• 한국수정란이식학회지
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• 제20권3호
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• pp.191-200
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• 2005

체외 배양 과정 중에 나타나는 생쥐 초기 2-세포 배의 "in vitro 2-cell block" 현상은 세포내 $Ca^{2+}$ 농도 변화와 밀접한 관련이 있다. 다양한 종류의 세포에서 acetylcholine은 세포막에 존재하는 muscarnic acetylcholine receptor를 통해 세포내 $Ca^{2+}$ 농도 증가를 유도한다. 본 실험에서는 생쥐 "in vitro 2-cell block" 현상에 있어서 ACh의 영향을 알아보기 위해 세포 내 $Ca^{2+}$ 농도 조절 물질을 처리한 후, 공초점 현미경을 이용하여 세포 내 $Ca^{2+}$ 농도 변화를 기록하였다. ACh은 세포 내에서 농도 의존적으로 $Ca^{2+}$ 농도 증가를 유도하며, "in Vitro 2-cell block" 현상을 극복하여 포배기로 발생을 유도하였다. ACh에 의한 $Ca^{2+}$ 농도 증가가 세포막에 존재하는 ACh receptor를 경유하여 나타나는 반응인지를 알아보기 위해 ACh receptor의 저해제인 atropine을 전처리한 결과, ACh에 의한 $Ca^{2+}$ 농도 증가가 완전히 저해되었다. 초기 2-세포 배에서 ACh이 결합하는 receptor의 종류를 확인하기 위하여 carbachol과 nicotin tartrate를 처리 하였다. Nicotinic AChR의 agonist인 nicotine tartrate 1 mM은 세포내 $Ca^{2+}$ 농도 증가를 보이지 않았다. 따라서 초기 2-세포 배의 세포막에는 muscarnic AChR가 기능적으로 작용함을 알 수 있다. ACh에 의한 세포내 $Ca^{2+}$ 농도 증가가 $Ca^{2+}$이 제거된 배양액에서도 나타나는 것으로 보아 ACh에 의한 세포내 $Ca^{2+}$ 변화는 주로 소포체와 같은 세포내 $Ca^{2+}$ 저장고로부터 분비됨을 알 수 있었다. 이러한 세포내 $Ca^{2+}$ 저장고로부터의 $Ca^{2+}$ 분비가 어떤 신호전달체계를 통해 나타나는 지를 조사하였다. 세포막의 PLC 저해제인 U73122를 전처리한 배는 ACh에 의한 $Ca^{2+}$ 농도 증가가 나타나지 않았으며, 세포 내 $Ca^{2+}$ 통로인 IP3R와 RyR의 저해제인 xestospongin과 heparin 혹은 dantrolene을 전처리한 결과 dantrolene에 의해 세포내 $Ca^{2+}$ 농도 증가가 억제되었다. 그리고 세포내 반복적인 $Ca^{2+}$ 농도 증가에 의해 활성도가 변화는 CaMKII의 작용을 확인하기 위하여 Ca MKII의 저해제인 KN-93을 전처리한 결과 $Ca^{2+}$ 농도 증가가 억제되는 것을 확인하였다. 이상의 결과로부터 ACh은 생쥐 초기 2-세포 배에서 ryano-dine receptor를 통하여 세포내 $Ca^{2+}$ 저장고로부터 $Ca^{2+}$ 분비를 유도하며, CaM KII에 의해서도 영향을 받는 것으로 보여진다. 생쥐 초기 2-세포 배에서 "in vitro 2-cell block"의 극복은 ACh에 의해 유도된 신호전달체계를 통해 세포내에 증가하는 $Ca^{2+}$ 농도 및 이에 따른 세포내 대사 작용의 활성화에 의하여 나타나는 것으로 생각된다.

• 한국발생생물학회:학술대회논문집
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• 한국발생생물학회 2003년도 제3회 국제심포지움 및 학술대회
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• pp.7-8
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• 2003

