DCFDA / H2DCFDA - Cellular ROS Assay试剂盒(ab113851)
Key features and details
- Assay type: Cell-based (quantitative)
- Detection method: Fluorescent
- Platform: Microplate reader, Fluor. microscope, Flow cyt.
- Assay time: 40 min
- Sample type: Adherent cells, Suspension cells
概述
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产品名称
DCFDA / H2DCFDA - Cellular ROS Assay试剂盒
参阅全部 Oxidative Stress 试剂盒 -
检测方法
Fluorescent -
样品类型
Adherent cells, Suspension cells -
检测类型
Cell-based (quantitative) -
检测时间
0h 40m -
产品概述
DCFDA - Cellular ROS Assay Kit / Reactive Oxygen Species Assay Kit (ab113851) uses the cell permeant reagent 2’,7’ –dichlorofluorescin diacetate (DCFDA, also known as H2DCFDA, DCFH-DA, and DCFH) to semi quantitatively assess reactive oxygen species in live cell samples.
DCFDA / H2DCFDA / DCFH-DA / DCFH is a fluorogenic dye that measures hydroxyl, peroxyl and other reactive oxygen species (ROS) activity within the cell. NB: DCFDA and DCFA are also available as free molecules as ab145286 (Carboxy-DCFDA N-succinimidyl ester) and ab145439 (5(6)-Carboxy-2',7'-dichlorofluorescein).
The DCFDA assay protocol is based on the diffusion of DCFDA / H2DCFDA / DCFH-DA / DCFH into the cell. It is then deacetylated by cellular esterases to a non-fluorescent compound, which is later oxidized by ROS into 2’, 7’ –dichlorofluorescein (DCF). DCF is highly fluorescent and is detected by fluorescence spectroscopy with excitation / emission at 485 nm / 535 nm.
DCFDA assay protocol / ROS assay protocol summary (microplate):
- collect suspension cells in tube / seed and allow attachment of adherent cells in 96-well plate
- wash in buffer
- stain with DCFDA for 30 min (suspension) / 45 min (adherent), wash with buffer
- if suspension cells, transfer to microplate
- analyze with microplate reader
DCFDA assay protocol / ROS assay protocol summary (flow cytometry):
- collect cells in tubes
- stain with DCFDA for 30 min (without washing)
- analyze with flow cytometer
DCFDA assay protocol / ROS assay protocol summary (fluorescent microscopy):
- wash adherent cells with buffer
- stain with DCFDA for 45 min
- wash in buffer
- analyze with fluorescent microscope
- maintain low light conditions to reduce photo-bleaching -
说明
Previously called DCFDA / H2DCFDA - Cellular Reactive Oxygen Species Detection Assay Kit.
This kit contains sufficient materials for approximately 300 measurements in microplate format and 70 measurements (35 mL) by flow cytometry. The number of measurements in microscopy is dependent on experimental setup.
This kit is not compatible with fixed samples. Stained cells must be measured live.
Related productsReview the oxidative stress marker and assay guide, or the full metabolism assay guide to learn about more assays for metabolites, metabolic enzymes, mitochondrial function, and oxidative stress, and also how to assay metabolic function in live cells using your plate reader.
For reactive oxygen species, the most popular live cell ROS assay is DCFDA Assay ab113851 (green). Alternative ROS assays are available in orange (ab186028), red (ab186027), and deep red (ab186029). ab238535 is used to measure ROS in biofluids, culture supernatants and cell lysates.
For assays designed to differentiate ROS, superoxides, and reactive nitrogen species: to assay ROS and superoxides use ab139476; to assay ROS, superoxides, and reactive nitrogen species use ab139473; to assay superoxides use ab219943.
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平台
Microplate reader, Fluor. microscope, Flow cyt.
性能
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存放说明
Store at -20°C. Please refer to protocols. -
组件 300 tests 10X Dilution Buffer (Sterile) 1 x 10ml 20 mM DCFDA (Label) 1 x 35µl 55mM TBHP 1 x 50µl -
研究领域
相关产品
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Related Products
图片
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Effect of anethole on excessive ROS generation in hMSCs.Image from Rhee YH et al., BMC Cell Biol, 2018, 19: 12, Fig. 3B.; doi: 10.1186/s12860-018-0163-2 Reproduced under the Creative Commons license https://creativecommons.org/licenses/by/4.0/
Effect of anethole on excessive ROS generation in hMSCs. hMSCs were exposed at 2 mM H2O2 for 30 min and incubated for 2 days in presence or absence of 50 μM anethole. ROS was measured by staining the cells with DCFDA cellular ROS detection assay kit according to the manufacturer’s instructions. ROS generation was observed under a fluorescence microscope at 200× magnification.
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DCFDA ROS assay used to study Doxorubicin cardiotoxicityKobashigawa et al. (Pubmed 28056084)Kobashigawa et al. (Pubmed 25127116) used the DCFDA ROS assay ab113851 to investigate the causes of the protective effects of metformin (Met) treatment in Doxorubicin (Dox) induced cardiotoxicity.
