• 대한임상검사과학회지
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• 제48권2호
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• pp.114-117
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• 2016

골은 일생에 걸쳐 지속적인 재형성과장을 거치면서 유지되고 이러한 기전에 대한 연구는 골다공증을 비롯한 골대사 질환의 병태생리와 치료에 있어 큰 진전을 이루고 있다. 특히 생체 내 골형성 및 재생과정을 연구하는데 있어 형광표지자를 이용하는 방법이 널리 알려져 있는데, 그 중 calcein은 칼슘 킬레이터로 골이 새롭게 형성하는 부위에 녹색을 띔으로써 유용한 마커로 사용된다. 그러나 대부분의 골형성 연구에서 실험동물의 경우 표본제작을 할 때 크기가 작고 뼈가 부숴지기 쉬워 rat이나 rabbit을 이용하였으며, mice의 femur를 cross-section해서 관찰한 연구는 거의 없는 실정이다. 그래서 본 연구에서는 어린 mice를 실험동물로 이용하였으며, 생체 내 calcein을 4주간, 8주간 투여한 후 골 형성 변화를 형광현미경으로 관찰한 결과 8주차 쥐에서 4주차보다 진하고 골 형성 간격도 넓게 관찰된 것을 확인 할 수 있었다. Mice는 빠른 시일 내에 결과를 얻을 수 있고 부작용이 적은 장점이 있어서 앞으로 knock-out mice를 이용한 생체 내 실험에 활용하기 적합하다고 생각되며, 골형성 속도 평가 등 다양한 분야에서의 골 형성과 재생연구에 있어 기초 정보를 제공할 것으로 기대한다.

• KSBB Journal
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• 제10권2호
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• pp.204-211
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• 1995

인지질 그 자체만으로는 안정한 이중층 리포좀을 형성하지 못하는 불포화 PE(DOPE)에 palmitoyl가 가 결합된 항체(p-IgG)를 지질층에 삽입시켜 lmm t unoliposome을 제조하고 그 특성에 관하여 살펴 보 았다. 우선 안정된 리포좀을 제조하기 위해서 고려 해야할 인자들로 항체 가공방법, 지질과 항체와의 몰 비, 그리고 각종 첨가제들에 대한 최적 조건을 조 사하였다. 예를 들면 p-IgG와 lipid의 볼비를 $2.5{\times}10^{-4}$ 으로 했을 때 안정한 리포좀을 만들 수 있었으며, 첨가제로 들어가는 DOC의 경우 최종 농도가 O.09wt % 일 때 calcein의 포집률이 최대가 되었고 c calcein의 최종 pH는 8.5~9.5 정도에서 안정한 라포좀이 제조될 수 있었다. 다중 빛 단일클론의 항체 를 삽입한 리포좀을 표면항원을 가진 표적세포와 결합시켰을 때 리포좀이 와해되면셔 포집된 calcein이 방출되는 것으로 보아 삽입된 p-IgG가 PE 리포좀을 형성하는데 필수척임을 알 수 있었다. 또 같은 리포좀을 비특이적인 세포와 접촉시켰을 때에는 아무 런 변화를 보이지 않아 calcein 방출이 항원-항체 반응에 의한 것임을 알 수 있었고 이로부터 표적 민 감성 PE 리포좀이 만들어졌음을 확인하였다.

• Ocean and Polar Research
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• 제31권4호
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• pp.349-357
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• 2009

Ballast water is widely recognized as a serious environmental problem due to the risk of introducing non-indigenous aquatic species. In this study we aimed to investigate measures which can minimize the transfer of aquatic organisms from ballast water. Securing more reliable technologies to determine the viability of aquatic organisms is an important initiative in ballast water management systems. To evaluate the viability of marine phytoplankton, we designed the staining methods of fluorescein diacetate (FDA) and Calcein-AM assay on each target species belonging to different groups, such as bacillariphyceae, dinophyceae, raphidophyceae, chrysophyceae, haptophyceae and chlorophyceae. The FDA method, which is based on measurements of cell esterase activity using a fluorimetric stain, was the best dye for determining live cells of almost all phytoplankton species, except several diatoms tested in this study. On the other hand, although fluorescence of Calcein-AM was very clear for a comparatively longer time, green fluorescence per cell volume was lacking in most of the tested species. According to the Flow CAM method, which is a continuous imaging technique designed to characterize particles, green fluorescence values of stained cells by FDA were significantly higher than those of Calcein-AM treatments and control, implying that the Flow CAM using FDA assay could be adapted as an important tool for distinguishing living cells from dead cells. Our results suggest that the FDA and Calcein-AM methods can be adapted for use on phytoplankton, though species-specific characters are greatly different from one organism to another.

