• 한국의학물리학회지:의학물리
• /
• 제11권2호
• /
• pp.157-165
• /
• 2000

목적: 방사선조사에 의해 형성된 DNA 손상정도가 산소에 의해 변화되는 추세을 이론적 모델을 이용하여 평가 및 분석하였다. 방법 및 대상: Water radiolysis(물의 방사성분해)시 생성되는 유리기 들간의 반응, 손상된 DNA의 형성, 손상의 복구, 및 산소에 의한 손상의 고정들을 시간 미분 방정식을 이용하여 표현하였다. 문헌에 나와 있는 반응상수(rate constants)들은 그대로 사용되었고 알려지지 않은 상수들은 실험에서 얻어진 데이터에서 얻은 곡선을 대입하여 얻었다. 화학반응상수 변화와 산소농도변화에 따른 세포 생존도를 구하였다. 모델을 통해 얻어진 세포 생존도와 방사선량의 상관관계를 세포 생존곡선으로 표시하였다. 산소에 의한 손상의 fixation(고착화)과정과 산소농도가 세포생존에 미치는 영향을 분석하여 보았다. 산소가 세포생존에 미치는 정도를 정량화 하기 위하여 산소증가효과비(Oxygen Ehhancement Ratio, OER)를 계산하여 실험치와 이론치를 비교하였다. 결과: 산소에 대한 민감성 연구에서 DNA생존도는 산소의 농도와 화학반응속도상수에 영향을 받았다. 산소의 농도가 0에서 1.0 $\times$ $10^{7}$ 으로 변화할 때 세포 생존도에는 변화가 없었다. 그러나 1.0 x $10^{7}$ 에서 1.0 $\times$ $10^{10}$ 변화할 경우 세포의 생존률이 감소하였다. 모의연구에서 얻은 OER치는 10% 세포생존시에는 2.32, 45% 세포생존시에는 1.9 이었다. 결론: 산소의 감수성 연구에서 보여주듯이 방정식을 이용하여 얻어진 새포생존곡선은 실험에서 얻어진 세포생존곡선을 재연할 수 있었다 또한 방사선조사시 생성되는 손상된 세포의 양은 산소 반응상수가 가장 크고 산소농도가 증가되는 경우에 증가됨을 알수있었다. 모의연구에서 얻은 산소증가효과비는 세포생존이 low level인 경우 높은 일치성을 보여 주었다 따라서 본 연구는 세포살해시 산소의 효과를 semi-empirical 모델을 사용하여 예측할수 있다는 것을 보여주고 있다.

• Journal of Chest Surgery
• /
• 제32권11호
• /
• pp.978-983
• /
• 1999

Background: Complement activation with transpulmonary leukocyte sequestration is considered a main mediator leading to ischemia-reperfusion lung(I-R) injury. We studied the role of leukocytes in the formation of I-R injury in ovine cardiopulmonary bypass(CPB) model with a membrane oxygenator. Material and Method: Five sheep were used. CPB circuitry consisted of a roller pump(American Optical Corp., Greenwich, CT, USA) and a membrane oxygenator(UNIVOX-IC, Bentley, Baxter Health Corp, Irvine, CA, USA). The CPB time was fixed at 120 min. Ten minutes after the start of CPB, total CPB was established. Thereafter a total CPB of 100 min was performed, followed by another 10 min of partial CPB. The CPB was discontinued and the animals were fully recovered. For measuring left and right atrial leukocyte counts, blood samples were taken before thoracotomy, 5 min and 109 in after the start of CPB, and 30 min and 120 min after weaning. C3a was measured before thoracotomy, 109 min after the start of CPB, and 30 min and 120 min after weaning. Plasma malondialdehyde(MDA) was checked before thoracotomy, 109 min after the start of CPB, and 30 min after weaning. One to two grams of lung tissue were taken for water content measurement before thoracotomy, 109 min after the start of CPB, and 30 min after weaning. Lung biopsy specimens were examined by light and electron microscopy. Result: Of 5 animals, 4 survived the experimental procedures. Of these, 3 animals survived on a long-term basis. No significant differences in transpulmonary gradients of leukocyte were found and no significant complement activation was expressed by C3a levels. MDA level did not show significant changes related to lung reperfusion despite an increase after the start of CPB. On both light and electron microscopic examinations, mild to moderate acute lung change was observed. Interstitial edema, leakage of erythrocytes into the alveolar space and endothelial cell swelling were the main findings. Water content of the lung showed a slight increase after the start of CPB, but there was no statistical significance. Conclusion: These findings indicate that ischemia-repersusion lung injury may not be from complement activation-leukocyte sequestration but from another source of oxygen free radicals related to CPB.