They identified that in metformin treated H9c2 rat immortalized cardiomyoblasts, Met treatment reduced ROS levels induced by Dox (A). Values represent mean ± S.D. (n = 4).
In combination with other assays, they developed the hypothesis that Dox induces increased ROS expression, leading to increased calcium levels and cell death, and that Met reduces this effect by increasing AMPK expression.
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Flow Cytometry - DCFDA - Cellular Reactive Oxygen Species Detection Assay Kit (ab113851)ab113851 (DCFDA) labeled and unlabeled Jurkat cells were treated with 50 µM tert-butyl Hydrogen Peroxide (tbHP), then analyzed by flow cytometry.
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p38 MAPK pathway involved in oxidative injury to HCECs challenged with C. albicans.Image from Hua X et al., Sci Rep, 2017, 7: 10421, Fig. 4A.; doi: 10.1038/s41598-017-09636-w Reproduced under the Creative Commons license http://creativecommons.org/licenses/by/4.0/p38 MAPK pathway involved in oxidative injury to HCECs challenged with C. albicans. Increased ROS generation in HCECs challenged with C. albicans and inhibition by the p38 activation inhibitor SB203580.
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AbReviewThis image is courtesy of an anonymous AbreviewROS levels analysis in human immortalized cardiomyocytes cells with ab113851 under different treatment conditions.
Data are mean ± SEM of three different experiments. H2O2 800μM was used as Positive Control. The values of fluorescence intensity at each time point are indicated as the ratio of the value at specific t-time point on the value at time point zero (first measurement) (t-time point/t0). Briefly, cells were plated (seeding density 2.5 x 104 cells/cm2) in FBS-supplemented medium w/o phenol red onto a 96 black well plate. After 24 hours the cells were washed one time with 1X buffer (provided in the kit), then the cells were incubated with DFCDA 10 μM for 30 min at 37° C protected from light. Following incubation the wells were washed with PBS and the cells were exposed to treatments of interest in FBS-supplemented medium w/o phenol red. ROS production was determined immediately by measuring the formation of fluorescent dichloro fluorescein (DCF), using a PerkinElmer VICTOR3, at an Ex-485 and Em-535 nm. Measurements were done every 30 min for six hours. The value of fluorescence intensity at each time point is reported. The value reported was obtained by the ratio of fluorescence at specific time point on fluorescence at time 0, which was measured immediately after DCFDA incubation.
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Functional Studies - DCFDA - Cellular Reactive Oxygen Species Detection Assay Kit (ab113851)Jurkat cells were labeled with DCFDA (20 µM) or unlabeled (none) and then cultured an additional 3 hours with or without 50 µM tert-butyl hydrogen peroxide (TBHP) according to the protocol. Cells were then analyzed on a fluorescent plate reader. Mean +/- standard deviation is plotted for 4 replicates from each condition. TBHP mimics ROS activity to oxidize DCFDA to fluorescent DCF.
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Acute Effect of anthracyclines on ROS production in HL60 cells.Labeled HL60 cells were treated with idarubicin or doxorubicin for 4 hours at multiple doses according to the protocol. At the end of the treatment cells were read end point in a fluorescent plate reader (Perking Elmer-Wallac 1420 Victor 2 Multilabel plate reader). Mean +/- standard deviation is plotted for 3 replicates from each condition. The dotted line represents the mean of 24 replicates of HL60 cells treated with 0.5% DMSO.
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Reactive oxygen species (ROS) measured using the DCFDA assayImage from Davidson et al., Sci Rep, 2018. Fig. 2B.; doi: 10.1038/s41598-018-35455-8 Reproduced under the Creative Commons license http://creativecommons.org/licenses/by/4.0/Reactive oxygen species (ROS) measured using the DCFDA assay in human primary articular chondrocytes. Cells were treated with 100 µM tert-butyl-hydroperoxide (tBHP) alone (4 h) ± pre-treatment with apigenin.
数据表及文件
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SDS download
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Datasheet download
文献 (743)
ab113851 被引用在 743 文献中.
- Liao CH et al. Inhibition of Polyinosinic-Polycytidylic Acid-Induced Acute Pulmonary Inflammation and NF-κB Activation in Mice by a Banana Plant Extract. Int J Med Sci 21:107-122 (2024). PubMed: 38164360
- Weng L et al. Surplus fatty acid synthesis increases oxidative stress in adipocytes and lnduces lipodystrophy. Nat Commun 15:133 (2024). PubMed: 38168040
- Jiang Y et al. Targeting NEDD8 suppresses surgical stress-facilitated metastasis of colon cancer via restraining regulatory T cells. Cell Death Dis 15:8 (2024). PubMed: 38177106
- Shrivastava G et al. Aedes aegypti saliva modulates inflammasome activation and facilitates flavivirus infection in vitro. iScience 27:108620 (2024). PubMed: 38188518
- Wang S et al. α-Mangostin Exhibits a Therapeutic Effect on Spinal Cystic Echinococcosis by Affecting Glutamine Metabolism. Antimicrob Agents Chemother 67:e0009823 (2023). PubMed: 37140388