• Applied Microscopy
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• 제2권1호
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• pp.7-15
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• 1972

난소상피에서 발생한 난원세포는 성장발육하여 제 1차 난모세포를 형성하며, 배란되어 난형성강 개구부에서 제2차 난모세포는 정자의 침입을 받은 후 2회의 감수분열을 하여 두개의 극체를 형성하고 난전핵과 정전핵이 적합하여 난할을 시작한다. 세포질의 변화 : 난원세포에서는 크기가 서로 비슷하던 미토콘드리아가 난모세포로 성장되어 감에 따라 자기증식을하여 제1차 난모세포에서는 크기가 서로 다르고 훨씬 많은 미토콘드리아가 나타난다. 편평낭상이던 소포체는 난모세포로 성장하여 세포질대사가 활발하여 짐에 따라 포상낭의 소포체로 변하며 배란후 난모세포에서는 세포질내 일부위에 층판상을 이룬다. 골지 장치는 성숙된 난모세포에서 더욱 뚜렷이 나타나며 망상의 사구체형성을 하고 그 내에 몇 개의 골지소포를 만들고 있다. 표층과립은 수정전 제1차 난모세포에서 매우 증가되어 있으나 수정후는 점차파괴되어 소실된다. 염색질은 난원세포에서 밀도가 높고 강공을 이루고 있는 이질염색질과 밀도가 낮은 소량의 진정염색질로 되어 있으며 배란전 난모세포에서는 이질염색질이 감퇴하고 진정염색질이 많아진다. 배란후 난모세포에서는 풍부한 진정염색질을 다시 가진다. 인은 난원세포에서 전자밀도가 높은 타원형이며 배란전 난모세포에서는 소실되었다가 배란후 난모세포에서는 다시 타원형의 인이 관찰된다.

• Parasites, Hosts and Diseases
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• 제23권2호
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• pp.269-284
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• 1985

The metabolism of Entamoeba histolytica would be affected by various environmental factors, and alteration of the environment was known to afEect the fine structure of 5. histolytica. The present study was designed electronmicroscopically to investigate the ultrastructure and enzyme activities in the aEonic and conventional strains of 5. histolytica. The trophozoites of axenically cultivated HK-9 strain and conventional YS-27 and YS-49 strains of 5. histolytica were collected and liKed with 4% paraformaldehyde/0.1M cacodylate buffier(pH 74), After washing them by centrifugation, 1% warm agar was added in the sediment. Solidified agar with the trophozoites was cut into $lmm^3$ cubes, and incubated in the various substrates to observe enzyme activities. Then, the specimen was post-fixed with 3% glutaraldehyde/0.1M cacodylate buffer (PH 7.4) and 1% osmium tetroBide/0.1M cacodylate buffier (pH 7.4) , dehydrated in ascending ethanol series and embedded in epoxy resin. These were sectioned on an ultramicrotome and observed with a transmission electronmicroscope. The procedures for the observation of the fine structure were same as the above, except for the incubation in the substrate. The sections were stained with uranyl acetate and lead citrate. For the observation of the surface of the amoebae, scanning-electronmicroscopy was carried out. The results obtained in the present study are summarized as follows: 1. The fuzzy coat around double-layered plasma membrane of 5. histolytica was more irregularly and densely distributed in the conventional strains (YS-27, YS-49 strains) than in the axonic strain (HK-9 strain). 2. The endosomes, button bodies and chromatin material were surrounded by a double-layered nuclear membrane having scattered nuclear fores. The paranuclear body, mono- or double-layered vacuoles, vacuolar membrane whorls, rosette-like cylindrical bodies, aggregation of cylindrical bodies and helical bodies were found in the cytoplasm of the amoebae. Helical bodies and glycogen granules were generally abundant, while a few smooth endoplasmic reticula were observed in the cytoplasm. 3. Alkaline phosphatase activity was mainly demonstrated in the plasma membrane, limiting membranes of vacuoles and smooth endoplasmic reticula. ATPase activity was observed in the nucleus, limiting membranes of vacuoles and vacuolar membrane whorls. 4. Acid phosphatase activity was commonly demonstrated in the limiting membranes an contents of vacuoles, Iysosome-like organelles, plasma membrane and the button bodies in the nucleus. The activity was more weakly demonstrated in the HK-9 strain than in the other conventional strains of 5. histolytica. No peroBidase activity was observed in the amoeba strains employed in the present study. 5. With a scanning electron-microscope, no distinct structural differences were observed between the amoeba strains. All the trophozoite forms of the amoebae showed crater-like depressions and rugged features on the outer surface.