• 대한수의학회지
• /
• 제42권2호
• /
• pp.153-162
• /
• 2002

For the induction of arthropathy, 5% hydrogen peroxide($H_2O_2$) was injected for 5 weeks into the intraarticular space of the New Zealand white rabbits to damage articular cartilage. Alginic acid of low molecular weight (2%) made from macromolecular alginate treated with enzyme was administered into articular space at the dose of 5 mg/kg twice a week for 3 and 6 weeks using 1 ml syringe and 26 G needle. Saline was injected for the control. Tissues surrounding the articulation were obtained for the measurements of superoxide dismutase(SOD) activity as a major antioxidant enzyme and malondialdehyde (MDA) as a lipid peroxidation level. Histopathologic examination on the surface of articular cartilage was carried out. Data showed that injection of hydrogen peroxide for 5 weeks had led to the induction of free radical damage and of articular cartilage change as confirmed by microscopic observation. The application of hydrogen peroxide caused a gradual increase in the SODs and MDA. These patterns were similar after 3 and 6 weeks of alginate treatment. Furthermore, microscopic examinations revealed that hydrogen peroxide caused flaking, fibrillation, fissuring, denudation, and hypocellularity in the articular surfaces. In conclusion, lipid peroxidation was demonstrated in the articular cartilage by the administration of hydrogen peroxide in the rabbit model. This lipid peroxidation could be caused by oxygen free radicals. The histologic and enzymatic correlations on lipid peroxidation in the articulation have provided a better understanding of arthropathy. It is possible to take advantage of these findings to evaluate effective alginate dosage more efficiently.

• Biomolecules & Therapeutics
• /
• 제21권4호
• /
• pp.270-276
• /
• 2013

Fucoxanthin is an important carotenoid derived from edible brown seaweeds and is used in indigenous herbal medicines. The aim of the present study was to examine the cytoprotective effects of fucoxanthin against hydrogen peroxide-induced cell damage. Fucoxanthin decreased the level of intracellular reactive oxygen species, as assessed by fluorescence spectrometry performed after staining cultured human HaCaT keratinocytes with 2',7'-dichlorodihydrofluorescein diacetate. In addition, electron spin resonance spectrometry showed that fucoxanthin scavenged hydroxyl radical generated by the Fenton reaction in a cell-free system. Fucoxanthin also inhibited comet tail formation and phospho-histone H2A.X expression, suggesting that it prevents hydrogen peroxide-induced cellular DNA damage. Furthermore, the compound reduced the number of apoptotic bodies stained with Hoechst 33342, indicating that it protected keratinocytes against hydrogen peroxide-induced apoptotic cell death. Finally, fucoxanthin prevented the loss of mitochondrial membrane potential. These protective actions were accompanied by the down-regulation of apoptosis-promoting mediators (i.e., B-cell lymphoma-2-associated ${\times}$ protein, caspase-9, and caspase-3) and the up-regulation of an apoptosis inhibitor (B-cell lymphoma-2). Taken together, the results of this study suggest that fucoxanthin defends keratinocytes against oxidative damage by scavenging ROS and inhibiting apoptosis.

