Atp colorimetric fluorometric assay kit

Manufactured by Abcam

Sourced in United States, United Kingdom

The ATP Colorimetric/Fluorometric Assay Kit is a tool used to quantify the level of adenosine triphosphate (ATP) in biological samples. It provides a sensitive and accurate method for measuring ATP concentrations through either a colorimetric or fluorometric detection system.

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125 protocols using atp colorimetric fluorometric assay kit

Mitochondrial Dynamics and Energy Metabolism

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OCRs and ECARs were measured using an XF24 Extracellular Flux Analyser (Seahorse Bioscience, North Billerica, MA, USA). HeLa cells (15×10³) transfected with siCtrl or siOPA1 were plated on XF24 microplates 3 days before OCR measurements. Dual-analyte sensor cartridges were soaked in XF Calibrant Solution (Seahorse Biosciences) in 24-well cell-culture microplates overnight at 37°C to hydrate. Approximately 1 h prior to experimentation, injection ports on the sensor cartridge were filled with oligomycin (1 µM), FCCP (1 µM), and rotenone (1 µM) plus antimycin A (1 µM). Plates were then loaded into the XF24 instrument for calibration. For measuring oxygen consumption, the DMEM of HeLa cells was replaced by DMEM supplemented with NaCl (143 mM), Phenol Red (3 mg/ml), glucose (10 mM), glutamine (2 mM) and pyruvate (2 mM) at pH 7.4, and the plates were maintained at 37°C 1 h prior to experimentation. Plates were then loaded into the Seahorse XF24 analyser following the manufacturer's instructions.
ATP measurements in HeLa cells were determined using an ATP Colorimetric/Fluorometric Assay kit (Abcam). Intracellular ATP levels were determined using the colorimetric assay, following the manufacturer's instructions, on 1.10⁶ HeLa cells transfected with control siRNA or OPA1 siRNA. ATP content was measured in duplicate (570 nm) and calculated per microgram of protein.

Millet A.M., Coustham C., Champigny C., Botella M., Demeilliers C., Devin A., Galinier A., Belenguer P., Bordeneuve-Guibé J, & Davezac N. (2023). OPA1 deficiency impairs oxidative metabolism in cycling cells, underlining a translational approach for degenerative diseases. Disease Models & Mechanisms, 16(9), dmm050266.

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ATP Colorimetric Assay Protocol

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The ATP levels were measured using an ATP Colorimetric/Fluorometric Assay Kit (Abcam 83355), according to the manufacturer’s instructions. The absorbance was recorded by spectrophotometer at OD 570 nm.

Majumder S., Ren L., Pushpakumar S, & Sen U. (2019). Hydrogen sulphide mitigates homocysteine-induced apoptosis and matrix remodelling in mesangial cells through Akt/FOXO1 signalling cascade. Cellular signalling, 61, 66-77.

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Metabolic Enzyme Activity Assay

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The activities of IDH2, glucose-6-phosphate dehydrogenase (G6PD), and catalase were measured as described previously [25] (link). The ATP levels were measured using an ATP Colorimetric/Fluorometric Assay Kit (Abcam), according to the manufacturer's instructions.

Han S.J., Choi H.S., Kim J.I., Park J.W, & Park K.M. (2017). IDH2 deficiency increases the liver susceptibility to ischemia-reperfusion injury via increased mitochondrial oxidative injury. Redox Biology, 14, 142-153.

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Quantifying Extracellular ATP Levels

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LLC and A549 cells were treated with DMF solvent, CDDP, MTX, OGD/R, or O + C for 24 h. Then, the cell supernatants were centrifuged at 400 × g for 5 min followed by centrifugation at 2000 × g for 10 min at 4 °C. Next, the supernatants were collected and deproteinized by using perchloric acid and potassium hydroxide. An ATP Colorimetric/Fluorometric assay kit (Abcam, ab83355) was used to quantify the extracellular ATP (ecto-ATP) level following the manufacturer’s instructions. Fluorescence was assessed by a FLUOstar OPTIMA multilabel reader (BMG Labtech, Offenburg, Germany).