• Journal of Pharmaceutical Investigation
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• 제36권5호
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• pp.309-314
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• 2006

The multicellular layers(MCL) of human cancer cells is a three dimensional(3D) in vitro model for human solid tumors which has been used primarily for the assessment of avascular penetration of anti-cancer drugs. For anti-cancer drugs with penetration problem, MCL represents a good experimental model that can provide clinically relevant data. Calcein-AM is a fluorescent dye that demonstrates the cellular vitality in a graded manner in cancer cell culture system. In the present study, we evaluated the use of calcein-AM for determination of anti-proliferative activity of anti-cancer agents in MCL model of DLD-1 human colorectal cancer cells. Optical sectioning of confocal imaging was compromised with photonic attenuation and penetration barrier in the deep layers of MCL. By contrast, fluorescent measurement on the cryo-sections provided a feasible alternative. Cold pre-incubation did not enhance the calcein-AM distribution to a significant degree in MCL of DLD-1 cells. However, the simultaneous determination of drug penetration and cellular vitality appeared to be possible in drug treated MCL. In conclusion, these data suggest that calcein-AM can be used for the simultaneous determination of drug-induced anti-proliferative effect and drug penetration in MCL model.

• 공업화학
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• 제8권1호
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• pp.59-66
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• 1997

Di(10-hemisuccinyloxy)decyl muconate(DDM)와 di(6-hemisuccinyloxy)hexyl muconate(DHM)가 합성되었으며, 수용액에 분산되어 각각 $97^{\circ}C$과 $79^{\circ}C$에서 상전이를 나타내었다. 이들은 자체적으로, 또는 콜레스테롤이나 dioleoylphosphatidylethanolamine (DOPE)을 혼합하여도 리포좀을 형성하지 않았지만, phosphatidylcholine(PC)과 혼합되면 리포좀을 형성하였다. 리포좀막에서 DHM이 254nm의 자외선에 노출될 때 1,2-중합반응이 쉽게 진행되었다. DOPE/dioleoylphosphatidylcholine(DOPC)/DHM(3/3/1)으로 구성된 리포좀은 중성 pH에서는 안정하지만 약산성 pH에서는 불안정하여 pH 4.8과 5.8의 phosphate-buffered saline(PBS, $37^{\circ}C$)에서 30분과 50분 이내에 각각 봉입된 calcein의 방출이 완료되었다. calcein의 방출은 pH가 감소됨에 따라서 증가하며 pH 5.5와 5.0 근처에서는 각각 봉입 calcein의 50%와 100%가 방출되었다.

• 약학회지
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• 제38권6호
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• pp.637-645
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• 1994

The effect of various drugs on the stability of the liposomal membrane of phosphatidylcholine and cholesterol was studied, employing the fluorescence self-quenching method. Calcein was entrapped into the phospholipid small unilamellar vesicles and the leakage of the fluorescence probe was monitored on adding the drug to the system. The results of the experiments showed that phenothiazine derivatives, some potent local anesthetics and surface active agents were very effective in inducing the leakage of calcein from the liposome. The leakage-inducing activity of these drug substances has been ascribed to their surface activity and the perturbation of the liposomal membrane by these substances. On the other hand drug substance with low surface activity or without amphiphilic moieties did not show any effect or only small effect on the leakage of calcein from the liposomes. The effect of lipid concentration on the stability of the liposomes was also investigated to show that the higher concentrations of lipid more drug was required to induce the leakage. The effect of surface charges of vesicles was also studied, and the results showed that the charge on the liposomes enhanced the stability of the liposomes against the leakage-inducing activity of these drug substances.