• 한국자원식물학회지
• /
• 제19권6호
• /
• pp.649-654
• /
• 2006

The objective of present study was to investigate the anti oxidative and hepatoprotective effects of tomato extracts. Total antioxidant capacity and total antioxidant response were 5.5 and $19.8{\mu}g$ Trolox equivalent per mg of tomato extract, respectively. DPPH radical scavenging activity of tomato extracts ($10mg\;ml^{-1}$) was 70% as compared to 100% by pyrogallol solution as a reference. The effect of the tomato extracts on lipid peroxidation was examined using rat liver mitochondria induced by iron/ascorbate. Tomato extracts at the concentration of $0.5mg\;ml^{-1}$ significantly decreased TBARS concentration. Tomato extracts prevented lipid peroxidation in a dose-dependent manner. The effect of the tomato extracts on reactive oxygen species (ROS) generation was examined using cell-free system induced by $H_2O_2/FeSO_4$. Addition of $1mg\;ml^{-1}$ of tomato extracts significantly reduced dichlorofluorescein (DCF) fluorescence. Tomato extracts caused concentration-dependent attenuation of the increase in DCF fluorescence, indicating that tomato extracts significantly prevented ROS generation in vitro. The effect of tomato extracts on cell viability and proliferation was examined using hepatocyte culture. Primary cultures of rat hepatocytes were incubated with 1mM tert-butyl hydroperoxide (t-BHP) for 90 min in the presence or absence of tomato extracts. MTT values by addition of tomato extracts at the concentration of 2, 10, and $20mg\;ml^{-1}$ in the presence of t-BHP were 13, 33 and 48%, respectively, compared to 100% as control. Tomato extracts increased cell viability in a dose-dependent manner. These results demonstrate that tomato extracts suppressed lipid peroxidation and t-BHP-induced hepatotoxicity and scavenged ROS generation. Thus antioxidant and hepatoprotective effects of tomato extracts seem to be due to, at least in part, the prevention from free radicals-induced oxidation, followed by inhibition of lipid peroxidation.

• The Korean Journal of Physiology and Pharmacology
• /
• 제11권3호
• /
• pp.85-88
• /
• 2007

Matrix metalloproteinases (MMPs) can degrade a wide range of extracellular matrix components. It has been reported that MMP-9 are activated after focal ischemia in experimental animals. (-)-Epigallocatechin-3-gallate (EGCG), a major constituent of green tea polyphenols, is a potent free radical scavenger and reduces the neuronal damage caused by oxygen free radicals. And it has been known that EGCG could reduce the infarction volume in focal brain ischemia and inhibit MMP-9 activity. To delineate the relationship between the anti-ischemic action and the MMP-9-inhibiting action of EGCG, we investigated the effect of EGCG on brain infarction and the activity of matrix metalloproteinase-9 induced by permanent middle cerebral artery occlusion (pMCAO) in ICR mice. EGCG (40 mg/kg, i.p. $15{\sim}30min$ prior to MCAO) significantly decreased infarction volume at 24 hr after MCAO. GM 6001 (50 mg/kg, i.p. $15{\sim}30min$ prior to MCAO), a MMP inhibitor, also significantly reduced infarction volume. In zymogram, MMP-9 activities began to increase at ipsilateral cortex at 2 hr after MCAO, and the increments of MMP-9 activities were attenuated by EGCG treatment. Western blot for MMP-9 also showed patterns similar to that of zymogram. These findings demonstrate that the anti-ischemic action of EGCG ire mouse focal cerebral ischemia involves its inhibitory effect on MMP-9.

• Journal of Korean Neurosurgical Society
• /
• 제64권6호
• /
• pp.873-881
• /
• 2021

Objective : Peripheral nerve injuries occur mostly as a result of mechanical trauma. Due to the microvascular deterioration in peripheral nerve damage, it becomes challenging to remove free oxygen radicals. Gallic acid is a powerful antioxidant with anti-inflammatory effects and a free radical scavenger. The purpose of the study is to show that gallic acid contributes to the restorative effect in mechanical nerve damage, considering its antioxidant and anti-inflammatory effects. Methods : Thirty male Sprague Dawley albino mature rats were included in the study. Ten of them constituted the control group, 10 out of 20 rats for which sciatic nerve damage was caused, constituted the saline group, and 10 formed the gallic acid group. Post-treatment motor functions, histological, immunohistochemical, and biochemical parameters of the rats were evaluated. Results : Compared to the surgery+saline group, lower compound muscle action potential (CMAP) latency, higher CMAP amplitude, and higher inclined plane test values were found in the surgery+gallic acid group. Similarly, a higher nerve growth factor (NGF) percentage, a higher number of axons, and a lower percentage of fibrosis scores were observed in the surgery+gallic acid group. Finally, lower tissue malondialdehyde (MDA) and higher heat shock protein-70 (HSP-70) values were determined in the surgery+gallic acid group. Conclusion : Gallic acid positively affects peripheral nerve injury healing due to its anti-inflammatory and antioxidant effects. It has been thought that gallic acid can be used as a supportive treatment in peripheral nerve damage.

