Affiliation:
1. Faculty of Medicine and Health Science, UIN Alauddin Makassar, Makassar, Indonesia.
2. Master of Islamic Education Management, UIN Alauddin Makassar, Makassar, Indonesia.
3. National Agency of Drug and Food Control, Makassar, Indonesia.
4. Department of Pharmacognosy, Faculty of Biomedical and Health Science at Hiroshima University, Japan.
Abstract
Cancer can usually develop due to exposure to sunlight. UV radiation from sunlight is known to damage DNA and is bad for the skin. Skin P stem cell carcinogenesis is caused by UV-A rays that penetrate deep into the dermis layer. UV-B damages cell DNA by being absorbed by proteins in the epidermis. Chromolaena odorata was extracted using methanol solvent, then partitioned into 5 solutions in the form of n-Hexane, Ethyl Acetate, Acetonitrate, n-Buthanol, and Ethanol. The five extracts obtained were tested with Human Epidermal Keratinocyte cells using the bioassay method. Results obtained from the microplate reader after incubation. Each extract was divided into three concentrations, it is 100, 50, 20(µg/mL). Then in the positive control (Etoposide), it was divided into four concentrations, 100, 50, 20, 10(µg/mL). After being analyzed with the results of the microplate reader, the IC50 of Chromolaena odorata was 48% in the ethyl acetate extract with a concentration of 100µg/mL. HaCaT cell proliferation was determined at indicated intervals using the MTT colorimetric assay. This assay was based on the ability of live cell succinate dehydrogenase to reduce the yellow salt MTT (3-(4,5-dimethylthiazol-2-yl-2,5-diphenyltetrazolium bromide)) (Sigma-Aldrich, St. Louis, MO, USA) to insoluble purple-blue formazan precipitate. Experiments were carried out on 96-well plates containing a final volume of 100µl of medium/well.