• 공업화학
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• 제17권2호
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• pp.138-143
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• 2006

Ethosome은 에탄올에 용해된 레시틴을 친수성 용액으로 수화시켜 만들어지는 액정형 베시클이다. Ethosome을 약물전달체로 개발하기 위해서는 베시클의 높은 포집효율과 작은 입자크기가 필수적이기 때문에 ethosome의 포집효율과 입자크기에 영향을 주는 인자들에 대한 연구를 시도하였다. Calcein을 친수성 지표물질로 사용하여 ethosome을 만들고, 구성 성분비와 제조조건에 따른 ethosome의 특성의 변화를 관찰하였다. 에탄올과 calcein 용액의 첨가량 레시틴 중 포스파티딜콜린의 함량, 제조온도, 교반속도 및 PBS 첨가방법 등이 ethosome의 특성에 상당히 큰 영향을 미치는 것을 확인하였다. 초음파 처리를 한 경우에는 ethosome의 포집효율이 감소하는 결과가 나타났는데 이러한 결과는 강한 초음파 진동에 의해 베시클에 포집되었던 성분이 방출되었기 때문이다.

• 약학회지
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• 제38권2호
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• pp.131-139
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• 1994

Calcein-encapsulated small unilamellar vesicles of various lipid composition were prepared using the sonication technique, and their stabilities at $20^{\circ}C$ were examined by measuring calcein leakage from the liposomes. The fluidity of these liposomal bilayers was also investigated by measuring the fluorescence polarization of DPH labelled into the liposomes. The results showed that liposomes made of PC mixtures with different acyl chain length were very stable, which may be due to the formation of interdigitated bilayer structure. The addition of cholesterol further stabilized these PC liposomes. However, addition of cholesterol reduced the encapsulation efficiences of liposomes. The fluidity of the liposomes was significantly decreased by cholesterol in the liquid crystalline state, but not changed in the gel state. These results suggest that the enhanced stability of PC mixture liposomes may be ascribed to the formation of stable interdigitated bilayer structure. In membrane-mimetic and drug-delivery studies, vesicles made of mixtures of various phospholipids are recommended instead of addition of cholesterol to the phospholipid.

• 한국양식학회지
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• 제12권3호
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• pp.237-245
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• 1999

In this study, we evaluated the efficiency of chemical marking of black rockfish scales by immersion in oxytetracycline hydrochloride (OTC, 500 ppm), alizarin red S (AR, 250 ppm) and calcein (CARL, 250 ppm) diluted rearing water. Immersion treatment of chemicals had no effects on both mortality and growth of black rockfish. Marking sucess was 100% in all treatment durations (24, 48 and 72 hours) with three chemicals and marking quality was higher in 48 and 72 hours than 24 hours treatment. Marking retention rates at 24 weeks after treatment were 100% in OTC and CAL treated group, but marking quality was higher in CAL treated group (brilliant 92%, bright 8% and dim 0%) than in OTC treated group (brilliant 4%, bright 70% and dim 26%). AR treated group had lower marking retention rates and marking quality than OTC and CAL treated group. As a results, immersion treatment with OTC and CAL was effective in marking scales of black rockfish and practical in releasing program and other studies requires same rearing environment.

• Macromolecular Research
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• 제13권1호
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• pp.54-61
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• 2005

We prepared temperature-sensitive liposomes (TS-liposomes) modified with a thermo sensitive polymer, such as poly(N-isopropylacrylamide) (PNIPAAm), to increase the degree of drug release from liposomes at the hyperthermic temperature. A PNIPAAm hydrogel containing TS-Iiposomes was also prepared to obtain a hydrogel complex at body temperature. In addition, a depot system for local drug delivery using the polymer hydrogel was developed to enhance therapeutic efficacy and prevent severe side effects in the whole body. The PNIPAAm-mod­ified TS-liposome was fixed into the PNIPAAm hydrogel having a high temperature-sensitivity. The release behavior of calcein, a model drug, from TS-liposomes in the PNIPAAm hydrogel was then initiated by external hyperthermia; the results indicated that sustained release as a function of temperature and time was caused by the thermosensitivity of the liposome surface and diffusion of the drug into the PNIPAAm hydrogel. Our results indicated that TS-liposomes in a PNIPAAm hydrogel represented a plausible system for local drug delivery.