• Proceedings of the Zoological Society Korea Conference
• /
• 1994.10a
• /
• pp.152.2-152
• /
• 1994

• Proceedings of the Zoological Society Korea Conference
• /
• 1996.04a
• /
• pp.44.2-44
• /
• 1996

• Korean Journal of Animal Reproduction
• /
• v.24 no.2
• /
• pp.143-154
• /
• 2000

Most eggs initiated the fertilization processes but arrested at specific stages. The stages included failure of the oocyte to exit from the meiotic metaphase-II with or without sperm penetration, failure of appropriate sperm aster formation, inability to form proper male and female pronuclei, failure of suitable pronuclear apposition, and failure to form proper number of either male or female pronuclei. Various images of defective microtubule organization and chromatin configuration during IVF and ICSI procedures were observed. We discussed the data with previous research results during normal fertilization in humans and other mammals. In conclusion, various aberrant patterns in microtubule assembly and chromatin configuration, which were assessed in the present study, could be used as criteria to improve assisted reproductive technology in clinics. However, further cellular and molecular characterization is needed to clarify these aberrant patterns of cytoskeletal assembly.

• Journal of Embryo Transfer
• /
• v.29 no.1
• /
• pp.51-57
• /
• 2014

The objectives of this study were to investigate the effects of trehalose as a cryoprotectant for porcine freeze-dried spermatozoa, to find the optimal freeze-drying time and storage periods of freeze-dried spermatozoa, and to find out pronuclear formation rates, cleaved rates, and embryo development through intracytoplasmic injection of freeze-dried spermatozoa on porcine oocytes. The survival rates of spermatozoa after freeze-drying with trehalose treatment were significantly higher than those of them without trehalose treatment (p<0.05). The highest survival rates were found at 75 mM trehalose treatment. The longer storage periods after freeze-drying seemed to have a lower survival rates. Development in culture of pig by ICSI with trehalose treatment were significantly higher than those of them without trehalose treatment (p<0.05). Shorter freeze-drying time of spermatozoa was resulted in the highest cleaved rates and embryo development.

• Korean Journal of Animal Reproduction
• /
• v.19 no.3
• /
• pp.205-216
• /
• 1995

Microtubules와 micrfilaments는 포유동물 난자이 주요한 세포 구조물들로, 이들은 난자의 성숙, 수정 및 배발달시 핵질의 이동과 세포질 분열에 직접 관여하는 것으로 알려져 왔다. 난자내 세포구조물의 정확한 움직임은 정상적인 배 발달을 위해 필수적이다. Microtubules는 $\alpha$, $\beta$- bubulin이 서로 연결되어 이루어져 있으며, 수정시 웅성.자성전핵 움직임과 세포분열시, 유사 및 감수분열시 그 역할을 한다. 생쥐를 제외한 대부분의 동물에서 microbubules의 역할은 수정시 정자가 centrosome을 난자내로 이전하여 sperm aster를 형성함으로써 시작된다고 보고되고 있다. 따라서 정자의 도움없이 배발달이 일어나는 단위발생시 microbubules의 형성은 연구들 사이에 흥미로운 연구대상이 되고 있다. 한편 microfilaments는 세포분열시 세포질을 분할하는 기계적인 역할을 하는 것으로 알려져 있으며, 최근 생쥐 난자에서는 정자의 난자내 융합과 웅성 및 자성 전핵의 이동에 관여한다고 보고되고 있다. 포유동물 난자의 체외성숙, 체외수정을 유도할 때 여러 가지 비정상적인 핵움직임과 세포분열이 관찰되어지고, 낮은 배발달율이 보고되고 있는데, 최근 연구자들은 세포구조물, 즉 microtubules와 microfilaments의 비정상적인 역할에서 기인한다고 보고 있다. 따라서 포유동물 난자의 성숙.수정 및 단위발생시 세포구조물의 움직임과 역할 및 상호관계에 대한 정확한 이해는 체외수정율 및 배발달 향상에 중요한 기초자료로 이용되리라고 본다.

• Korean Journal of Optics and Photonics
• /
• v.3 no.2
• /
• pp.123-132
• /
• 1992

We designed and constructed the Cs beam tube which consists of a Ramsey cavity, four C-field rods, fluorescence detecting systems, and etc. for developing an optically pumped Cs atomic clock. A semiconductor laser was used for optical pumping and probing in the Cs beam. We observed Ramsey resonance signal by detecting the fluorescence signal in the probing region as the microwave frequency injected into the Ramsey cavity was scanned near 9192.6 MHz which corresponds to the "clock transition" of Cs atoms. We found that the linewidth of the Ramsey signal was 200 Hz, the magnetic field intensity was $8.61\muT$ when the current of 0.8A flowed in the C-field rods, and the second order Zeeman shift by the magnetic field was 3.17 Hz.s 3.17 Hz.