• Macromolecular Research
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• 제10권3호
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• pp.158-167
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• 2002

In order to endow with new bioactive functionality from small intestine submucosa (SIS) powder as natural source to poly (L-lactide) (PLA) and poly (lactide-co-glycolide) (PLGA) synthetic biodegradable polymer, porous SIS/PLA and SIS/PLGA as natural/synthetic composite scaffolds were prepared by means of the solvent casting/salt leaching methods for the possibility of the application of tissue engineered bone and cartilage. A uniform distribution of good interconnected pores from the surface to core region was observed the pore size of 40~500 ${\mu}{\textrm}{m}$ independent with SIS amount using the solvent casting/salt leaching method. Porosities, specific pore areas as well as pore size distribution also were almost same. After the fabrication of SIS/PLA hybrid scaffolds, the wetting properties was greatly enhanced resulting in more uniform cell seeding and distribution. Five groups as PGA non-woven mesh without glutaraldehyde (GA) treatment, PLA scaffold without or with GA treatment, and SIS/PLA (Code No.3 ; 1 : 12 of salt content, (0.4 : 1 of SIS content, and 144 ${\mu}{\textrm}{m}$ of median pore size) without or with GA treatment were implanted into the back of nude mouse to observe the effect of SIS on the induction of cells proliferation by hematoxylin and eosin, and von Kossa staining for 8 weeks. It was observed that the effect of SIS/PLA scaffolds with GA treatment on bone induction are stronger than PLA scaffolds, that is to say, in the order of PLA/SIS scaffolds with GA treatment > PLA/SIS scaffolds without GA treatment > PGA nonwoven > PLA scaffolds only with GA treatment = PLA scaffolds only without GA treatment for the osteoinduction activity. The possible explanations are (1) many kinds of secreted, circulating, and extracellular matrix-bound growth factors from SIS to significantly affect critical processes of tissue development and differentiation, (2) the exposure of SIS to GA resulted in significantly calcification, and (3) peri-implant fibrosis due to covalent bonding between collagen molecule by crosslinking reaction. In conclusion, it seems that SIS plays an important role for bone induction in SIS/PLA scaffolds for the application of tissue engineering area.

• 한국동물학회지
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• 제12권4호
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• pp.114-122
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• 1969

成體 albino 흰쥐를 實驗群과 對照群으로 나누어 對照群에는 0.9% 生理食鹽水를, 實驗群에는 methylene blue(38mg/kg, pH 7.4)를 各各 腹腔에 注射한 後 約 30 分後에 總線量 360 rads의 $^{60}Co-\gamma$ 線을 一時全身照射하였다. 照射後 64時間區 와 212時間區로 나누어서 肝 및 心臟組織을 觀察하였다. 照射直後 肝 및 心臟組織을 6% glutaraldehyde (pH 7.4)와 1% osmium tetroxide (pH 7.4)로 冷室에서 二重固定하였으며 脫水한 後 Epon 812로 胞埋하여 MT-2 Porter Blum ultramicrotome 으로 超薄切斷하여 切片을 만들었다. 이를 uranyl acetate 와 lead citrate 로 二重染色한후 Hi9tachi HU-11 E型 電子顯微鏡으로 觀察하였다. 64時間區의 methylene blue 處理群과 對照群에서 肝組織은 顯著한 組織學的 變化의 差를 나타냈다. 다시 말하면 methylene blue 處理群에 比하여 對照群에서는 mitochondria 의 膨大, cristae 의 切斷, endoplasmic reticulum 의 破壞를 觀察할 수 있었으며 또한 endoplasmic reticulum 에 glycogen 粒子의 蓄積을 觀察할수 있었다. 한편 methylene blue 處理群에 比하여 對照群의 212時間區에서도 같은 變化樣相을 나타냈으나 endoplasmic reticulum 에 많은 vacuole 이 形成되었음을 觀察할 수가 있었다. 그러나 methylene blue 處理群은 正當群($\gamma$ 線의 照射와 methylene blue를 處理하지 않음)에 比하여 若干의 差가 觀察되었을 뿐 顯著한 組織學的變化는 나타나지 않았다. 心臟組織에서는 兩群 卽 實驗群과 正當群사이에 顯著한 差는 別로 觀察할 수 없었으나 methylene blue 群에 比하여 對照群에 若干의 變化가 觀察되었다. 다시말하면 methylene blue 處理群에 比하여 64時間區의 對照群에서는 mitochondria의 若干의 膨大, cristae 에 若干의 切斷을 觀察할수 있었고 212時間區의 對照群에서는 sarcoplasmic reticulum에서 若干의 液胞와 glycogen 粒子의 若干의 增加를 觀察할수 있었다. 이로 미루어 보아 methylene blue 가 放射線에 對하여 防禦 果가 있는 것으로 思料된다.

