Antioxidant activity of extracts from Schinus molle L . and Gleditsia triacanthos L .

Methanolic and chloroform extracts obtained from various parts of Schinus molle and Gleditsia triacanthos were evaluated by DPPH radical scavenging assay. The methanolic extracts from S. molle showed scavenging activity ranging from 35.97±1.02 to 83.38±2.74%, while the chloroform seed extract showed relatively weak scavenging activity ranging from 8.20±1.02 to 68.82±3.17%. The IC50 values of S. molle methanolic leaves extract, S. molle methanolic stem-bark extract and S. molle chloroform seed extract (SMMELS, SMMESB and SMCHSD) were found to be 476.43, <250 and ~3000 μg mL -1 , respectively. The methanolic extracts from G. triacanthos showed scavenging activity ranging from 35.97±1.02 to 92.36±0.11%, while the chloroform seed extract showed relatively very weak scavenging activity ranging from 3.74±1.04 to 15.47±4.57%. The IC50 values for G. triacanthos methanolic leaves extract, G. triacanthos methanolic stem-bark extract, G. triacanthos methanolic thorns extract and G. triacanthos chloroform seed extract (GTMELS, GTMESB, GTMETS and GTCHSD) were found to be 452.32, 720.56, <250 and >3000 μg mL -1 , respectively. The positive controls, GAMEOH and GAETAC, showed an IC50 value <250 μg mL -1 each. From this study, we concluded that the extracts from these two medicinal plants, S. molle and G. triacanthos, showed promising antioxidant activity. Therefore, further investigations, such as bioactive guided isolation of pure compounds, antioxidant activity of pure compounds, application of these extracts or pure compounds in culinary, etc., are required.

Author(s) agree that this article remain permanently open access under the terms of the Creative Commons Attribution License 4.0 International License a tree that grows to 7 to 10 m height; it is native to South and Central America and has been cultivated in Southern African countries.The fruits (seeds) of S. molle are edible and they are about 5 mm diameter (Trevor et al., 2013).The seeds of S. molle are reddish pink and have a taste similar to pepper.It has been reported that S. molle has antibacterial, analgesic, cytotoxic, anti-inflammatory, antifungal, antiseptic, insecticidal, and antioxidant activities (Deveci et al., 2010;Diaz et al., 2008;Ferrero et al., 2006;Ruffa et al., 2002;Yueqin et al., 2003;Abir et al., 2016;Abderrahim et al., 2018;Bendaoud et al., 2010;Mohamed et al., 2016).
The species of Gleditsia triacanthos L. is a deciduous tree belonging to the Fabaceae family.G. triacanthos is also known by other names such as honey locust and thorny locust.G. triacanthos is native to Asia and North America (Benhamiche et al., 2016;Mohammed et al., 2014).G. triacanthos grows to 15 to 30 m height (Stubbendiek and Conard, 1989).The yellow flowers of G. triacanthos have strong pleasant smell.G. triacanthos has thorns which are single or branched and grow to 3 to 10 cm.The edible fruits of G. triacanthos are about 15 to 40 cm long and about 2.5 to 3.5 cm wide (Blair, 1990).GreenTech S.A. uses extract from seeds of G. triacanthos and has been sold in the name of Gleditschia as cosmetic product (Miguel et al., 2010).
Gleditsia species have been used for personal care and medicinal applications that include hair protection, local medicine for smallpox, skin diseases, whooping, measles, asthma and difficult labour in the Native American (Miyase et al., 2010).It has been reported that G. triacanthos has anti-inflammatory, analgesic, hepatoprotective, antimicrobial and antioxidant activities (Tahia et al., 2013;Mohammed et al., 2014;Miguel, 2010).
The antioxidant study of essential oils and extracts from S. molle and G. triacanthos were reported previously (Abir et al., 2016;Abderrahim et al., 2018;Bendaoud et al., 2010;Mohamed et al., 2016;Mohammed et al., 2014;Miguel, 2010).However, the scavenging activity of methanolic and chloroform extracts of various parts of S. molle and G. triacanthos has not been reported previously, particularly the plant species gathered from the Kingdom of Lesotho.Therefore, the aforementioned plant extracts were screened for their DPPH radical scavenging assay and the results thus obtained are reported.

Plant materials
The plant materials, S. molle and G. triacanthos, were collected from Botanical Garden, Roma Campus, National University of Lesotho.Both plant materials were collected in August 2017 and were identified by Mr. Moretloa Polaki, Lecturer, Department of Biology, Faculty of Science and Technology, National University of Lesotho.From S. molle, the following parts of plant materials were used for this study: leaves (596.744g), stem-bark (241.246g) and seeds (115.126g).From G. triacanthos, the following parts were used for this study: leaves (337.000g), stem-bark (247.271g), thorns (165.169g) and seeds (217.705g).A voucher specimen for each part of the plants is kept at Organic Chemistry Laboratory, Department of Chemistry and Chemical Technology, Faculty of Science and Technology, National University of Lesotho.The following labelling was used to represent various parts of plant materials: KMSMLS, KMSMSB and KMSMSD for leaves, stem-bark and seeds of S. molle, respectively; KMGTLS, KMGTSB, KMGTTS and KMGTSD for leaves, stem-bark, thorns and seeds of G. triacanthos, respectively.

