• Journal of Applied Biological Chemistry
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• 제62권4호
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• pp.399-406
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• 2019

현삼(Scrophularia buergeriana) 뿌리를 80% Methanol수용액으로 추출한 뒤, 감압 농축한 추출물을 EtOAc, n-BuOH과 H₂O층으로 계통 분획을 실시하였다. n-BuOH분획에 대하여 silica gel, octadecyl SiO₂ column chromatograph 및 중압분취(MPLC) 장비를 반복 실시하여 4종의 phenylethanoid glycoside 및 iridoid glycoside계의 화합물을 분리하였다. NMR 및 Mass데이터를 해석하여, harpagoside (1), angoroside C (2), aucubin (3) 및 acetoside (4)로 구조 동정하였다. 분리한 4종의 화합물에 대하여 HPLC 분석법을 이용하여 정량분석한 결과, 11.5 mg/g (1), 7.6 mg/g (2), 41.2 mg/g (3), 및 4.8 mg/g (4) 이 현삼 뿌리에 함유된 것을 확인하였다. 현삼으로부터 분리된 화합물 중 angoroside C 및 acetoside는 에탄올에 의해 저해된 세포 성장률을 검증한 결과, 간암세포종인 HepG2세포에 대해서 간세포를 보호하는 효과가 있음을 확인하였다.

• 신재생에너지
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• 제19권4호
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• pp.27-34
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• 2023

In this study, microalgal oil was extracted from Nannochloropsis oceanica cultured in an open raceway pond and converted into biodiesel using a solid acid catalyst. Microalgal oil was extracted from two types of microalgae with and without nitrogen starvation using the KOH-solvent extraction method and the fatty acid content and oil extraction yield from each microalgae were compared. The fatty acid content of N. oceanica was 184.8 mg/g cell under basic conditions, and the oil content increased to 340.1 mg/g under nitrogen starvation conditions. Oil extraction yields were 90.8 and 95.4% in the first extraction, and increased to 97.5 and 98.8% after the second extraction. Microalgal oil extracted by KOH-solvent extraction was yellow in color and had reduced viscosity due to chlorophyll removal. In biodiesel conversion using the catalyst SO₄^2-/HZSM-5, solvent-extracted oil showed a FAME content of 4.8%, while KOH-solvent-extracted oil showed a FAME content of 90.4%. Solid acid catalyst application has been made easier by removal of chlorophyll from microalgal oil. The FAME content increased to 96.6% upon distillation, and the oxidation stability increased to 11.07 h with addition of rapeseed biodiesel and 1,000 ppm butylated hydroxyanisole.

• 한국수산과학회지
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• 제34권2호
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• pp.114-118
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• 2001

저염창란젓갈 제조 공정에 시 숙성공정에 교반과정을 도입하여 숙성기간의 단축과 제품의 균일화를 시도하였다. 먼저 시험구의 경우에는 원료창란을 연속교반 염장한 후 생성된 유출수를 제거하고 $0\pm2^{\circ}C$에서 4시간마다 10rpm으로 10분간 교반숙성하였으며, 대조구의 경우는 정치염장한 후 유출수를 포함하여 $0\pm2^{\circ}C$에서 정치숙성하였다. 60일간 숙성시키면서 이들의 품질변화를 측정한 결과 숙성일수가 경과할수록 pH는 낮아졌으며, 숙성 60일째에는 초기 pH 7.0에서 $6.2\~6.3$ 정도로 떨어졌으며 시험구가 대조구 보다 대체로 낮은 값을 나타내었다. 또한 시험구의 경우 숙성 30일째에Brix는 27.4, VBN은 $54.3 mg\%$ , 아미노태질소는 $87.9 mg\%$를 나타내었는데 비하여 대조구는 경우 숙성 50일째 Brix는 27.1, VBN은 $57.8 mg\%$, 아미노태질소는 $96.6mg\%$를 나타내었다. 숙성 중 미생물 변화는 대조구의 경우 50일째 $1.9\times10^6CFU/g$, 시험구의 경우 30일째 $2.6\times10^6CFU/g$으로 최대로 증가한 후 서서히 감소하는 경향을 보였다. 또한 관능검사 평가 결과도 대조구의 경우 50일째, 시험구의 경우 30일째에 최고값을 나타내어 창란젓갈의 최적 숙성기간은 대조구의 경우 50일, 시험구의 경우 30일로, 교반숙성 시키는 경우가 정치숙성에 비해 20일정도 공정일수를 단축할 수 있었다.