• 청정기술
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• 제21권4호
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• pp.224-228
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• 2015

포스포라이페이즈디를 공유결합을 통해서 초미세다공성막에 고정화하였다. 고정화는 폴리에틸렌이민, 글루타알데하이드, 포스포라이페이즈디를 순차적으로 처리함으로써 수행되었다. X선 광전자 분광기를 이용하여 고정화가 확인되었다. 포스퍼티딜콜린이 분산된 버퍼용액의 pH값을 시간에 따라 모니터링하여 고정화된 경우와 그렇지 않은 경우에 대해 촉매활성을 산출하였다. 속도상수는 폴리스타이렌나노입자에 고정화된 포스포라이페이즈디에서는 0.64 s^-1, 다공성 셀룰로스아세테이트막에 고정화된 포스포라이페이즈디에서는 0.52 s^-1, 그리고 고정화되지 않은 포스포라이페이즈디에서는 0.75 s^-1의 결과가 도출되었다. 재사용에 대한 연구가 10차례까지 수행되었으며, 초기 사용시의 활성대비로 95%가 유지되었다. 열과 저장성에 대한 안정성도 고찰되었으며, 다공성막에 고정화된 포스포라이페이즈디의 경우에 활성손실이 가장 적은 것으로 관찰되었다. 이 연구결과들로부터, 포스퍼티딕산의 생산용 포스포라이페이즈디의 고정화에 대한 지지체로 다공성 막을 사용할 수 있음을 알 수 있다.

• Restorative Dentistry and Endodontics
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• 제13권2호
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• pp.283-294
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• 1988

The purpose of this study was to investigate the characteristic features of the cells and tissues of the chronic periapical lesions using light microscope and electron microscope. Fifteen dental periapical lesions were obtained from the patients undergoing periapical surgery. Each specimen was divided into two parts along the tooth axis. One part was routinely processed for histopathologic examinations. 12 periapical lesions were diagnosed as granuloma and 3 periapical specimens as periapical cyst. The other part was fixed in 2.5% glutaraldehyde in 0.1M sodium cacodylate buffer at pH 7.4 and 1% osmic acid in same buffer. They were embedded in Epon 812. The semithin sections were used for the orientation of the lesions and the ultrathin sections were stained conventionally and examined with AEI Corynth 500 electron microscope. The results were as follows. 1. PMN and macrophages, which were dominant cell type, were scattered in small or large numbers throughout the central destructive area of granuloma. In the granulomatous area, plasma cells and lymphoytes were found in significant number and a lot of new capillary formation were revealed. Clefts caused by cholesterol were often seen in the connective tissue. Occasionally foam cells became collected in groups and epithelial proliferation were present. 2. In both granuloma and cyst, some plasma cells contained narrow cisternae of granular endoplasmic reticulum of which was tightly packed with electron dense materials, and other cells exhibited dilated profiles of granular endoplasmic reticulum. 3. In the area where plasma cells and lymphocytes were collected in groups, lymphocytes with well developed nucleolus and profuse cytoplasm were found and differentiating plasma cells were also present. 4. In the epithelial strands of the granulomatous area, epithelial cells contained enlarged endoplasmic reticulum, tonofilaments and ribosoms. Toward the intercellular space epithelial cells protruded a few microvilli. In the intercellular space, exudate-like electron dense materials, most of which was attached to the plasma membrane, appeared. 5. Some foam cells filled with numerous lipid droplets and others had lipid droplets and crystal-like structures. 6. Cyst epithelium consisted of bright cells and dark cells. The former had bright cytoplasm and small amounts of ribosoms, and the latter dark cytoplasm, many ribosoms, mitochondria and elongated microvilli. 7. Epithelial cells near the cyst lumen protruded a lot of long microvilli toward intercellular space and cyst lumen.