Processing of materials
The plant materials were allowed to air dry at room temperature for two weeks.The air dried leaves and seeds of S. molle were ground into powder using a commercial blender (Waring Blender, Blender 80119, Model HGB2WT93, 240V AC, 50-80 Hz, 3.6 AMPs, Laboratory and Analytical Supplier).The air dried stem-bark of S. molle was chopped into small pieces and then crushed using a Woodworking Table Saw 250 mm machine (Serial Number: JFD1412109-13, Model Number: SAWLD001, Motor, 1500W, 220 V, 50 Hz, Blade Rising Range: 0-80 mm, Motor Speed: 4500 rpm, Max.Depth of Cutting (90° and 45°): 80 mm and 5 mm).The crushed materials were further ground into powder using the aforementioned Waring Blender.The same procedures mentioned were repeated to get powder from the air-dried leaves, seeds, thorns and stem-bark of G. triacanthos.

Preparation of plant extracts
The powdered leaves of S. molle were extracted first with methanol at room temperature for two days by shaking manually and occasionally.The solution was filtered using Whatman No.1 filter paper and the solvent methanol was removed using water bath and/or Buchi rota-vapour.The same procedure was repeated once again.Finally, the material was extracted with methanol at reflux condition for 5 h.All three filtrates were combined and 63.00 g of methanolic extract was obtained.The same procedure was followed for the powdered stem-bark of S. molle and 7.19 g of methanolic extract was obtained.The powdered seeds of S. molle was extracted first with chloroform with at room temperature by shaking manually and occasionally followed by at reflux condition for 5 h.The extracts were combined and 12.91 g of chloroform extract was obtained after removal of solvent using water bath and/or Buchi rota-vapour.The same methanolic extraction procedure was followed for leaves, stem-bark and thorns of G. triacanthos, respectively, 47.51, 8.44 and 7.51 g of methanolic extracts were obtained.Similarly, the same chloroform procedure was followed for seeds of G. triacanthos and 8.94 g of resinous chloroform extract was obtained after removal of solvent using water bath and/or Buchi rota-vapour.

DPPH radical scavenging assay and determination of IC50 values
DPPH radical scavenging activity of various extracts of S. molle and G. triacanthos was conducted according to the method described in the literature (Sasidharan et al., 2007) with slight modification.Briefly, stock solutions of methanolic extracts were prepared at a concentration of 3.0 mg of extract in 1 mL of 50% methanol (v/v).Further dilutions were made from these stock solutions such that solution was obtained with concentrations of 3000, 2000, 1000, 500 and 250 µL for each extract.50 µL of each one of them was mixed with 1 mL of 0.1 mM solution of DPPH in 50% methanol (v/v).The mixture without extract sample was used as blank and just spiked with 50 µL of 50% methanol (v/v).A stock solution of commercial antioxidant, gallic acid, of the same concentration in 50% methanol (v/v) was prepared and further dilutions were made as previously and served as positive control for methanolic extracts.Similarly, stock solutions of chloroform extracts were prepared at a concentration of 3.0 mg of extract in 1 mL of ethyl acetate.Further dilutions were made from these stock solutions such that extract solution was obtained with concentrations of 3000, 2000, 1000, 500 and 250 µL for each extract.50 µL of each one of them was mixed with 1 mL of 0.1 mM solution of DPPH in ethyl acetate.The mixture without extract sample was used as blank and just spiked with 50 µL of ethyl acetate.A stock solution of gallic acid of the same concentration in ethyl acetate was prepared and further dilutions were made as previously and served as positive control for chloroform extracts.The mixtures were incubated for 30 min and their optical density was measured at 517 nm.The IC50 values were calculated from graphs by plotting extract concentrations versus percentage inhibition of DPPH radical using Microsoft Excel.
The extract concentration that causes 50% reduction in the initial concentration of DPPH is defined as the IC50 value of extract which is important measure of potency for a given extract.Each experiment was carried out in triplicate and the averages of the three values were used to calculate IC50 values.Standard deviation was calculated for each concentration from the three values of the experiment.The ability to scavenge DPPH radical was calculated by Equation 1

Statistical analysis
Results were expressed as means of three determinations.One way analysis of variance (ANOVA) was used to compare means at the significance level p < 0.05.All analysis were performed by Microsoft Excel software., respectively.This result showed that SMMESB has comparable activity as that of positive control at low concentrations and at high concentrations; the scavenging , respectively.In this case, the positive control (GAETAC) showed 76.96±1.50,92.49±5.18,93.12±0.39,93.67±4.06 and 94.57±1.02% of scavenging activity at concentrations of 250, 500, 1000, 2000 and 3000 µg mL -1 , respectively.This result showed that SMCHSD exhibited very weak activity at low concentrations relative to positive control, GAETAC.However, at high concentrations such as 2000 and 3000 µg mL -1 , it showed higher scavenging activity of 63.40±2.69 and 68.82±3.17%,respectively.Among the three extracts (SMMELS, SMMESB and SMCHSD) from S. molle, SMMELS showed highest scavenging activity (refer to Table 1).

Conclusion
DPPH radical scavenging activity of methanolic and chloroform extracts obtained from various parts of two medicinal plants viz.S.molle and G. triacanthos collected from the Kingdom of Lesotho have been evaluated.The methanolic extracts from S. molle showed scavenging activity ranging from 35.97±1.02 to 83.38±2.74%,while the chloroform seed extract showed scavenging activity ranging from 8.20±1.02 to 68.82±3.17%.The methanolic extracts from G. triacanthos showed scavenging activity ranging from 35.97±1.02 to 92.36±0.11%,while the chloroform seed extract showed scavenging activity ranging from 3.74±1.04to 15.47±4.57%.From this study, it was concluded that the extracts from these two medicinal plants, S. molle and G. triacanthos, showed promising antioxidant activity.The IC 50 values of these extracts were also determined and found to be between <250 and 3000 µg mL -1 .

Table 1 .
The percentage radical scavenging activity of various extracts from S. molle and G. triacanthos at various concentrations.

Table 2 .
The IC50 values of various extracts of S. molle and G. triacanthos based on DPPH radical scavenging assay.