• Journal of Nutrition and Health
• /
• 제40권2호
• /
• pp.111-117
• /
• 2007

시판 목초액 A (원액 35%)을 사용하여 음용수에 0%, 1.0%, 25.0%, 50.0%, 75.0%가 되도록 조제한 다음, CD계 수컷 흰쥐 (150 ${\pm}$ 10 g)에 2개월 동안 조제사료와 함께 자유 음용케 하여 간조직 중의 활성산소로서 수퍼옥시드 라디칼(O$_{2}\;^-$), 히디록시 라디칼, 과산화수소 및 제거효소로서 수퍼옥시드 디스무타아제 (SOD), 글루타치온 퍼옥시다아제 (GPx) 및 카탈라아제 (CAT)에 미치는 영향을 평가하였다. 목초액 PL-25 및 PL-50 투여군의 간조직의 미토콘드리아 획분에서는 O$_{2}\;^-$의 생성량은 대조군 대비 12${\sim}$14%의 O$_{2}\;^-$의 생성량 억제효과가 나타났고, 간조직의 마이크로솜획분에서는 대조군 대비 각각 11.0${\sim}$15.0의 O$_{2}\;^-$의 생성량 억제효과가 나타났다. 간조직 미토콘드리아획분에서 ${\cdot}$OH 생성량이 목초액 PL-25 및 PL-50 투여군에서 대조군 대비 12${\sim}$20%의 ${\cdot}$OH 생성 억제효과가 나타났고, 간조직의 마이크로솜획분에서는 대조군 대비 17${\sim}$20%의 ${\cdot}$OH 생성 억제효과가 나타났다. 목초액 PL-25 및 PL-50 투여군의 간조직의 미토콘드리아획분에서는 대조군 대비 12${\sim}$15%의 유의적인 H$_{2}$O$_{2}$의 생성 억제효과가 나타났고, 간조직의 마이크로솜획분에서는 대조군 대비 20${\sim}$22%의 상당히 유의적인 H$_{2}$O$_{2}$의 생성 억제효과가 나타났다. 목초액 PL-25 및 PL-50 투여군의 간조직의 Mn-SOD 활성은 대조군 대비 15${\sim}$25%나 유의적인 활성 증가효과가 인정되었고, 간조직의 Cu/Zn-SOD 활성은 대조군 대비 11${\sim}$16%의 유의적인 SOD활성 증가효과가 인정되었다. 목초액 PL-25 및 PL-50 투여군의 간조직의 미토콘드리아획분의 GPx 활성은 대조군 대비 10${\sim}$17%의 GPx 활성 증가효과가 인정되었고, 간조직의 마이크로솜획분의 GPx 활성 증가효과가 인정되었다. 목초액 PL-25 및 PL-50 투여군의 간조직의 미트콘드리아획분의 CAT 활성은 대조군 대비 12${\sim}$14%의 유의적인 CAT 활성 증가효과가 나타났고, 간조직의 시토졸 1획분에서는 대조군 대비 15${\sim}$27%의 CAT 활성 증가효과가 인정되었다. 이상의 결과에서 목초액의 장기간 투여는 간조직 중의 활성산소의 억제효과뿐만 아니라 방어시스템으로서 활성산소 제거효소의 역할도 충실히 수행하여 노화를 효과적으로 예방하고 억제할 수 있을 것으로 기대된다.

