구조물의 손상 진단을 위해 측정 가속도 데이터를 사용한 비선형 시간영역 SI 알고리듬을 개발하였다. 구조물의 비선형 거동을 고려하기 위하여 측정 가속도 증분과 해석에 의한 가속도 증분의 차이로 출력오차를 정의하고, 구속 비선형 최적화 문제를 풀어 최적 구조변수를 구하였다. 개발된 알고리듬은 시간에 따라 변하는 강성도와 감쇠 변수를 추정하도록 하였다. 구조물의 비선형 거동에 의한 복원력은 추정된 시간에 따라 변하는 구조변수와 Newmark-\beta법으로 계산한 변위를 사용하여 복원하였으며, 복원 과정에서 비탄성 거동에 대한 어떤 모델도 사전에 설정하지 않았다. 개발한 알고리듬에서는 측정오차와 공간 및 상태에 대한 불완전 측정의 경우를 고려하였다. 개발한 알고리듬을 검증하기 위하여 3층 전단건물에 대한 수치 모의시험과 실내 모형실험을 통한 연구를 수행하였다.

This study showed the increase of antitumor activities of water soluble E. sinica extract by nano-encapsulation process with lecithin. Five groups of lecithin only group (LO), lecithin nano-encapsulated E. sinica group (LE), E. sinica only group (EO), one negative control group (NCO) and positive control group (PCO) were set for several anticancer experiment and fed into Sarcoma-180 injected mice. The cytotoxicity of LE on the human normal kidney cell (HEK293) showed 14.8% lower than 19.2% of EO and 18.4% of LO. Growth of human liver carcinoma cell and human stomach carcinoma cell as representative of digestive system in vitro was inhibited up to about 85.1% and 87.3%, in adding 1.0 mg/ml of LE, which values 15% higher than that from conventional EO. The survival rates of each mice group were 40%, 63%, 48%, 33% and 100%, respectively after 40 days of injecting Sarcoma-180. The increment of their body weights of the extract feeding groups was suppressed down to 10~15%, compared to the negative control. The nano-particles also reduced the hypertrophy of the internal organs such as spleen and liver down to 15~20%, compared to those as the other groups. Among them, LE effectively reduced the size of tumor form to 20%. From these results, in vitro and in vivo antitumor activities of E. sinica could be enhanced by using nano-encapsulation process with lecithin because of better permeation into the cancer cells by confocal observations.

Hepatoprotective and antioxidant activities of Acer mono and A. okamotoanum were compared after beingextracted by low temperature and high pressure (LTHP) at 20 MPa and 60℃ for 15 minutes. Extraction yield of both A.mono and A. okamotoanum was increased about 40~43% by this extraction process. On scavenging activities, the bark of A.okamotoanum from this extraction process showed the highest activity as about 97%. This value was higher than that fromconventional water extraction and A. mono extracts. Both of A. mono and A. okamotoanum showed high ability on nitritescavenging, but decreasing tendency according to increasing of pH. On SOD-like test, A. okamotoanum had the highestactivity as 46.28% at 1.0㎎/㎖ concentration. A. okamotoanum extracted by LTHP also showed the highest activity as197.38% in adding 1.0㎎/㎖ concentration. Generally, the extracts from low temperature and high pressure extraction pro-cess are higher hepatoprotective and antioxidant activities than that from conventional water extraction. It can concludethat the bark of A. okamotoanum has better biological activities than other parts of A. mo