Zhang S., Li Y., Liu S., Ma P., Guo M., Zhou E., Duan L., Fan J., Liao T., Tan Q., Wang X., Wu F, & Jin Y. (2022). Ischemia and reperfusion injury combined with cisplatin induces immunogenic cell death in lung cancer cells. Cell Death & Disease, 13(9), 764.

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Measurement of Neurotransmitter Release in Mesenteric Arteries

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To measure the release of NA, ATP, nitrite and CGRP, we used a Noradrenaline research EIA (Labor Diagnostica Nord, Gmbh & Co., KG), an ATP Colorimetric/Fluorometric Assay kit (Abcam, Cambridge, UK), Nitric Oxide Assay Kit (Abcam, Cambridge, UK) and a rat CGRP enzyme immunoassay kit (Spibio, Bertin group), following the manufacturers’ instructions. For sample collecting, endothelium-denuded segments of rat mesenteric arteries from all experimental groups were preincubated for 30 minutes in 5 mL of KHS at 37 °C and continuously gassed with a 95% O₂–5% CO₂ mixture (stabilisation period). This was followed by two washout periods of 10 min in a bath of 0.4 mL of KHS. Then, the medium was collected to measure basal release. Next the organ bath was refilled and cumulative EFS periods of 30 s at 1, 2, 4, 8 and 16 Hz were applied at 1 min intervals. Afterwards, the medium was collected to measure EFS-induced neurotransmitter release. Samples were immediately frozen in liquid nitrogen and conserved at −70 °C until experiments were performed. The EFS-induced neurotransmitter release was calculated by subtracting basal release from that evoked by EFS. Results were expressed as pg NA/mL mg tissue, pmol ATP/mL mg tissue, pmol nitrite/mg tissue and pg CGRP/mL mg tissue.

Sastre E., Caracuel L., Prieto I., Llévenes P., Aller M.Á., Arias J., Balfagón G, & Blanco-Rivero J. (2016). Decompensated liver cirrhosis and neural regulation of mesenteric vascular tone in rats: role of sympathetic, nitrergic and sensory innervations. Scientific Reports, 6, 31076.

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Hepatic ATP Assay Using Colorimetric Kit

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Hepatic ATP was estimated by using an ATP Colorimetric/Fluorometric Assay Kit (Abcam, ab83355) according to the manufacturer instructions. Briefly, liver tissue (20–30 mg) was freeze clamped by an aluminum block precooled in liquid nitrogen and was immediately immersed in liquid nitrogen. Liver samples were stored at -80 °C. On the day of the assay, the liver samples were pulverized in liquid nitrogen and homogenized with 6% perchloric acid. Homogenates were centrifuged at 13,000 g for 5 min at 4 °C, and the supernatants were neutralized to pH 7.8 with 2 M KOH, placed on ice for 1 h, and centrifuged at 13,000 g for 5 min at 4 °C. Absorbance was measured at 570 nm after 30 min incubation in a microplate plate reader (Thermo, Multiskan GO). The concentration of ATP was calculated using an ATP standard curve and expressed in nmol/mg protein.

Lee Y.J., Kim J.Y., Lee D.Y., Park K.J., Kim G.H., Kim J.E., Roh G.S., Lim J.Y., Koo S., Lim N.K., Park H.Y, & Kim W.H. (2020). Alcohol consumption before pregnancy causes detrimental fetal development and maternal metabolic disorders. Scientific Reports, 10, 10054.

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ATP Assay Fluorometric Quantification

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ATP measurements were determined using the ATP Colorimetric/Fluorometric Assay kit (Abcam, Cambridge, MA, USA). Measurements were performed with the fluorometric assay in 96-well black bottom plates at the 48 hour time point, following the manufacturer’s instructions.