• Clinical and Experimental Reproductive Medicine
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• 제25권1호
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• pp.77-86
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• 1998

The uptake of glucose for metabolism and growth is essential to most animal cells and is mediated by glucose-transporter (GLUT) proteins. The aim of this study was to determine which class of glucose transporter molecules was responsible for uptake of glucose in the mouse early embryo and at which stage the corresponding genes were expressed. In addition, co-culture system with vero cell was used to investigate the effect of the system on GLUT expression. Two-cell stage embryos were collected from the superovulated ICR female and divided into 3 groups. As a control, embryos were cultured in 0.4% BSA-T6 medium which includes glucose. For the experimental groups, embryos were cultured in either co-culture system with vero cells or glucose-free T6 medium supplemented with 0.4% BSA and pyruvate as an energy substrate. 2-cell to blastocyst stage embryos in those groups were respectively collected into microtubes (50 embryos/tube). Total RNA was extracted and RT-PCR was performed. The products were analysed after staining ethidium bromide by 2% agarose gel electrophoresis. Blastocysts were collected from each group at l20hr after hCG injection. They were fixed in 2.5% glutaraldehyde, stained with hoechst, and mounted for observation. In control, GLUT1 was expressed from 4-cell to blastocyst. GLUT2 and GLUT3 were expressed in morula and blastocyst. GLUT4 was expressed in all stages. When embryos were cultured in glucose-free medium, no significant difference was shown in the expression of GLUT1, 2 and 3, compared to control. However GLUT4 was not expressed until morular stage. When embryos were co-cultured with vero cell, there was no significant difference in the expression of GLUT1, 2, 3 and 4 compared to control. To determine cell growth of embryos, the average cell number of blastocyst was counted. The cell number of co-culture ($93.8{\pm}3.1$, n=35) is significantly higher than that of control and glucose-free group ($76.6{\pm}3.8$, n=35 and $68.2{\pm}4.3$, n=30). This study shows that the GLUT genes are expressed differently according to embryo stage. GLUTs were detectable throughout mouse preimplantation development in control and co-culture groups. However, GLUT4 was not detected from 2- to 8-cell stage but detected from morula stage in glucose-free medium, suggested that GLUT genes are expressed autocrinally in the embryo regardless of the presence of glucose as an energy substrate. In addition, co-culture system can increase the cell count of blastocyst but not improve the expression of GLUT. In conclusion, expression of GLUT is dependent on embryo stage in preimplantation embryo development.

• Journal of Periodontal and Implant Science
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• 제40권5호
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• pp.232-238
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• 2010

Purpose: To prolong the degradation time of collagen membranes, various cross-linking techniques have been developed. For cross-linking, chemicals such as formaldehyde and glutaraldehyde are added to collagen membranes, but these chemicals could adversely affect surrounding tissues. The aim of this study is to evaluate the ability of porous non-chemical cross-linking porcine-derived collagen nanofibrous membrane to enhance bone and associated tissue regeneration in one-wall intrabony defects in beagle dogs. Methods: The second and third mandibular premolars and the first molars of 2 adult beagles were extracted bilaterally and the extraction sites were allowed to heal for 10 weeks. One-wall intrabony defects were prepared bilaterally on the mesial and distal side of the fourth mandibular premolars. Among eight defects, four defects were not covered with membrane as controls and the other four defects were covered with membrane as the experimental group. The animals were sacrificed 10 weeks after surgery. Results: Wound healing was generally uneventful. For all parameters evaluating bone regeneration, the experimental group showed significantly superior results compared to the control. In new bone height (NBh), the experimental group exhibited a greater mean value than the control ($3.04{\pm}0.23\;mm/1.57{\pm}0.59$, P=0.003). Also, in new bone area (NBa) and new bone volume (NBv), the experimental group showed superior results compared to the control (NBa, $34.48{\pm}10.21%$ vs. $5.09{\pm}5.76%$, P=0.014; and NBv, $28.04{\pm}12.96$ vs. $1.55{\pm}0.57$, P=0.041). On the other hand, for parameters evaluating periodontal tissue regeneration, including junctional epithelium migration and new cementum height, there were no statistically significant differences between two groups. Conclusions: Within the limitations of this study, this collagen membrane enhanced bone regeneration at one-wall intrabony defects. On the other hand, no influence of this membrane on periodontal tissue regeneration could be ascertained in this study.