Since it was first reported in 1997, somatic cell cloning has been demonstrated in several other mammalian species. On the mouse, it can be cloned from embryonic stem (ES) cells, fetus-derived cells, and adult-derived cells, both male and female. While cloning efficiencies range from 0 to 20%, rates of just 1-2% are typical (i.e. one or two live offspring per one hundred initial embryos). Recently, abnormalities in mice cloned from somatic cells have been reported, such as abnormal gene expression in embryo (Boiani et al., 2001, Bortvin et al., 2003), abnormal placenta (Wakayama and Yanagimachi 1999), obesity (Tamashiro et ai, 2000, 2002) or early death (Ogonuki et al., 2002). Such abnormalities notwithstanding, success in generating cloned offspring has opened new avenues of investigation and provides a valuable tool that basic research scientists have employed to study complex processes such as genomic reprogramming, imprinting and embryonic development. On the other hand, mouse ES cell lines can also be generated from adult somatic cells via nuclear transfer. These 'ntES cells' are capable of differentiation into an extensive variety of cell types in vitro, as well assperm and oocytes in vivo. Interestingly, the establish rate of ntES cell line from cloned blastocyst is much higher than the success rate of cloned mouse. It is also possible to make cloned mice from ntES cell nuclei as donor, but this serial nuclear transfer method could not improved the cloning efficiency. Might be ntES cell has both character between ES cell and somatic cell. A number of potential agricultural and clinical applications are also are being explored, including the reproductive cloning of farm animals and therapeutic cloning for human cell, tissue, and organ replacement. This talk seeks to describe both the relationship between nucleus donor cell type and cloning success rate, and methods for establishing ntES cell lines. (중략)

• 한국가축번식학회지
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• 제18권2호
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• pp.87-94
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• 1994

본 연구는 생쥐 초기배 및 부화후 체외신장에 미치는 인간 양수의 첨가효과를 조사하고자 실시하였다. 생쥐 수정란의 체외발달에 미치는 인간 양수의 적정농도를 확인하고자 기본배양액 (Whitten's medium)에 16주령의 양수 농도를 각각 달리하여 체외배양을 실시한 결과, 20%를 첨가한 구에서 가장 높은 배반포로의 발달율과 부화율을 나타내었으며, 그 이상의 농도에서는 배발달율이 저하되었다. 포유동물 수정란 체외배양시 가장 많이 사용되는 첨가제인 fetal calf serum (FCS)과 bovine serum albumin(BSA)을 첨가한 구화의 배발달 성적을 비교한 결과, 임신중기 양수를 20% 첨가한 구의 배반포로의 발달율 (92.8%)과 부화율 (75.7%)은 기본배양액에서 배양된 것보다 배반포로의 발달율 (82.8%)과 부화율 (31.3%)은 높았으나 0.3% BSA (90.5%, 70.8%)나 10% FCS 첨가구 (94.3%, 74.3%)와는 유의한 차이가 인정되지 않았다. 임신주령에 따른 양수의 첨가효과를 조사한 결과 20%의 임신말기 양수를 첨가한 구의 배반포로의 발달율 (71.9%)과 부화율 (57.3%)은 20% 임신중기 양수를 첨가한 구보다 낮았으며, 부화후 배의 체외신장은 임신중기 양수와 FCS이 첨가된 구에서는 유기되었으나, 임신말기 양수와 BSA가 첨가된 구에서는 배의 체외신장이 유기되지 않았다. 이상의 본 연구결과를 통해 임신중기 양수 내에는 배발달 촉진인자와 배의 체외신장을 유기시키는 물질이 함유되어 있어 포유동물 배의 체외배양에 상당한 영향을 미치고 있다고 사료된다.

• Clinical and Experimental Reproductive Medicine
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• 제22권2호
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• pp.191-201
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• 1995

Transcriptional activation of the embryonic genome initiates at 2-cell stage in mouse embryo and is characterized by the synthesis of TRC which is restricted to 2-cell stage. To investigate the roles of various protein kinases on the embryonic gene activation, the effects of protein kinase inhibitors on in vitro development and protein synthetic profiles of the early mouse embryos were examinded. None of ${\alpna}-amanitin$ which is a mRNA synthetic inhibitor, H8 which is a PKA inhibitor, and H7 which is a PKC inhibitor, affected on first cleavage of mouse 1-cell embryos in vitro. However, all of these drugs inhibited the second cleavage. When the drugs were removed following treatment for 6 hours, H8 or H7 treatment showed little inhibition on subsequent development of 1-cell embryos to 2-cell stage or further. In contrast, ${\alpna}-amanitin$ irreversibly inhibited the development of 1-cell embryos to 2-cell stage following removal of the drug. Genistein, a TPK inhibitor, inhibited both the first cleavage of 1-cell embryos and the second cleavage of 2-cell embryos, suggesting that TPK activity may be important during the early cleavages. All of the above four drugs inhibited TRC synthesis as shown by the fluorographic analysis of $[^{35}S]-Met$ labeled protein profiles. When late 1-cell embryos were treated with H7 and analyzed synthetic patterns of $[^{35}S]-Met$ labeled protein, the quantitative differences of protein synthesis on SDS-PAGE appeared on 77 kD and 33 kD region at $32{\sim}38$ hours post hCG. From these studies, transcriptional activation of embryonic genome is not essenting to the mouse 1-cell embryos to develop to 2-cell stage. Hawever, TPK activity is reguisite for both the first cleavage and second cleavage. Similarly, both PKC and PKA activities are required for the second cleavage of mouse embryos, but not for the first cleavage.