• Proceedings of the Korean Society of Fisheries Technology Conference
• /
• 2000.05a
• /
• pp.157-158
• /
• 2000

김(Porphyra)속 식물은 색깔, 체형, 크기, 촉감 등의 식별형질에 근거하여 분류가 시작되었고, Kurogi는 일본산 김속 식물의 분류학적 연구를 개괄하면서 김속의 식별형질로서 엽체의 세포층수, 거치상 돌기의 유무, 생식유형, 정자낭반의 형태, 정자낭 및 과포자낭 분열형식, 무성포자의 형성 유무, 지리적 분포, 각포자의 형태 및 생태적 특성 등을 종합하였다. 그러나 전통적인 분류 특징을 가지고 70종이나 되는 김을 분류한다는 것은 지금까지 불충분하여왔다. (중략)

• Korean Journal of Animal Reproduction
• /
• v.17 no.4
• /
• pp.339-346
• /
• 1994

An understanding of the structure and function of mammalian spermatozoa requires the iso-lation of these components. In this study, frozen-thawed bovine spermatozoa were treated by physical treatments (vortexing, 26 gauge needle, strained 26 gauge needles and freezing-thawing) or chemical treatments (trypsin, dithiothreitol, sodium dodecylsulfate and $\beta$-mercaptoethanoJ) to yield free heads and tails. The most effective treatment was repeated pumping of sperm suspension through a strained 26 gauge needle conneted to a syringe. Spermatozoa by this treatment were mainly broken at the junction of the head and the tail, resulting in 90-100% yields. Also, sperm head surface did not modify during strained 26 gauge needle treatment when either spermatozoa or sperm heads were incubated in 250${\mu}\textrm{g}$/ml of FITC-UEA 1 for 1 h at room temperature to detect the modification of sperm surface components. Other physical treatments were less efficient for the breakdown of spermatozoa. The effects of chemical treatments on bovine spermatozoa are not noticeable. Dissected sperm heads and tails should be fractional leading to nearly pure components by sucrose gradient centrifugation at 1,000 rpm for 15 min. The result suggest that the established method may be useful for the biochemical study of spermatozoal components, and the understanding of oocyte activation mechanism either by spermatozoal components during fertilization or microinjection of isolated components.

• Development and Reproduction
• /
• v.2 no.1
• /
• pp.101-109
• /
• 1998

Spermatogenesis and reproductive cycle of the razor clam, solen grandis, were investigated monthly by histological and cytological observations. Samples were collected from natural intertidal population at Oshik-do, Kunsan, Korea, for one year, beginning from January to December, 1993. solen grandis is dioecious. Morphological structures of the spermatozoon of this species ar esimilar to those of other bivalve spermatozoa having a primitive type; i.e., a small head, a cap-shaped acrosome and a short mid-piece with four mitochondria surrounding axial filament. The head of spermatozoon is approximately 2 \mu m in length and sperm tail is about 20 \mu m long. The axoneme of tail flagellum consists of nine pairs of peripheral microtubules at the periphery and a pair of central microtubules at the center. Four spherical mitochondria form the paranucleus. Spawning occures once a year between early June and July, and the main spawning was observed in July when seawater temperature reaches above 20 \circ C. The reproductive cycle of male razor clam can be divieded into fivesuccessive stages; early active (December to january), late active (January to march), mature (March to early August), partially spawned (June to July), and spent/inactive stage (August to December).

• Korean Journal of Veterinary Research
• /
• v.32 no.3
• /
• pp.281-293
• /
• 1992

Classification of the cycle of seminiferous epithelia into 12 stages by the morphological changes in acrosomal system and evaluation of the relative frequency of stages and the cell association were histologically performed in the mature Korean native Jin-do dogs. The results were summarized as follows; 1. The minimum number of type A spermatogonia averaged 1.01 at stages I, while maximum number averaged 2.47 at stages XII. Some type A spermatogonia divided at stage XII to produce the type intermediate(IN) spermatogonia at the following stage I. The type IN spermatogonia divided at stage IV to produce the type B spermatogonia at stage V. 2. The type B spermatogonia divided at stage VI to produce the preleptotene primary spermatocytes at stage VII. The secondary spermatocytes observed at stage XII. The secondary spermatocytes observed at stage XII divided to give rise to the round spermatids at the following stage I. The numbers of the first spermatocytes and spermatids were almost constant, respectively, through all the cycles of seminiferous epithelium. 3. The acrosomal vesicle was invaginated to occupy one third to half of spermatid nucleus at the cap phase, which was different from that of rodent and ruminant spermatid nuclei. 4. The relative frequencies of stages I to XII of seminiferous epithelia cycle were 10.34, 4.84, 5.03, 8.22, 10.86, 6.63, 6.42, 18.88, 10.17, 6.18, 7.62% and 4.81%, respectively.