• Applied Microscopy
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• 제15권2호
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• pp.111-129
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• 1985

The morphology and histology of the gastrointestinal mucosa of the mole, Talpa micrura coreana (Thomas), were studied using light and scanning electron microscopes. Tissue specimens were taken from body and pyloric portions of the stomach, and from the initial, proximal, middle, distal and terminal portions of the intestine. For light microscopy, tissue blocks were fixed in 10% buffered neutral formalin, embedded in paraffin wax, and sectioned at a thickness of $5{\mu}m$. These sections were stained with hematoxylin-eosin. For scanning electron microscopy, tissue blocks were fixed in 1% glutaraldehyde-1.5% paraformaldehyde, and postfixed in 1% osmium tetroxide, dehydrated in graded alcohol, transferred to isoamylacetate and dried by the critical point drier(Polaron E 3000). Subsequently, specimens were coated with gold and observed with a JSM-35C scanning electron microscope. The results were as follows: The mucous membrane of the body portion of the stomach had numerous irregular folds and the pyloric mucosa formed the strawberry-shaped folds, and general histological structures of each portion were similar to those of man. The intestine could not be differentiated macroscopically and microscopically into small and large intestines. There was no cecum, appendix, taenia coli, haustra coli or appendices epiploicae. In the initial portion (4 mm long), conical or tongue-shaped villi with the height of $143.3{\pm}10.7{\mu}m$ were present, and large mucous glands were seen in the submucosa. In the proximal, middle and distal portions, wavy folds composed of the epithelium and lamina propria were densely and transversely arranged, and their heights were $440.4{\pm}45.5{\mu}m,\;454.4{\pm}19.9{\mu}m\;and\;205.2{\pm}33.5{\mu}m$, respectively. The mucosa of the terminal portion (3 cm long) formed several longitudinal folds, and the intestinal glands were directly opened on the smooth surface of the folds. Aggregated lymphoid follicles were observed in the major portions of the intestine except the initial and terminal portions. There was no circular or semilunar fold throughout the intestine.

• Applied Microscopy
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• 제29권1호
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• pp.57-66
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• 1999

한국산 플라나리아 뇌신경절을 실험에 사용할 수 있도록 적당한 크기로 적출하여 부위별로 잘라낸 후 2.5% paraformaldehyde-3% glutaraldehyde로 1시간 30분 전고정을 하고 이러서 $OsO_4$로 2시간 후 고정을 한 다음 전자현미경 관찰방법에 따라 실험한 후 다음과 같은 결론을 얻었다. 뇌신경절을 구성하고 있는 세포는 신경세포와 신경분비세포, 신경아교세포 그리고 신경섬유들로 이루어진 신경망 등이었다. 신경세포는 직경이 $5{\mu}m$ 정도인 원형 또는 타원형의 작은 세포로서, 핵은 타원형체로 세포질에 비해 크고 이질염색질이 고르게 발달해 있었으나, 세포질은 세포 소기관의 발달이 미진하여 비교적 단순하게 보였다. 신경분비세포는 그 모양이 긴 타원형이거나 방추형세포로서 타원형의 큰 핵을 소지하였다. 또한 이들의 세포질속에는 직경 60nm 정도의 분비성과립들로 가득차 있었다. 신경아교세포는 매우 드물게 나타나는 방추형의 세포로서 (크기, $6\times0.8{\mu}m$) 이들은 신경섬유 사이에서 주로 관찰되었다. 신경망을 구성하고 있는 신경섬유와 신경종말 속에는 사립체와 신경소관 그리고 4종류의 분비성소포(직경, 75nm, 50nm, 그리고 37nm 정도의 전자밀도가 높은 과립소포 3종과 30nm 크기의 전자밀도가 낮은 투명과 립소포 1종) 등이 존재하였는데, 이들은 단일소포 형태와 혼합소포형태로 존재하였다. 또한 이들의 신경연접 형태는 축삭-수상돌기연접과 축삭-축삭돌기연접 등의 신경 연합만이 주로 관찰되는 특징을 보였다.