• 한국어업기술학회:학술대회논문집
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• 한국어업기술학회 2001년도 추계 수산관련학회 공동학술대회발표요지집
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• pp.239-240
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• 2001

Collagenases are generally defined as enzymes capable of degrading the polypeptide backbone of native collagen under conditions which do not denature the protein. Two types of proteases with collagenolytic activity have been reported and thought to play different physiological functions. Metallo-collagenases, firstly discovered in tadpole tissue explants are zinc-containing enzymes requiring calcium for optimum activity and stability, and These enzymes have been widely studied from various mammalian tissues as well as from bacteria, such as Bacillus cereus, Clostridium histolyticum, Achromobacter, Vibrio alginolyticus and Clostridium perfringens and snake venoms. (omitted)

• Journal of Periodontal and Implant Science
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• 제28권4호
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• pp.703-721
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• 1998

본 실험에서는 치주질환 발병에 위험인자이고 창상치유에 위해한 영향을 미치는 흡연이 치주조직에 미치는 반응을 규명하기 위해 치은 섬유아세포의 중요한 기능인 교원질 합성과 분비된 단백질 분해에 영향을 주는 효소활성도를 중심으로 Nicotine과 NNK가 이 세포에 미치는 영향을 관찰하고 또한Nicotine이 NNK로 대사되어 작용을 나타내는 것인지, Nicotine과 NNK가 서로 다른 경로를 통하여 치은 섬유아 세포에 영향을 주는지를 규명하고자 이들 화합물의 돌연변이성 실험, 세포 증식을 보기위한 MTT test와 교원질과 collagenase의 mRNA 수준 및 교원질 분해 효소의 효소활성들을 실험하여 다음과 같은 결과를 얻었다. 1. Nicotine은 대사 활성계의 존재 여부와 상관없이 돌연변이성을 나타내지 않았고 NNK 의 경우에는 그 자체로는 돌연변이성이 없었으나, 대사활성계가 존재하는 경우에 농도의존적으로 돌연변이성을 나타내었다. 2. 증식능 실험에서 흡연자의 세포증식능은 비흡연자에 비해 감소되었다. 3. 비흡연자의 치은 섬유아세포에 Nicotine 과 NNK를 처리한 경우에 대조군에 비해농도 의존적으로 세포 증식능이 감소되었으며, 고농도에서 Nicotine의 경우 세포 독성을 나타내었으나, NNK는 세포독성을 나타내지 않았다. 4. 교원질 분자의 mRNA 수준에 대한 Nicotine의 효과는 proa1과 pro ${\alpha}2$ 모두에 영향을 주지 않았고, NNK는 pro ${\alpha}1$의 경우에는 감소하였으나, proa2에는 영향을 주지 않았다. 5. Collagenase의 mRNA 수준에 대한 효과에서 Nicotine은 없었으나 NNK는 감소하였다. 6. 교원질 분해 효소에 대한 Nicotine과 NNK의 효과는 I형 교원질의 분해 효소를 알기 위한 collagenase 효소 활성의 경우에는 효과가 모두 증가되었으나, IV형 교원질의 분해 효소인 gelatinase 효소 활성에는 영향을 주지 않았다. 또한 흡연자의 collagenase 효소활성은 비흡연자의 치은 섬유아세포에 Nicotine이나 NNK를 처리한 경우와 비슷한 수준으로 증가되었다. 이상의 결과로 보아 Nicotine과 NNK는 모두 치은 섬유아세포에 영향을 주어 교원질의 양을 감소시키며, 그 기전은 서로 다른 경로를 통하여 일어나는 것으로 사료된다.

