Optimized DPPH assay in a detergent-based buffer system for measuring antioxidant activity of proteins.

TitleOptimized DPPH assay in a detergent-based buffer system for measuring antioxidant activity of proteins.
Publication TypeJournal Article
Year of Publication2014
AuthorsNicklisch, SCT, Waite, JH
JournalMethodsX
Volume1
Pagination233-238
Date Published2014
ISSN2215-0161
Abstract

The 1,1-Diphenyl-2-picryl-hydrazyl (DPPH) assay is well established for the in vitro determination of antioxidant activity in food and biological extracts. The standard DPPH assay uses methanol or ethanol as solvents, or buffered alcoholic solutions in a ratio of 40%/60% (buffer/alcohol, v/v) to keep the hydrophobic hydrazyl radical and phenolic test compounds soluble while offering sufficient buffering capacity at different pHs tested. Following this protocol, we were unable to keep proteinaceous antioxidants soluble at different pHs to test for their antioxidant activity. Thus, the assay protocol was modified as follows to improve its utility: Non-ionic detergents were added to keep the DPPH radical soluble and to provide a mild and non-denaturing environment for the antioxidant protein.Maximal concentration of DPPH was limited to 100 μM to stay within the sensitivity range of the detector at the given wavelength (515 nm) and to increase the dynamic range of the assay.0.1 M citrate phosphate buffer was introduced to prevent experimental artifacts due to changing buffer compositions at different pHs.

DOI10.1016/j.mex.2014.10.004
Alternate JournalMethodsX
PubMed ID25530949
PubMed Central IDPMC4268772
Grant ListR01 DE018468 / DE / NIDCR NIH HHS / United States