• 한국가축번식학회지
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• 제19권3호
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• pp.227-234
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• 1995

본 연구는 1-세포기배의 glucose에 대한 노출이 상실배기 이후의 배발생에 미치는 영향을 검토하고자 실시되었다. hCG 주사 후 24~25시간 째에, F1hybrid(C57BL/6, ♀ $\times$CBA/N, ♂) 계통 생쥐를 도살하여 1-세포기배를 회수한 후 0.1% hyaluronidase로 처리하여 난구세포를 제거하였다. 1-세포기배는 hCG 주사 후 72시간째 다양한 농도의 glucose(5.5, 16.5, 27.5 및 38.5mM)에 1분 노출 후 glucose가 첨가되어 있거나 혹은 첨가되지 않은 CR1aa배양액에서 계속 배양함으로써 배발생을 유도하였다. 이 실험의 결과를 요약하면 다음과 같다. 1. M2 배양액에서 회수한 후 3mg/ml의 Fatty-acid free BSA가 첨가된 배양액에서 배양한 경우 27.5%의 확장배반포까지의 배발생율과 16.6%의 탈출 배반포까지의 배발생율을 나타낸 반면, TL HEPES 배양액에서 회수한 경우는 전혀 상실배기 이후의 배발생이 나타나지 않았다. 2. hCG 주사 후 72시간째에 단 1분간의 27.5mM glucose에 대한 노출만으로도 68.8% (CR1aa＋BSA)와 77.1%(CR1aa＋FBS)의 확장배반포까지의 발생을 유도할 수 있었다. 그러나 1분 노출과 이후 계속되는 노출간에는 배발생에 있어서 유의차는 인정되지 않았다. 3. hCG 주사 후 72시간째에 5.5, 16.5, 27.5 및 38.5mM의 glucose 첨가에 따른 확장 배반포까지의 배발생율은 45.7~61.5%로 각 처리군의 유의차는 없었으며, 따라서 고농도의 glucose 첨가에 따른 저해효과는 확인할 수 없었다.

• 대한의생명과학회지
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• 제8권4호
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• pp.229-234
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• 2002

Chlorella is rich in chlorella growth factor (CGF). A review of the literature has described that CGF improves the capability of a Th1-based immunity, anticancer, antioxidant antibacterial activity, growth promotion, wound healing and so on, but has not studied the effect for the metabolism and the proliferation of human skin keratinocyte. The aim of this study was to examine the effect of metabolism and the proliferation of human skin keratinocyte in vitro. CGF was extracted with an autoclaving method which is a modified hot-water extraction method from dried chlorella and conformed by means of absorbance 0.22 at 260 nm. We have measured the extracellular acidification rate (ECAR) of the CGF by Cytosensor$^{\circledR}$ Microphysiometer and evaluated responsiveness depending upon the dosage on the HaCaT cell. The ECAR for the concentrations of 0.15, 1.5, 15, 150 $\mu\textrm{g}$/ml of CGF increased as a 103.6, 128.2, 149.0 and 423.9%, respectively compared to control (0.0 $\mu\textrm{g}$/ml, 100% ECAR). The ECAR for ErbBl tyrosine kinase inhibited by 4-anilinoquinazolines, $C_{16}$H$_{14}$BrN$_3$O$_2$.HCl on tile HaCaT cells with the amounts of 10 $\mu\textrm{g}$/ml of the CCF compared with 100 $\mu\textrm{g}$/ml of rhEGF. The conclusion of the study is that CGF might increase human epidermal keratinocyte proliferation through the interaction between the epidermal growth factor receptor and itself.

• Journal of Microbiology
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• 제34권1호
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• pp.37-37
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• 1996

The internal regions of nuclear small subunit rRNA from 6 plaeurotus species and 5 Pleurotus ostreatus strains were amplified by PCR and sequenced. The DNA sequences of 8 Pleurotus strains (P. ostreatus NFFA2, NFFA4501, NFFA4001, KFFA4001, KFCC11635, P florida, P. florida, P. sajor-cuju, P. pulmonarius, and P. spodoleucus) were idential, but P. cornucopiae differed from them in two bases out of 605 bases. However, p[hylogenetic analysis of the sequences by DNA-distance matrix and UPGMA methods showed that P. ostreatus NFFA2m1 and NFFA2m2, known as mutants of P. ostreatus NFFA2, belonged to anther group of Basidiomycotina, which is close to the genus Auricularia. The difference of the SSU rDNA sequences of P. cornucopiae from other Pleurotus species tested corresponds to the difference of mitochondrial plasmid type present in Pleurotus species as observed by Kim et al. (1993, Korean J. Microbiol. 31, 141-147).ishement of silencing at the HMR/hsp82 locus can occur in G1-arrested cells. Cell cycle arrest at G1 phase was achieved by treatment of early log a cell cultures with .alpha.-factor mating pheromone, which induces G1 arrest. The result suggests that passage through S phase (and therefore DNA replication) is nor required for re-establishing silencer-mediated repression at the HMNRa/HSP82 locus. Finally, to test whether de nono protein synthesis is required for re-establishment of silencer-mediated repression, cells were pretreated with cycloheximide (500 /.mu.g/ml) 120 min. It was apparent that inhibiting protein synthesis delays, but does not prevent, re-establishment of silencer-mediated repression. Altogether, these results indicate that re-establishment of silencer-mediated repression is not dependent on the DNA replication and has no requirement for protein synthesis.