• 한국수정란이식학회지
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• 제15권3호
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• pp.247-253
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• 2000

This study was undertaken to optimize enucleation and reconstitution methods for the production of cloned mice by somatic cell nuclear transfer Outbred ICR mouse oocytes at the metapahse- II stage were retrieved from female mice superovulated by PMSG and hCG. In Experiment 1, oocytes were enucleated in medium supplemented with cytochalasin B (CCB) of 3 levels (0, 7.5 or 15 $\mu\textrm{g}$/mL), and higher rate of encleation was obtained at 7.5 and 15 $\mu\textrm{g}$/mL than at $\mu\textrm{g}$/mL. In Experiment 2, oocytes enucleated in 7.5 $\mu\textrm{g}$/mL CCB-containing medium were reconstituted with different types of somatic cell by following methods; 1) cumulus cells by direct cell injection, 2) cumulus cells by electric fusion (1.25 kV/cm, 2 pulses for each 70 $mutextrm{s}$) or 3) STO cells by the electrofusion. Electrofusion of STO cells with enucleated oocytes yielded the greatest (P<0.05) rate of reconstitution without lysis (76%) than any other combinations. Although significant decrease in the rate of somatic cell introduction was found, the electrofusion of cumulus cells yielded better rate of reconstitution than direct injection (0 vs. 18%). In Experiment 3, the duration of electric stimulation for the fusion was changed to either 50 $mutextrm{s}$ or 90 $mutextrm{s}$, but no significant improvement of reconstitution efficacy was obtained. In conclusion, this study showed that ICR mouse oocytes could be used for the production of reconstituted oocytes and a fusion method of 1.25 KV/cm with 2 pulses using 570 cell was the optimal.

• 한국수정란이식학회지
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• 제12권3호
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• pp.283-291
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• 1997

In vitro development of bovine embryos is affected by many factors such as energy substrates, amino acids, and some growth factors. It has been reported that mRNA of insulin, PDGF and their receptors are detected in cow embryos, and that some chelating agents such as EDTA and transferrin have beneficial role on mouse and bovine embryos. The author hypothesized that insulin, transferrin arid PDGF added to a culture medium increase in vitro development of bovine embryos by chelating toxic substance(s) or increasing cell growth and metabolism. Immature oocytes from slaughtered ovaries of Holstein cows and heifers were matured for 24 hours in a TCM199 containing 10% fetal calf serum, FSH, LH and estradiol with granulosa cells in vitro. Matured oocytes were coincubated with sperm for 30 hours in a modified Tyrode's medium (IVF). Embryos cleaved to 2- to 4-cell at 30 hours after IVF were selected and cultured in a 30-$\mu$l drop of a synthetic oviduct fluid medium (SOFM) containing 0.8% BSA, Minimum Essential Medium essential and non-essential amino acids, and insulin, transferrin or PDGF for 9 days. Supplementation of a SOFM with insulin, and /or transferrin did not increase develop-mental rate to expanding and hatching blastocyst of 2- to 4-cell bovine embryos compared with control. The highest developmental rate to hatching blastocyst was shown when PDGF was added at the concentration of 10 ng /ml among the supplementing doses tested in the present study (p<0.05). Addition of PDGF without insulin to a SOFM could not increase embrye development, but combined addition of PDGF with insulin significantly increased (p<0.05) embryo development to hatching blastocyst (50%) compared with control (38%). In conclusion, insulin and PDGF supplemented to a SOFM may act synergistically and have beneficial effect on in vitro development of 2- to 4-cell bovine embryos matured and fertilized in vitro.

• 한국수정란이식학회:학술대회논문집
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• 한국수정란이식학회 2002년도 국제심포지엄
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• pp.94-94
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• 2002

Lactadherin (formerly known as BA46), a major glycoprotein of the human milk fat globule membrane, is abundant in human breast milk and breast carcinomas and may prevent symptomatic rotavirus infections. In this study, under the control of mouse whey acidic protein (WAP) promoter, the expression pattern of lactadherin (Ltd) in lactogenic hormone-dependent mouse mammary epithelial cell line HC11 were tested. pLNWLtd construct containing 2.4 kilobases of the WAP promoter and 1.5 kilobases of human lactadherin gene was stably transfered into HC11 cells using retroviral vector system. Integration and expression level of the transgene was estimated using PCR and RT-PCR, respectively. Prominent induction of Ltd gene under the WAS promoter was accomplished in the presence of insulin, hydrocortisone and prolactin, while induction with insulin alone resulted in lower expression. Our results demonstrate that the expression of the transgene is increased by synergistic effect of several lactogenic hormones, including insulin, hydrocortisone, and prolactin.

