본 연구는 갈근 추출물의 항산화 활성 및 멜라닌세포 효과를 평가하기 위하여 총 폴리페놀 함량, 총 플라보노이드 함량, DPPH radical 소거 활성을 통하여 항산화 활성을 살펴보고, B16F10 melanoma 세포에 대한 세포 독성 및 멜라닌 생합성 억제능 효과를 측정하였다. 연구 결과 B16F10 melanoma 세포에 대해 독성을 나타내지 않았으며, B16F10 melanoma 세포에 α-MSH로 멜라닌 생성 을 유도한 후 멜라닌 생합성 억제능을 측정한 결과 멜라닌의 생성 증가가 농도 의존적으로 억제되는 것 을 확인하였다. 항산화 활성에 대한 결과로는, 갈근 추출물은 폴리페놀과 플라보노이드의 함량이 높아 추출물의 농도가 증가함에 따라 DPPH radical 소거 활성이 증가되는 것을 확인하였다. 이와 같은 결과 를 통하여 갈근 추출물이 항산화 활성과 멜라닌세포 대한 멜라닌생성억제 효과가 뛰어나고 피부 세포에 대한 독성이 낮으며, 피부의 멜라닌 세포에 대한 안전성이 확인됨에 따라 화장품 소재로서의 가능성을 확인하였다.

This study was conducted to investigate the effect of ultraviolet light (UV-B) on plant growth and petal antioxidants of edible flower pansy (Viola × wittrochiana ‘Rose’ and ‘Yellow’, V. cornuta ‘Purple’). The plants were grown under white LED of 100 μmol·m-2·s-1 PPFD and treated by UV-B of 10, 20 and 30 minutes per day: UVB-10, UVB-20, and UVB-30 respectively. The plant growth was significantly inhibited as longer UV-B radiation exposure, even ‘Rose’ could not f lower under UVB-30. NPQ increase was observed in all cultivars with longer UV-B irradiation exposure. Also, anthocyanin in ‘purple’ and ‘Rose’ or carotenoid in ‘Yellow’ increased in the petals as longer UV-B radiation exposure. Unexpectedly the contents of total phenol and DPPH did not show the significance in UV-B treatments. In conclusion, the applicable UVB exposure to edible pansy in order to more accumulate antioxidants in petals would be in 20 minutes per day.

In this study, we evaluated anti-oxidation and whitening effects of Ligularia stenocephala extract for use as the cosmeceuticals. L. stenocephala was extracted by three different solvents which was n-Hexane, ethyl acetate, H2O. The free radical (1,l-diphenyl-2-picrylhydrazyl, DPPH) scavenging activity of extract of L. stenocephala was in the order: ethyl acetate fraction of leaf (IC50 value of 10.512ug/mL) 〉 ethyl acetate fraction of stem (IC50 value of 31.877ug/mL) 〉 H2O fraction of leaf (IC50 value of 129.194ug/mL). Reactive oxygen species (ROS) scavenging activity of extract of L. stenocephala was in the order: ethyl acetate fraction of leaf (IC50 value of 0.230mg/mL) 〉 ethyl acetate fraction of stem (IC50 value of 0.528mg/mL) 〉 H2O fraction of leaf (IC50 value of 0.799mg/mL). Tyrosinase inhibition activity of L. stenocephala extracts was reduced 29.477% on ethyl acetate fraction of leaf, 13.583% on ethyl acetate fraction of stems. Therefore, L. stenocephala extracts may be useful as a new antioxidant and whitening agent to inhibit melanogenesis.