logo
AAT Bioquest

Amplite® Fluorimetric Hydrogen Peroxide Assay Kit *Red Fluorescence*

Hydrogen peroxide (H2O2) is a reactive oxygen metabolic by-product that serves as a key regulator for a number of oxidative stress-related states. It is involved in a number of biological events that have been linked to asthma, atherosclerosis, diabetic vasculopathy, osteoporosis, a number of neurodegenerative diseases and Down's syndrome. Perhaps the most intriguing aspect of H2O2 biology is the recent report that antibodies have the capacity to convert molecular oxygen into hydrogen peroxide to contribute to the normal recognition and destruction processes of the immune system. Measurement of this reactive species will help to determine how oxidative stress modulates varied intracellular pathways. Amplite® Hydrogen Peroxide Assay Kit uses our Amplite® Red peroxidase substrate to quantify hydrogen peroxide in solutions and cell extracts. It can also be used to detect a variety of oxidase activities through enzyme-coupled reactions. The kit is an optimized 'mix and read' assay that is compatible with HTS liquid handling instruments.

Example protocol

AT A GLANCE

Protocol summary

  1. Prepare H2O2 working solution (50 µL)
  2. Add H2O2 standards or test samples (50 µL)
  3. Incubate at room temperature for 10 - 30 minutes
  4. Monitor fluorescence intensity at Ex/Em = 540/590 nm

Important notes
Thaw all the kit components at room temperature before starting the experiment.

Important notes
The component A is unstable in the presence of thiols such as DTT and β-mercaptoethanol. Thiols higher than 10 uM (final concentration) would significantly decrease the assay dynamic range.

Important notes
NADH and glutathione (reduced form: GSH) may interfere with the assay.

PREPARATION OF STOCK SOLUTION

Unless otherwise noted, all unused stock solutions should be divided into single-use aliquots and stored at -20 °C after preparation. Avoid repeated freeze-thaw cycles.

1. Amplite™ Red Peroxidase Substrate stock solution (100X):
Add 250 µL of DMSO (Component E) into the vial of Amplite™ Red Substrate (Component A). This stock solution should be used promptly.

2. Peroxidase stock solution (20 U/mL):
Add 1 mL of Assay Buffer (Component C) into the vial of Horseradish Peroxidase (Component D).

3. H2O2 standard solution (20 mM):
Add 22.7 µL of 3% H2O2 (0.88 M, Component B) into 977 µL of Assay Buffer (Component C). Note: Diluted H2O2 solution is not stable. Any unused portions should be discarded.

PREPARATION OF STANDARD SOLUTION

H2O2 standard

For convenience, use the Serial Dilution Planner: https://www.aatbio.com/tools/serial-dilution/11501

Add 1 µL of 20 mM H2O2 stock solution into 1999 µL of Assay Buffer (Component C) to get a 10 µM H2O2 standard (HS7). Take 10 µM H2O2 standard and perform 1:3 serial dilutions to get serial dilutions of H2O2 standard (HS6 - HS1).

PREPARATION OF WORKING SOLUTION

Add 50 μL of Amplite™ Red Peroxidase Substrate stock solution (100X) and 200 μL of Peroxidase stock solution (20 U/mL) into 4.75 mL of Assay Buffer (Component C) to make a total volume of 5 mL. Note: Keep from light.

For guidelines on cell sample preparation, please visit
https://www.aatbio.com/resources/guides/cell-sample-preparation.html

SAMPLE EXPERIMENTAL PROTOCOL

Table 1. Layout of H2O2 standards and test samples in a solid black 96-well microplate. HS = H2O2 standard (HS1-HS7, 0.01 to 10 µM); BL = blank control; TS = test sample.

BLBLTSTS
HS1HS1......
HS2HS2......
HS3HS3  
HS4HS4  
HS5HS5  
HS6HS6  
HS7HS7  

Table 2. Reagent composition for each well. Note that high concentrations of H2O2 (e.g., >100 µM, final concentration) may cause reduced fluorescence signals due to the overoxidation of Amplite™ Red (to non-fluorescent products).

WellVolumeReagent
HS1 - HS750 µLserial dilution (0.01 to 10 µM)
BL50 µLAssay Buffer (Component C)
TS50 µLsample

H2O2 assay in supernatants

  1. Prepare H2O2 standards (HS), blank controls (BL), and test samples (TS) into a solid black 96-well microplate according to the layout provided in Table 1 and Table 2. For a 384-well plate, use 25 µL of reagent per well instead of 50 µL.

  2. Add 50 µL of H2O2 working solution into each well of H2O2 standard, blank control, and test samples to make the total H2O2 assay volume of 100 µL/well. For a 384-well plate, add 25 µL of H2O2 working solution instead, for a total volume of 50 µL/well.