• 한국식품영양과학회지
• /
• 제30권4호
• /
• pp.668-672
• /
• 2001

흰쥐에 있어서 구기자 추출물 첨가식이가 간조직의 유해산소대사기구와 알콜대사에 어떠한 효과가 있는지를 알아보기 위하여 구기자 알콜 추출물을 사료에 2%, 4%를 첨가시켜 1개월간 사육한 후 처치하여 다음과 같은 결과를 얻었다. 구기자 추출물 첨가식이로 성장하는 동안 체중증가율은 대조군보다 오히려 약간 감소되는 경향을 보였으며 간기능은 대조군과 별다른 차이가 없었다. 간조직의 xanthine oxidase 활성은 구기자 첨가식이군과 대조군간에는 별다를 차이를 볼 수 없었으며 cytochrome P450 함량은 2%및 4% 구기자 추출물 첨가식이군이 대조군보다 높게 나타나는 경향을 보였다. 그리고 간조직의 catalase 활성은 2% 및 4% 구기자 추출물 첨가식이군 모두 대조군보다 유의한 (p<0.05) 증가를 보였으나 두 실험군 간에는 별다른 차이를 볼 수 없었다. 또한 superoxide dismutase 활성은 2% 구기자 추출물 첨가식이군이 대조군보다 유의한 (p<0.05) 증가를 보였으며, 4% 구기자 추출물 첨가식이군은 대조군과는 별다른 차이가 없었으나 2% 구기자 추출물 첨가식이군에 비해서는 다소 감소하는 경향을 보였다. 그러나 glutathine 함량, glutathione-S-transferase 활성은 구기자 추출물 첨가식이군과 대조군 간에는 별다른 차이를 볼수 없었다. 한편 간조직의 alcohol dehydrogenase 활성은 2% 및 4% 구기자 추출물 첨가식이군 모두 대조군보다 유의한 (p<0.001) 증가를 보였다. 그리고 구기자 추출물 첨가식이군과 대조군의 Km치는 980mM로 동일한 값을 나타내었으나, Vmax치는 2% 및 4% 구기자 추출물 첨가식이군이 대조군보다 각각 71%(660 nmole)및 40%(526nmole)로 증가하였다. 이상 실험결과는 식이중 구기자 알콜 추출물 첨가는 유해산소 및 알콜의 해독효과를 나타냄을 시사해 주고 있다.

• 동의생리병리학회지
• /
• 제21권5호
• /
• pp.1163-1169
• /
• 2007

Effects of Sotosaja hwan on Blood Glucose, Hyperlipidemia, Polyol Pathway and Antioxidative Mechanism in ob/ob Mouse Diabetes is a disease in which the body does not produce or properly use insulin. Etiological studies of diabetes and its complications showed that oxidative stress might play a major role. Therefore, many efforts have been tried to regulate free oxygen radicals for treating diabetes and its complications. Sotosaja-hwan has been known to be effective for the antiaging and composed of four crude herbs. In male ob/ob mouse in severe obesity, hyperinsulinemia and hyperlipidemia, which are features of NIDDM, the hyperglycemic activites and mechanisms of Sotosaja-hwan were examined. Mice were grouped and treated for 5 weeks as follows. Both the lean (C57/BL6J black mice) and diabetic (ob/ob mice) control groups received standard chow. The experimental groups were fed with a diet of chow supplemented with 30 and 90 mg Sotosaja-hwan per 1 kg of body weight for 14 days. The effects of Sotosaja-hwan extract on the ob/ob mice were observed by measuring the serum levels of glucose, insulin, lipid components, and the kidney levels of superoxide anion radical $({\cdot}O_2)$, MDA+HAE, GSH/GSSG ratio, and also the enzyme activities involved in polyol pathway. Sotosaja-hwan lowered the levels of serum glucose and insulin in a dose dependent manner. Total cholesterol, triglyceride and free fatty acid levels were decreased, while the HDL-cholesterol level was increased, in Sotosaja-hwan treated groups. Renal aldose reductase and sorbitol dehydrogenase activities were increased in the ob/ob mice, whereas those were inhibited in the Sotosaja-hwan-administered groups. Sotosaja-hwan inhibited the generation of ${\cdot}O_2$ in the kidney. Finally, MDA+HAE levels was increased and GSH/GSSG ratio was decreased in the ob/ob mice, whereas those were improved in the Sotosaja-hwan-administered groups. Sotosaja-hwan showed the antidiabetic and anti hyperlipidemic activities by regulating the activities of polyol pathway enzymes, scavenging reactive oxygen species and reducing the MDA+HAE levels in the ob/ob mice.