• Applied Microscopy
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• 제28권3호
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• pp.379-390
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• 1998

Dermal wound healing responses in the skin of the toad, Bombina orientalis, were examined using transmission electron microscopy. At 12 hours after wounding, debridement and collagenolysis occurred in damaged dermis. Histocyte has a large nucleus and long cytoplasm process. Phagocytic vesicle and lysosome were observed in the cytoplasm. Damaged blood cells were transformed spindle to irregular shape. Autolysis was observed in their cytoplasm. Histocytes are found in poly-band. The irregularly shaped nucleus is located peripheral region in cytoplasm. At 2 days after wounding, partial aggregation of blood cells is observed. Phagocytic, activity is observed in histocyte and collagenolytic collagen fibers are scattered. Fibroblast is observed in the dermis at 3 days after wounding. Clusters of ribosomes and some short cisternae of rough-surfaced endoplasmic reticulum are found in the cytoplasm. In histocyte at 7 days post wounding, various size granules composed of moderately dense material are found the cytoplasm. In this period histocyte is round to rod in profile, with slender processes projecting from the surface. At 7 day after injury, it was observed that formation of connective tissue fibers and amorphous ground substance in regenerating skin.

• Biomolecules & Therapeutics
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• 제12권1호
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• pp.1-8
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• 2004

In chronic airway inflammatory diseases such as asthma and chronic bronchitis, it has been suggested that matrix metalloproteinases secreted from infiltrating neutrophil contribute the pathogenesis of the disease and have been a focus of intense investigation. We report here that hamster tracheal surface epithelial goblet cells (HTSE cells) produce matrix metalloproteinase-2 (MMP-2) and tissue inhibitor of metalloproteinase-2 (TIMP-2). Matrix metalloproteinase activities were investigated using [$^3H$]collagen-digestion assay and gelatin zymography. The subtype of matrix metalloproteinases expressed from HTSE cells was MMP-2 (gelatinase A), which was determined by Western blot with various subtype selective anti-matrix metalloproteinase antibodies. The MMP-2 and TIMP-2 cDNAs from HTSE cells were partially cloned by RT-PCR and they reveal more than 90% of sequence homology with those from human, rat and mouse. The collagenolytic activity was increased with the secretory differentiation of the HTSE cell and it was found that zymogen activation was responsible for the increased MMP-2 activity in HTSE cells. The results from the present study suggest that the metaplastic secretory differentiation of airway goblet cells may affect chronic airway inflammatory process by augmenting the zymogen activation of MMP-2.

• Journal of Periodontal and Implant Science
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• 제27권1호
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• pp.1-17
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• 1997

Tetracycline is known to be effective in eliminating periodontopathogens and have collagenolytic activity. This study was performed to observe the desorption kinetics and structural changes of tetracycline-treated barrier membranes for guided tissue regeneration. Four kinds of barrier membranes were tested : $Tefgen^{(R)}$(American Custom Medical, USA) and $Gore-Tex^{(R)}$(W.L. Gore & Associates Inc., USA) as nonresorbable membranes ; Resolut(polyglycolide & polylactide copolymer, W.L. Gore & Associates Inc., USA) and $Biomend^{(R)}$(collagen, Collatec Co., USA) as resorbable membranes. The membranes were cut into discs(diameter : 4mm) and were immersed in 5% tridodecylmethylammonium chloride(TIMAC) ethanol and air-dried. The membrane discs were absorbed with $100{\mu}g/ml tetracycline solution(pH8) for one minute and dried. For desorption kinetics, TC treated discs were immersed in phosphate buffered saline solution (PBS, pH 7.4). PBS was exchanged daily and TC concentration was measured by absorbance at 276nm on UV spectrophotometer. To measure remaining antibacterial activity, discs of 1 day to 4 weeks after desorption were placed on Mueller Hinton agar containing Bacillus cereus and incubated aerobically in $37^{\circ}C$ for twelve hours and the inhibition diameters were measured. To observe the structural change of membranes after TIMAC treatment or immersion in PBS, the membrane discs were examined under SEM. The results were as follows : 1. Total amounts of TC absorbed into membrane discs($0.7536mm^2$) were $2000{\mu}g$, $1800{\mu}g$, $2625{\mu}g$ and $2499{\mu}g$ for $Tefgen^{(R)}$, $Gore-Tex^{(R)}$, $Biomend^{(R)}$ and $Resolut^{(R)}$. 2. The concentration of TC released from barrier membrane discs was maintained over $4{\mu}g/ml$ until the fifth day in nonresorbable membranes and $Resolut^{(R)}$, but until the fourth day in $Biomend^{(R)}$, Until the ninth day in nonresorbable membranes and until the seventh day in resorbable membranes, the TC concentration was maintained over $1{mu}g/ml$. 3. The four membrane discs in the first day showed similar size of inhibition zone. One to four weeks later, the inhibition zone was much smaller in resorbable membrane discs than nonresorbable membrane discs. 4. Any structural change due to treatment of TIMAC was not observed on the nonresorbable membranes. $Resolut^{(R)}$ did not show any structural change except fibrillar loosening during immersion period, but Biomend showed destruction of membrane structure from the first week of immersion. This study indicates that tetracycline treated barrier membranes lead to the sustained release of tetracycline for over 7 days. This slow release pattern of tetracycline may contribute to the favorable clinical outcome of guided tissue regeneration.

