DPPH Antioxidant Capacity Assay

The DPPH method was performed as described by other authors [31 (link),32 (link)], with modifications. First, a 0.238 mg/mL DPPH stock was prepared in methanol and maintained at 4 °C. Before each batch, a working solution (0.048 mg/mL) was prepared by diluting the DPPH stock (1 in 5). For the analysis, 0.5 mL of the DPPH working solution was added to 0.5 mL of methanol diluted extract or standard. The solution was homogenized and left in the dark for 30 min at room temperature. Sample blanks were prepared by mixing 0.5 mL of the extract with 0.5 mL of methanol to eliminate the extract color interference. The absorbances were read at 520 nm (Genesys 150 UV-Vis, Thermo Fisher Scientific, Waltham, MA, USA) and compared with a Trolox curve (2.5–8 mg/L). All analyses were performed in duplicate. Results were expressed as μmol of Trolox equivalents (μmol TE) per g of dry seaweed and g of dry extract.

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Erpel F., Mariotti-Celis M.S., Parada J., Pedreschi F, & Pérez-Correa J.R. (2021). Pressurized Hot Liquid Extraction with 15% v/v Glycerol-Water as An Effective Environment-Friendly Process to Obtain Durvillaea incurvata and Lessonia spicata Phlorotannin Extracts with Antioxidant and Antihyperglycemic Potential. Antioxidants, 10(7), 1105.

Publication 2021

Genesys 150 UV-Vis

Methanol Trolox

Corresponding Organization : Pontificia Universidad Católica de Chile

Other organizations : Finis Terrae University, Austral University of Chile

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Variable analysis

independent variables

Concentration of DPPH stock solution
Dilution of DPPH stock solution to prepare working solution
Volume of DPPH working solution added to extract or standard
Volume of methanol added to extract or standard

dependent variables

Absorbance at 520 nm
Trolox equivalents (μmol TE) per g of dry seaweed
Trolox equivalents (μmol TE) per g of dry extract

control variables

Temperature (4 °C for DPPH stock, room temperature for analysis)
Incubation time (30 min)
Spectrophotometer used (Genesys 150 UV-Vis, Thermo Fisher Scientific)

positive control

Trolox standard (2.5–8 mg/L)

negative control

Sample blanks (0.5 mL extract + 0.5 mL methanol)

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