  3. Incubate the reaction at room temperature for 15 to 30 minutes, protected from light.

  4. Monitor the fluorescence increase with a fluorescence plate reader at Excitation = 540 ± 10 nm, Emission = 590 ± 10 nm (optimal Ex/Em = 540/590 nm). Note: The contents of the plate can also be transferred to a white clear bottom microplate and read by an absorbance microplate reader at the wavelength of 576 ± 5 nm. However, the absorption detection has a lower sensitivity compared to that of a fluorescence reading.

H2O2 assay for cells
The Amplite™ Fluorimetric Hydrogen Peroxide Assay Kit can be used to measure the release of H2O2 from cells. The following is a suggested protocol that can be modified to meet the specific research needs.

  1. The H2O2 cell working solution should be prepared as above, except that the Assay Buffer (Component C) should be replaced with the media that is used in your cell culture system. Suggested medias include (a) Krebs Ringers Phosphate Buffer (KRPB); (b) Hanks Balanced Salt Solution (HBSS); or (c) Serum-free media.

  2. Prepare cells in a 96-well plate (50 - 100 µL/well), and activate the cells as desired. Note: The negative controls (media alone and non-activated cells) are included for measuring background fluorescence. For a 384-well plate, use 25 µL/well of cell media instead.

  3. Add 50 µL of H2O2 cell working solution into each well of cells and H2O2 standards. For a 384-well plate, add 25 µL of H2O2 cell working solution into each well instead.

  4. Incubate the reaction at room temperature for 15 to 30 minutes, protected from light.

  5. Monitor the fluorescence increase with a fluorescence plate reader at Excitation = 540 ± 10 nm, Emission = 590 ± 10 nm (optimal Ex/Em = 540/590 nm).

Spectrum

Citations

View all 20 citations: Citation Explorer
An Oxygen Supply Strategy for Sonodynamic Therapy in Tuberculous Granuloma Lesions Using a Catalase-Loaded Nanoplatform
Authors: Hu, Can and Qiu, Yan and Guo, Jiajun and Cao, Yuchao and Li, Dairong and Du, Yonghong
Journal: International Journal of Nanomedicine (2023): 6257--6274
Redox-Active Polyphenol Nanoparticles Deprive Endogenous Glutathione of Electrons for ROS Generation and Tumor Chemodynamic Therapy
Authors: Wang, Yifei and Wang, Jia and Jiao, Yunke and Chen, Kangli and Chen, Tianhao and Wu, Xin-Ping and Jiang, Xingwu and Bu, Wenbo and Liu, Changsheng and Qu, Xue
Journal: Acta Biomaterialia (2023)
Pleiotropic Microenvironment Remodeling Micelles for Cerebral Ischemia-Reperfusion Injury Therapy by Inhibiting Neuronal Ferroptosis and Glial Overactivation
Authors: Li, Chao and Wu, Yuxing and Chen, Qinjun and Luo, Yifan and Liu, Peixin and Zhou, Zheng and Zhao, Zhenhao and Zhang, Tongyu and Su, Boyu and Sun, Tao and others,
Journal: ACS nano (2023)
Macrophage metabolism reprogramming EGCG-Cu coordination capsules delivered in polyzwitterionic hydrogel for burn wound healing and regeneration
Authors: Li, Qinghua and Song, Huijuan and Li, Shuangyang and Hu, Pengbo and Zhang, Chuangnian and Zhang, Ju and Feng, Zujian and Kong, Deling and Wang, Weiwei and Huang, Pingsheng
Journal: Bioactive Materials (2023): 251--264
Neutrophil-Biomimetic “Nanobuffer” for Remodeling the Microenvironment in the Infarct Core and Protecting Neurons in the Penumbra via Neutralization of Detrimental Factors to Treat Ischemic Stroke
Authors: Liu, Shanshan and Xu, Jianpei and Liu, Yipu and You, Yang and Xie, Laozhi and Tong, Shiqiang and Chen, Yu and Liang, Kaifan and Zhou, Songlei and Li, Fengan and others,
Journal: ACS Applied Materials \& Interfaces (2022): 27743--27761