• Journal of the Korean Association of Oral and Maxillofacial Surgeons
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• 제32권4호
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• pp.295-307
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• 2006

Styela clava, called non-native tunicate or sea squirt, is habitat which include bays and harbors in Korea and several sites in the sea faced world. We fabricate cellulose membrane nerve conduit (CMNC) from this native sea squirt skin, and evaluate the capacity of promoting peripheral nerve regeneration in the rat sciatic nerve defect model. After processing the pure cellulose membrane from the sea squirt skin as we already published before, CMNC was designed as a non-tubular sheet with 14 mm length and 4 mm width. Total eleven male Spraque-Dawley rats (12 weeks, weighing 250 to 300g) were divided into sham group (n=2), silicone tube grafted control group (n=3) and experimental group (n=6). Each CMNC grafted nerve was evaluated after 4, 8 and 12 weeks in the experimental group, and after 12 weeks, sciatic function was evaluated with sciatic function index (SFI) and gait analysis, and histomorphology of nerve conduit and the innervated tissues of sciatic nerve were all examined using image analyzer and electromicroscopic methods in the all groups. The regenerated axon and nerve sheath were found only in the inner surface of the CMNC after 4 weeks and became more thicker after 8 and 12 weeks. In the TEM study, CMNC grafted group showed more abundant organized myelinated nerve fibers with thickened extracellular matrix than silicone conduit grafted group after 12 weeks. The sciatic function index (SFI) and ankle stance angle (ASA) in the functional evaluation were $-47.2{\pm}3.9$, $35.5^{\circ}{\pm}4.9^{\circ}$ in CMNC grafted group (n=2) and $-80.4{\pm}7.4$, $29.2^{\circ}{\pm}5.3^{\circ}$ in silicone conduit grafted group (n=3), respectively. And the myelinated axon was 41.59% in CMNC group and 9.51% in silicone conduit group to the sham group. The development of a bioactive CMNC to replace autogenous nerve grafts offers a potential and available approach to improved peripheral nerve regeneration. As we already published before, small peptide fragment derived from the basement membrane matrix proteins of squirt skin, which is a kind of anchoring protein composed of glycocalyx, induced the effective axonal regeneration with rapid growth of Schwann cells beneath the inner surface of CMNC. So the possibilities of clinical application as a peripheral nerve regeneration will be able to be suggested.

• Journal of Korean Neurosurgical Society
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• 제64권5호
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• pp.705-715
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• 2021

Objective : Through our previous clinical trials, the demonstrated therapeutic effects of MSC in chronic spinal cord injury (SCI) were found to be not sufficient. Therefore, the need to develop stem cell agent with enhanced efficacy is increased. We transplanted enhanced Wnt3-asecreting human mesenchymal stem cells (hMSC) into injured spines at 6 weeks after SCI to improve axonal regeneration in a rat model of chronic SCI. We hypothesized that enhanced Wnt3a protein expression could augment neuro-regeneration after SCI. Methods : Thirty-six Sprague-Dawley rats were injured using an Infinite Horizon (IH) impactor at the T9-10 vertebrae and separated into five groups : 1) phosphate-buffered saline injection (injury only group, n=7); 2) hMSC transplantation (MSC, n=7); 3) hMSC transfected with pLenti vector (without Wnt3a gene) transplantation (pLenti-MSC, n=7); 4) hMSC transfected with Wnt3a gene transplantation (Wnt3a-MSC, n=7); and 5) hMSC transfected with enhanced Wnt3a gene (1.7 fold Wnt3a mRNA expression) transplantation (1.7 Wnt3a-MSC, n=8). Six weeks after SCI, each 5×10⁵ cells/15 µL at 2 points were injected using stereotactic and microsyringe pump. To evaluate functional recovery from SCI, rats underwent Basso-Beattie-Bresnahan (BBB) locomotor test on the first, second, and third days post-injury and then weekly for 14 weeks. Axonal regeneration was assessed using growth-associated protein 43 (GAP43), microtubule-associated protein 2 (MAP2), and neurofilament (NF) immunostaining. Results : Fourteen weeks after injury (8 weeks after transplantation), BBB score of the 1.7 Wnt3a-MSC group (15.0±0.28) was significantly higher than that of the injury only (10.0±0.48), MSC (12.57±0.48), pLenti-MSC (12.42±0.48), and Wnt3a-MSC (13.71±0.61) groups (p<0.05). Immunostaining revealed increased expression of axonal regeneration markers GAP43, MAP2, and NF in the Wnt3a-MSC and 1.7 Wnt3a-MSC groups. Conclusion : Our results showed that enhanced gene expression of Wnt3a in hMSC can potentiate axonal regeneration and improve functional recovery in a rat model of chronic SCI.