• 한국동물번식학회:학술대회논문집
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• 한국동물번식학회 2003년도 학술발표대회 발표논문초록집
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• pp.52-52
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• 2003

Granulocyte-macrophage colony stimulating factor (GM-CSF) is synthesized in the female reproductive tract and has been shown to play an important role in human and murine embryo development and implantation. However, the mechanism of GM-CSF on the embryo development is unknown. Recent studies suggested that GM-CSF may be increase the expression of implantation relented genes, such as interleukin-1 (IL-1) system. Our aim of this study was to compare the interleukin-1$\alpha$ (IL-1$\alpha$), interleukin-1$\beta$ (IL-1$\beta$) and interleukin-1 receptor antagonist (IL-lra) mRNA between the GM-CSF supplemented group and control group in mouse embryos. Mouse 2-cell embryos were cultured in P-1 medium supplemented with or without mouse GM-CSF (10 ng/ml). The number of total and apoptotic cell in blastocyst were assessed by TUNEL. And then, the expression of IL-1$\alpha$, IL-1$\beta$ and IL-1ra mRNA in blastocyst were examined by RT-PCR.

• Clinical and Experimental Reproductive Medicine
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• 제45권3호
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• pp.110-115
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• 2018

Objective: To compare our in-house method of embryo freezing with Cryotop vitrification in terms of immediate survival, subsequent cleavage and blastocyst formation, and cell numbers in blastocysts. Methods: Two-cell mouse embryos were randomly allocated into three groups: a non-frozen control group (group 1, n = 300), a group that underwent Cryotop vitrification (group 2, n = 300), and a group that underwent our in-house freezing method (group 3, n = 300). Results: There were no significant differences between groups 2 and 3 in the immediate survival rate (96.3% vs. 98.6%, respectively; p= 0.085), the further cleavage rate (91.7% vs. 95.0%, respectively; p= 0.099), or the blastocyst formation rate (80.7% vs. 78.6%, respectively; p= 0.437). The cell numbers in the blastocysts from groups 1, 2, and 3 were comparable ($88.99{\pm}10.44$, $88.29{\pm}14.79$, and $86.42{\pm}15.23$, respectively; p= 0.228). However, the percentage of good-quality blastocysts in the Cryotop vitrification group was significantly higher than in the group in which our in-house method was performed, but was lower than in the control group (58.0%, 37.0%, and 82.7%, respectively; p< 0.001). Conclusion: At present, our method is inferior to the commercial Cryotop vitrification system. However, with further improvements, it has the potential to be useful in routine practice, as it is easier to perform than the current vitrification system.

• Clinical and Experimental Reproductive Medicine
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• 제42권3호
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• pp.94-100
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• 2015

Objective: The goal of this study was to ascertain optimal assisted hatching (AH) method in frozen embryo transfer. We compared the effect of depending on whether mechanical or laser-AH was performed before or after the vitrification of embryo development rate and blastocyst cell numbers. Methods: In order to induce superovulation, pregnant mare's serum gonadotropin followed by human chorionic gonadotropin were injected into 4- to 5-week-old female mice. 2-cell embryos were then collected by flushing out the oviducts. The Expanded blastocysts were recovered after the collected embryos were incubated for 48 hours, and were then subjected to artificial shrinkage (AS) and cross-mechanical AH (cMAH) or quarter-laser zona thinning-AH (qLZT-AH) were carried out using the expanded blastocysts before or after vitrification. After 48 hours of incubation, followed by vitrification and thawing (V-T), and blastocysts were fluorescence stained and observed. Results: The rate of formation of hatched blastocysts after 24 and 72 hours of incubation was significantly higher in the AS/qLZT-AH/V-T group than in the other groups (p<0.05). The cell number of the inner cell mass was higher in AS/V-T/non-AH and AS/V-T/cMAH groups than those of others (p<0.05). In the control group, the number of trophectoderm and the total cell number were higher than in the AS-AH group (p<0.05). Conclusion: The above results suggest that AS and AH in vitrification of expanded blastocysts lead to the more efficient formation of hatched blastocysts in mice.