Harris F.T., Rahman S.M., Hassanein M., Qian J., Hoeksema M.D., Chen H., Eisenberg R., Chaurand P., Caprioli R.M., Shiota M, & Massion P.P. (2014). Acyl-Coenzyme A Binding Protein Regulates Beta Oxidation Required for Growth and Survival of Non-Small Cell Lung Cancer. Cancer prevention research (Philadelphia, Pa.), 7(7), 748-757.

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Hepatic Lipid and Metabolite Analysis

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To determine triglyceride (TG) content, lipids were extracted from approximately 50 mg of frozen liver homogenized in 20 volumes of 2:1 chloroform–methanol mixture and incubated at 4 °C for a 48 h. Samples were washed with 0.2 volumes of 0.9% NaCl, the upper phase was suctioned off and the chloroform and methanol left to evaporate over several days. Remaining lipid was dissolved in 100% ethanol and TG were quantified using biochemical kits (Randox Laboratories, London, UK). Photometric absorbances were read at 500 nm. TG values were normalized to protein concentrations from the same liver tissue as measured with a BCA kit (Thermo Fischer Scientific). Adenosine triphosphate (ATP) levels in liver was determined using the ATP Colorimetric/Fluorometric Assay kit (Abcam, Toronto, ON, Canada; n = 6 mice per group). Measurements were performed following manufacturer's instructions on 10 mg of frozen tissue after perchloric acid and potassium hydroxide deproteinization. ATP was measured in duplicate and expressed as µmol per gram of wet tissue. Plasma alanine transaminase (ALT) levels were measured using an activity assay kit (Abcam), and plasma albumin was measured using a colometric assay kit (Abcam).

Arvidsson Kvissberg M.E., Hu G., Chi L., Bourdon C., Ling C., ChenMi Y., Germain K., van Peppel I.P., Weise L., Zhang L., Di Giovanni V., Swain N., Jonker J.W., Kim P, & Bandsma R. (2022). Inhibition of mTOR improves malnutrition induced hepatic metabolic dysfunction. Scientific Reports, 12, 19948.

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Mitochondrial ATP Levels Assay

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ATP levels of cells were determined by ATP Colorimetric/Fluorometric Assay kit (ab83355, Abcam, Hong Kong) for mitochondrial dysfunction. Measurements were performed with the colorimetric assay, following the manufacturer's instructions, on 10⁶ cells. ATP contents were measured in triplicate and expressed as % control.

Du J., Zhang X., Han J., Man K., Zhang Y., Chu E.S., Nan Y, & Yu J. (2017). Pro-Inflammatory CXCR3 Impairs Mitochondrial Function in Experimental Non-Alcoholic Steatohepatitis. Theranostics, 7(17), 4192-4203.

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ATP Assay Protocol for Cytotoxicity Evaluation

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The ATP assay was performed using a commercial ATP Colorimetric/Fluorometric assay kit (Catalog number: ab83355, Abcam, UK) according to the manufacturer’s instructions. In brief, cells were seeded in 75 cm² tissue culture flask at a density of 2 × 10⁵ cell/mL and incubated overnight under culturing conditions. Cells were then treated with rotenone or thapsigargin at IC₅₀ concentrations and incubated for 24 h. Untreated cells were included as control. Next, cells were harvested and homogenized in 100 μL of ATP assay buffer. Samples were then mixed with ATP reaction mix and incubated at room temperature for 30 min. ATP level of each well was measured using a microplate reader at OD 570 nm, and quantitation was performed against a standard calibration curve generated using known amounts of ATP. The data was normalized to the percentage of control before statistical analysis.

Weldemariam M.M., Woo J, & Zhang Q. (2022). Pancreatic INS-1 β-Cell Response to Thapsigargin and Rotenone: A Comparative Proteomics Analysis Uncovers Key Pathways of β-Cell Dysfunction. Chemical research in toxicology, 35(6), 1080-1094.

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