• 한국수산과학회지
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• 제29권2호
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• pp.230-237
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• 1996

본 연구는 살수여상공법을 양어장 순환수 처리 장치로 설치하여 유기물질 제거 효율, 암모니아 제거효율, 동력학적 상수, 슬러지 생산량과 산소소요량 등의 최적 운전방법을 도출하였다. 유기물질 부하율이 $0.500\~0.082kg\;COD/m^3/day$에서 $66.4\~81.2\%$의 SCOD 제거 효율과 $74.5\~84.0\%$의 SBOD 제거 효율을 보였다. 암모니아 부하율이 $0.271\~0.044kg\;NH_4^+-N/M^3/day$에서 $43.7\~61.8\%$ 의 암모니아성 질소 제거 효율을 보였으며 암모니아 제거량은 $27.2\~119.5mg\;NH_4^+-N/L/day$로 나타났다. Eckenfelder 식에 의해 구한 K, n값은 각각 $0.168\;min^{-1}$과, 0.132로 나타났으며 총 생성된 슬러지 생산량은 0.233g VSS/day로 kg BOD 제거량당 생성되는 슬러지 생산량은 0.572 kg VSS/kg $BOD_{rem}$로 나타났다. 산소소요량은 3.89mg $O_2/L/hr$로 수리학적부하가 $6.712\~40.341\;m^3/m^2/day$에서 $1.33\~7.22\;mg\;O_2/L/hr$로 수리학적 부하가 증가할수록 산소소요량이 증가하였으며 미생물당 산소소모율은 1.08kg $O_2/kg$ VSS로 나타났다.

• 한국동물번식학회:학술대회논문집
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• 한국동물번식학회 2001년도 춘계학술발표대회
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• pp.22-22
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• 2001

To produce reconstituted rabbit embryos with fetal fibroblasts, the present study was evaluated the efficiencies of the different fusion and activation conditions as assessments of subsequent development and chromosome in the embryos. New Zealand White rabbits were used throughout the study. Fetal fibroblasts collected from 22-d of fetuses were cultured in DMEM ＋ 10% FBS in 5% $CO_2$ in air. The culture was maintained for 10 passages. In every passage half of cell suspension were kept In frozen. From rabbits treated with FSH in 30% PVP solution and hCG, oocytes were surgically collected from oviducts at 14 h post-hCG injection and stripped off their cumulus cells by re-pipetting in a 300 IU hyaluronidase solution. Oocytes with an extruded first polar body and dense cytoplasm were enucleated by micromanipulation in Ham's F-10 medium＋7.5 g/$m\ell$ cytochalasin B. Euncleation was confirmed under a fluorescence microscope after staining with 5 g/$m\ell$ bisbenzimide for 2 min. Each enucleated oocyte was injected with a fetal fibroblast into a perivitelline space. Reconstructed eggs were compared fusion rates either at 2.0 ㎸/cm or 1.6 ㎸/cm(60 sec, double pulses). After fusion, all eggs were activated with the combination of 5 M ionomycin (5 min) and 10 g/$m\ell$ cycloheximide (CHX, 3h), and cultured in CRlaa medium and transferred into TCM199＋10% FBS on day 3. Although there was not significantly differ in fusion rate between treatments (60%, 2.0 ㎸/cm vs. 79.4%, 1.6 ㎸/cm), none of them in the eggs fused with 2.0 ㎸/cm developed to blastocyst. In comparison of development and chromosome status between different activation treatments (Group 1; 5 M ionomycin/10 g/$m\ell$ CHX, Group 2; 5 M ionomycin/5 g/$m\ell$ CHX ＋ 2 mM DMAP after fusion with 1.6 ㎸/cm), there were not differ in cleavage and development rates (67.3% and 28.9% in Group 1; 67% and 33% in Group 2). All out of 8 embryos evaluated in Group 1 appeared a normal diploid chromosome sets and mean number of cells (Mean SEM) on day 4.5 of culture was 141.5 23.15 (n=8). It can be concluded that the use of cycloheximide has not happened in chromosome abnormalities, and fetal fibroblasts can be used for cloning in rabbit.