References

View all 152 references: Citation Explorer
A parallel proteomic and metabolomic analysis of the hydrogen peroxide- and Sty1p-dependent stress response in Schizosaccharomyces pombe
Authors: Weeks ME, Sinclair J, Butt A, Chung YL, Worthington JL, Wilkinson CR, Griffiths J, Jones N, Waterfield MD, Timms JF.
Journal: Proteomics (2006): 2772
Effect of antisense oligonucleotide against Smac/DIABLO on inhibition of hydrogen peroxide induced myocardial apoptosis of neonatal rats
Authors: Liang PF, Huang XY, Long JH, Xiao MZ, Yang XH, Zhang PH.
Journal: Zhonghua Shao Shang Za Zhi (2006): 175
Cardioprotective role of endogenous hydrogen peroxide during ischemia-reperfusion injury in canine coronary microcirculation in vivo
Authors: Yada T, Shimokawa H, Hiramatsu O, Haruna Y, Morita Y, Kashihara N, Shinozaki Y, Mori H, Goto M, Ogasawara Y, Kajiya F.
Journal: Am J Physiol Heart Circ Physiol (2006): H1138
Simple and rapid determination of hydrogen peroxide using phosphine-based fluorescent reagents with sodium tungstate dihydrate
Authors: Onoda M, Uchiyama T, Mawatari K, Kaneko K, Nakagomi K.
Journal: Anal Sci (2006): 815
Specific aquaporins facilitate the diffusion of hydrogen peroxide across membranes
Authors: Bienert GP, Moller AL, Kristiansen KA, Schulz A, Moller IM, Schjoerring JK, Jahn TP.
Journal: J Biol Chem. (2006)
Page updated on November 24, 2024

Ordering information

Price
Unit size
Catalog Number11501
Quantity
Add to cart

Additional ordering information

Telephone1-800-990-8053
Fax1-800-609-2943
Emailsales@aatbio.com
InternationalSee distributors
Bulk requestInquire
Custom sizeInquire
Technical SupportContact us
Purchase orderSend to sales@aatbio.com
ShippingStandard overnight for United States, inquire for international
Request quotation

Spectral properties

Excitation (nm)

571

Emission (nm)

584

Storage, safety and handling

Certificate of OriginDownload PDF
H-phraseH303, H313, H333
Hazard symbolXN
Intended useResearch Use Only (RUO)
R-phraseR20, R21, R22
UNSPSC12171501

Platform

Fluorescence microplate reader

Excitation540 nm
Emission590 nm
Cutoff570 nm
Recommended plateSolid black

Components

Hydrogen Peroxide dose response was measured in a solid black 384-well plate with the Amplite® Flourimetric Hydrogen Peroxide Assay Kit using a Gemini fluorescence microplate reader (Molecular Devices).
Hydrogen Peroxide dose response was measured in a solid black 384-well plate with the Amplite® Flourimetric Hydrogen Peroxide Assay Kit using a Gemini fluorescence microplate reader (Molecular Devices).
Hydrogen Peroxide dose response was measured in a solid black 384-well plate with the Amplite® Flourimetric Hydrogen Peroxide Assay Kit using a Gemini fluorescence microplate reader (Molecular Devices).
Concentrations of Concentrations of H<sub>2</sub>O<sub>2</sub> produced by DA alone and with various peptides from the C-terminal sequence of &alpha;-syn 15 min (light gray), 30 min (dark gray), and 60 min (black) after incubation. DA alone (no peptide) produced increasing amounts of H<sub>2</sub>O<sub>2</sub> over time. Co-incubation of DA with the YEMPS peptide enhanced H<sub>2</sub>O<sub>2&nbsp;</sub>production, while the Y127- (EMPSEEGY) and S129- (NEAYEMP) lacking peptides produced less H<sub>2</sub>O<sub>2</sub> than DA alone or with the YEMPS peptide. Moreover, co-incubation of DA with the methionine-mutated peptide (YEAPS) produced the highest amounts of H<sub>2</sub>O<sub>2</sub> among all conditions. *p&lt;0.01 vs. no peptide, **p&lt;0.01 vs. no peptide and YEMPS (ANOVA). *Source: Graph from <strong>Dopamine-Mediated Oxidation of Methionine 127 in &alpha;-Synuclein Causes Cytotoxicity and Oligomerization of &alpha;-Synuclein</strong> by Kazuhiro Nakaso, et al., <em>PLOS ONE</em>, Feb. 2013.&nbsp;&nbsp;
<strong>GW9662 treatment in C22 cells induces PPRE activity and PPAR&alpha; upregulation. C22 cells were treated with PPAR&gamma; antagonist (GW9662) for 24 h with a concentration of 5 &mu;M.</strong><br>Total RNA was isolated from these cultures and subjected to qRT-PCR analysis for PPAR&alpha; (A). The expression of the house keeping gene HPRT was used for normalization. Values &plusmn; SEM represent the mean relative fold induction from three independent experiments. **P &le;0.01; ***P &le;0.001. Dual luciferase reporter activity of PPRE was measured in C22 cells treated either with control (Con) or GW9662 (B). The activity of luciferase was measured in cell lysates and normalized to the activity of renilla. (E.V-empty vector). Data represent &plusmn; SD of three independent experiments, P value, unpaired Student t-test. The culture supernatants were collected subjected to H2O2 assay as per manufacture instructions (C).Source:&nbsp;<strong>PPAR&alpha;-mediated peroxisome induction compensates PPAR&gamma;-deficiency in bronchiolar club cells</strong> by Srikanth Karnati et al., <em>PLOS</em>, Sept 2018.