK-2 antibody. (B) Bioactive lipids that activate TREK-2 channels when preincubated with T-REx-TREK-2 cells for 5 min at a 10 µM concentration. (C) Tl+ flux (arrow) into thallos loaded TREK-2 expressing cells with (blue) or without (red) pretreatment with 11-deoxy prostaglandin F2α ± SEM (p < 0.001 after 300 s). (D) Dose–response curve for TREK-2 activation with 11-deoxy prostaglandin F2α ± S.E.M.; fitting determined an EC50 value of 0.294 µM. (E) Calculation of the Z′ using the slope of Tl+ influx for each well of a 384 well plate containing TREK-2 expressing cells treated with 11-deoxy prostaglandin F2α (top) or vehicle (bottom, Z′ of 0.752).
150 Ll Of Abf Dye Reagent Working Solution, supplied by Promega, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/150 ll of abf dye reagent working solution/product/Promega
Average 90 stars, based on 1 article reviews
150 ll of abf dye reagent working solution - by Bioz Stars, 2026-03
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Image Search Results


Identification of TREK-2 bioactive lipid activators with a thallium flux assay. (A) Thallos fluorescence monitored before and after addition of Tl+ (arrow) to T-REx-TREK-2 cells induced with tetracycline (1 µg/mL, blue traces) or not induced (red traces). Inset is a Western blot run with T-REx-TREK-2 cell lysates with (+) or without (−) tetracycline induction and probed with a TREK-2 antibody. (B) Bioactive lipids that activate TREK-2 channels when preincubated with T-REx-TREK-2 cells for 5 min at a 10 µM concentration. (C) Tl+ flux (arrow) into thallos loaded TREK-2 expressing cells with (blue) or without (red) pretreatment with 11-deoxy prostaglandin F2α ± SEM (p < 0.001 after 300 s). (D) Dose–response curve for TREK-2 activation with 11-deoxy prostaglandin F2α ± S.E.M.; fitting determined an EC50 value of 0.294 µM. (E) Calculation of the Z′ using the slope of Tl+ influx for each well of a 384 well plate containing TREK-2 expressing cells treated with 11-deoxy prostaglandin F2α (top) or vehicle (bottom, Z′ of 0.752).

Journal: ACS chemical neuroscience

Article Title: Selective Small Molecule Activators of TREK-2 Channels Stimulate Dorsal Root Ganglion c-Fiber Nociceptor Two-Pore-Domain Potassium Channel Currents and Limit Calcium Influx

doi: 10.1021/acschemneuro.6b00301

Figure Lengend Snippet: Identification of TREK-2 bioactive lipid activators with a thallium flux assay. (A) Thallos fluorescence monitored before and after addition of Tl+ (arrow) to T-REx-TREK-2 cells induced with tetracycline (1 µg/mL, blue traces) or not induced (red traces). Inset is a Western blot run with T-REx-TREK-2 cell lysates with (+) or without (−) tetracycline induction and probed with a TREK-2 antibody. (B) Bioactive lipids that activate TREK-2 channels when preincubated with T-REx-TREK-2 cells for 5 min at a 10 µM concentration. (C) Tl+ flux (arrow) into thallos loaded TREK-2 expressing cells with (blue) or without (red) pretreatment with 11-deoxy prostaglandin F2α ± SEM (p < 0.001 after 300 s). (D) Dose–response curve for TREK-2 activation with 11-deoxy prostaglandin F2α ± S.E.M.; fitting determined an EC50 value of 0.294 µM. (E) Calculation of the Z′ using the slope of Tl+ influx for each well of a 384 well plate containing TREK-2 expressing cells treated with 11-deoxy prostaglandin F2α (top) or vehicle (bottom, Z′ of 0.752).

Article Snippet: Cells were loaded with 20 μL of Thallos Ion Channel reagent (AM) (TEFLabs, Austin, TX) dye loading solution for 45 min at ambient temperature for the HTS (dye solution: 50 μg of Thallos-AM in 20 μL of pure, dry DMSO with 10 μL of 20% pluronic F-127, diluted to 2 μM in assay buffer) and for 1 h for subsequent experiments.

Techniques: Flux Assay, Fluorescence, Western Blot, Concentration Assay, Expressing, Activation Assay

Optimization of the secondary TREK-1 Tl+ flux assay. (A) Thallos fluorescence (F488) monitored before and after addition of Tl+ (arrow) to T-REx-TREK-1 cells induced with tetracycline (1 µg/mL, blue) or not induced (red) ± SEM. (B) Tl+ flux (arrow) into thallos loaded T-REx-TREK-1 expressing cells with (red) or without (blue) 10 min pretreatment with 1.8 µM 11-deoxy prostaglandin F2α ± SEM.

Journal: ACS chemical neuroscience

Article Title: Selective Small Molecule Activators of TREK-2 Channels Stimulate Dorsal Root Ganglion c-Fiber Nociceptor Two-Pore-Domain Potassium Channel Currents and Limit Calcium Influx

doi: 10.1021/acschemneuro.6b00301

Figure Lengend Snippet: Optimization of the secondary TREK-1 Tl+ flux assay. (A) Thallos fluorescence (F488) monitored before and after addition of Tl+ (arrow) to T-REx-TREK-1 cells induced with tetracycline (1 µg/mL, blue) or not induced (red) ± SEM. (B) Tl+ flux (arrow) into thallos loaded T-REx-TREK-1 expressing cells with (red) or without (blue) 10 min pretreatment with 1.8 µM 11-deoxy prostaglandin F2α ± SEM.

Article Snippet: Cells were loaded with 20 μL of Thallos Ion Channel reagent (AM) (TEFLabs, Austin, TX) dye loading solution for 45 min at ambient temperature for the HTS (dye solution: 50 μg of Thallos-AM in 20 μL of pure, dry DMSO with 10 μL of 20% pluronic F-127, diluted to 2 μM in assay buffer) and for 1 h for subsequent experiments.

Techniques: Flux Assay, Fluorescence, Expressing