Sunlight, and in particular its UV component, is the major environmental trigger that underlies the major signs of human skin and skin cancer in general. Therefore, this study was carried out to investigate the UV protection effects of R. coreanus. R. coreanus was extracted by ultra high pressure extraction process at 500 MPa and 30℃ for 5 and 15 minutes. The cytotoxicity of the extracts extracted by ultra high pressure process on human dermal fibroblast cell CCD-986sk, human kidney normal cell HEK293, and human lung normal cell HEL299 was measured as 17.5%, 16.5% and 14.0%, respectively in adding 1.0 mg/ml of the samples, which was much lower than that from conventional water extraction method at 100℃ as 23.2%, 22.5%, 21.2%. The secretion of NO- from macrophage showed 15.9 μM on the R. coreanus extract from this process, which was higher than others. Prostaglandin E2 (PGE2) production from UV-induced human skin cells was also greatly decreased down to 510 pg/ml, compared to the control. From the results, we considered that the extracts from R. coreanus could be potent natural materials for skin anti-inflammation agent, and could be used as a potential anti-aging for the photo-damaged skin.

The low quality fresh ginseng was fermented by Phelinus linteus or Hericium erinaceum mycelium. This fermented ginseng was extracted by water at 100℃ or water with ultrasonification at 60℃. Total phenolic compounds was improved by ultrasonification extraction process, compare to conventional water extraction. All extracts enhanced the growth of human B and T cells, showing 2.68 times and 3.43 times higher, respectively, than the control. The secretion of TNF-α and IL-6 from human immune cells was enhanced as 3.53×10-4 pg/cell, 3.40×10-4 pg/cell by adding H. erinaceum mycelium fermented ginseng. H. erinaceum mycelium fermented ginseng yielded higher nitric oxide production from macrophage than Lipopolysaccharides (LPS). The cytotoxicity on human normal kidney cell (HEK293) was as low as 20.5% in adding the maximum concentration of 1.0 mg/ml of fermented ginseng. Generally, the extracts from ultrasonification extraction process showed 10% lower toxicity than that by conventional process. H. erinaceum mycelium fermented ginseng had the highest anticancer activity on human lung cancer and stomach cancer cells as 69.33% and 75.32%, respectively at 1.0 mg/ml. It can be concluded that, in general, H. erinaceum mycelium fermented ginseng has relatively better immune and anticancer activities than P. linteus fermented ginseng. Expecially, the extracts treated with ultrasonification had higher activities than that from conventional extraction process.

This study was performed to compare the effects of immuno-modulating activities of Rhodiola sachalinensis A. Bor. fractionized by consecutive solvent separation. The Cytotoxicity of all fractionized extracts on human kidney cell (HEK293) was lower than crude extracts. Generally, the butanol and chloroform extracts showed less cytotoxicity on about 10.07% and 9.67% than the crude extracts. For human immune B and T cell growth, chloroform fraction showed the highest cell growth compared to the control. The secretion of cytokines (IL-6, TNF-α) on human B and T cells were increased by adding chloroform extracts. Also, NK cell growth was significantly improved up to nearly 30% by adding the supernatant of B cell medium grown with the chloroform fraction. It was also found that chloroform fraction could yield higher nitric oxide production from macrophage than untreated control cells. Differentiation of HL-60 cells was increased up to 131.9% after treatment with chloroform fraction extracts, compared to the control. These results indicate that the chloroform fraction of R. sachalinensis have high immune activation activity than others fractions and the crude extracts, implying that this chloroform fractions could be used a new functional material.

This study was performed to compare alcohol fermentation ability and saccharification of potatoes and sweet potatoes. Cooperated with ultrasonification process is not contain pass through cook process, but contain process using ulrasonification instead cook process. In result of sugar contents measurements sweet potato and potato was highest of a family at 6 hours fermentation, and it showed the highest sugar contents as each 11.5 brix, 10.4 brix. In result of alcohol contents measurements of sweet potato and potato, highest of a family in 4 days, and it showed th highest alcohol contents as each 8.2, 6.0%. Finally complex enzymes II process revealed similar activities like cook process.