• Restorative Dentistry and Endodontics
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• 제33권2호
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• pp.148-161
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• 2008

본 연구는 상아질 혼성층의 교원섬유를 가수분해하는 효소인 MMPs (Matrix metalloproteinses)의 억제제로 알려진 chlorhexidine (CHX)을 적용 후 결합강도를 측정하였으며, 이를 각각 열순환 처리 후 결합강도를 측정하였다. 또한 주사전자현미경으로 접착계면에서의 파괴 양상을 비교 분석하였다. 우식이 없는 발거한 32개의 제3대구치의 교합면 상아질을 노출시키고 GI그룹에서는 dentin conditioner를 처리 후 2% chlorhexidine을 적용시키고, 산부식 접착제 그룹에서는 인산 산부식을 시행하고 2% chlorhexidine을 적용 후 3단계 산부식형 상아질 접착제 (Scotchbond Multipurpose, SM), 2단계 산부식형 상아질 접착제 (Single Bond, SB)를 도포하고, 자가부식 접착제 그룹에서는 2% chlorhexidine 적용 후 자가부식 상아질 접착제 (Clearfil Tri-S, TS)를 도포한다. 이후 복합 레진 (Z-250)과 GI (Fuji-II LC)를 충전한 시편을 $1\;mm^2$의 단면을 갖는 beam으로 제작하여 열순환 하지 않거나, 10,000회 열순환 ($5\;{\sim}\;55^{\circ}C$)하였다. Universal testing machine (EZ-test; Shimadzu, Japan)에서 cross head speed 1 mm/min로 인장력을 가하여, 미세인장결합강도를 측정하였다. 실험 결과는 유의수준 0.05 level에서 two-way ANOVA를 이용하여 통계분석하였다. 그 후 파절된 시편의 파괴 양상을 현미경 (SEM)으로 관찰하여 다음과 같은 결론을 얻었다; 1. 2% CHX을 적용한 모든 실험군에서 상아질과의 미세인장결합강도가 증가하였고, 열순환은 상아질과의 미세인장결합강도를 감소시켰다 (P > 0.05). 2. CHX 적용 후 열순환 한 군은 CHX을 적용하지 않고 열순환한 군에 비하여 상아질과의 미세인장결합강도가 높았으며, 특히 GI와 TS군에서 유의한 차이를 나타내었다 (P < 0.05). 3. 파괴 양상 분석 결과, 혼성층에서의 접착성 파괴를 보이며, CHX을 적용하면 혼성층 기저부에서 상부로 파괴 부위가 옮겨가는 양상을 나타내었다. 이상의 연구 결과를 토대로, MMPs 억제제인 2% CHX은 글래스 아이오노머 시멘트와 상아질 접착제의 초기 미세인장결합강도에는 영향을 미치지 않으며, CHX 적용이 접착내구성을 유지하는데 도움이 되었다.