This study was performed to enhance anticancer activities of E. sinica, and A. gigas by ultra high pressure extraction process. The cytotoxicity of E. sinica and A. gigas on human kidney cell (HEK293) was as low as 24.94% and 25.3% in adding 1.0 mg/ml of the sample extracted at 500 Mpa for 15 minute. Generally, the inhibition of cancer cell growth on A549 and MCF-7 was increased over 20% in the ultra high pressure samples, compared to the conventional extraction process. Under the extracts from ultra high pressure process showed not only the strongest anticancer activities, but also had better stability than normal extracts. It was also found that the extracts of A. gigas reduced the hypertrophy of the internal organs, such as adrenal and spleen caused stresses in several mouse models.

This study was performed to improve antioxidant activities and skin-whitening effects of Rubus coreanus Miquel extracts by nano-encapsulation. R. coreanus was extracted at 60℃ and encapsulated by lecithin and gelagine. Nano-encapsulated extracts showed highest free radical scavengering effect as 97.62% in adding sample (500 μg/ml), compared to the extracts from conventional processes. It was showed strong inhibition effect on melanin production test by Clone M-3 cells as 55.23%. High inhibitory potency on tyrosinase was also measured as 155.8% by adding nano-sample of 1 mg/ml. The improvement of biological activity was demonstrated by real time confocal microscope. We could consider that the water soluble extracts of R. coreanus could be definitely enhanced by nano-encapsulated as a potent natural resources for antioxidant and skin-whitening agent.

This study was performed to investigate improving immune activities of natural water-soluble sulforaphane extracted from Brassica oleracea var. italica by nano encapsulation process. The nanoparticles of the sulforaphane extracted with ultrasonification process at 60℃ promoted human B and T cell growth, about 7~35% compared to the control. The secretion of IL-6 and TNF-α from T cells were also enhanced as 2.6×10-4pg/cell and 2.1×10-4 pg/cell, respectively, by the adding nano samples. NK cell activation was improved about 8%, compare to the control in adding cultured medium of T cell added nano samples. It was also found that sulforaphane extracted from B. oleracea var. italica had highly inhibitory activity on hyaluronidase as IC50 about 200 μg/ml. It can be concluded that natural water-soluble sulforaphane samples by nano-encapsulation, each size is 200 nm, extracted from B. oleracea var. italica has high immune activities through higher efficiency of bio-activation than conventional extracts.

본 연구는 병풀의 초음파 추출 시 용매에 따른 면역활성 증진 효과를 탐색하고자 수행되었다, 각 추출공정의 수율 비교에서 초음파 공정을 병행한 60℃ 에탄올 추출이 일반 100℃ 물 추출에 비해 15% 높은 수율을 나타냈으며, 에탄올을 용매로 한 추출이 동일한 조건의 물 추출에 비해 모두 높은 수율을 나타냈다. 이는 용매의 극성과 용출되는 병풀 내 성분의 극성에 기인하는 것으로 사료된다. 인간 정상 섬유아세포인 CCD-986sk를 이용한 세포독성 측정을 통해 모든 병풀 추출물이 32% 이하의 세포독성을 나타냈다. 인간 면역 B, T세포의 생육도 측정에서 초음파를 병행한 60℃ 에탄올 추출물이 무첨가 대조구에 비해 10%의 증진 효과를 나타내었으며, 면역세포의 cytokine 분비량 측정에서도 IL-6, TNF-α의 분비를 각각 4.86 × 10-4 pg/cell과 5.73 × 10-4 pg/cell로 나타내 증진 효과를 나타냈다. 또한, 초음파 병행 에탄올 시료를 첨가한 면역 T세포의 분비물에 의한 NK 세포 활성에서도 10%의 생육증진효과를 나타내었다. 이를 통해 병풀의 에탄올 추출물이 면역 활성을 가지고 있으며 초음파 공정을 통해 활성의 증진이 나타날 수 있음을 확인하였다. 이는 에탄올 용매를 통해 병풀 유용성분의 용출이 증진되고, 초음파 공정을 통해 병풀 유용 성분의 수율 향상 및 유용성분의 변화, 신규물질 용출 등이 일어나기 때문인 것으로 사료된다.