• 한국가축번식학회지
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• 제21권3호
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• pp.287-292
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• 1997

This study was carried out to investigate the effects of concentration and kinds of cryoprotectants, equilibraction time, thawing temperature and time, sucrose concentration on the survival rates of frozen bovine demi-embryos. The bovine demi-embryos following dehydration by cryoprotectants a various concentration of sucrose were freezed by cell freezer and thawed in 3$0^{\circ}C$ water bath. Survival and in vitro developmental rates was defined as development rates on in vitro culture or FDA-test. The results are summarized as follows : 1. The high survival rates of demi-embryos after frozen-thawing in freezing medium was attained 2.0M glycerol. The high survival rates of demi-embryos after frozen-thawing in freezing medium was obtained using single cryoprotectant(25.0~30.0%) than mixed cryoprotectants(16.7~19.0%). 2. The survival rates of demi-embryos after frozen-thawing in freezing medium added 1.5M, 2.0M glycerol＋0.25M sucrose(37.5~33.3%) were higher survival rates than those of sucrose concentration of 0.50, 0.75M(12.5~26.7%). 3. The equilibration time on the survival rates of demi-embryos was attained after short period of time(30.0~35.0%) in the freezing medium higher than long period of time(21.1%). 4. The thawing temperature on the survival rates of demi-embryos was attained at 3$0^{\circ}C$ of thawing temperature(26.7~40.0%) higher than $25^{\circ}C$ or 37$^{\circ}C$ of thawing temperature(13.3~20.0%). 5. The thawing time on the survival rates of demi-embryos was attained at 1~5 minutes of thawing time(26.7~33.3%) in the freezing medium higher than 10 minutes of thawing time(13.3~18.8%).

• Clinical and Experimental Reproductive Medicine
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• 제24권3호
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• pp.325-333
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• 1997

The use of hormonal stimulation in human in vitro fertilization and embryo transfer (IVF-ET) leads to increased production of embryos for ET. So to avoid high pregnancies and to allow conception in future, unstimulated cycles, cryopreservation of spare embryos is desirable. One of the improvement of cryopreservation methods is vitrification. We cryopreserved mouse day 3 embryos by vitrification using the three different vitrification solution (EFS40, VS11 and VS3a). EFS40 solution is consisted of 40% (v/v) ethylene glycol, Ficol170 30% (w/v) and 0.5M sucrose and VS11 is 6.0M ethylene glycol and 1.8M glycerol. And VS3a is 6.5M glycerol and 6% (w/v) BSA (bovine serum albumin). First we tested the toxicity of three vitrification solution by exposure to these solution during 3 min. After washing by thawing solution, the survival rates of each groups are 95.5%, 90.9% and 84.4% (EFS40, VS11 and VS3a). High percentages of them developed to expanded blastocyst and hatching embryos in culture 48hrs 94.2%, 97.7%, 100% and 97.4% (no treatment group, EFS40, VS11 and VS3a). So there is no significant differences among the each group. Second, after thawing of vitirfied embryos, the survival rates of each groups are 96.8% (slow freeze), 94.1% (EFS40), 85.5% (VS11) and 80.0% (VS3a, P vs. no freeze or EFS40 is 0.01). Vitrified embryos exhibited a high rate of development in vitro after 48hrs culture. The percentages of each group to blastocyst and hatching embryos are 88.7% (no freeze), 91.8% (slow freeze), 93.4% (EFS40), 87.7% (VS11) and 73.0% (VS3a, P vs. other group is 0.01). The results suggest that there is no significant differences in exposure of various vitrification solution and day 3 mouse embryos can be vitrified in solution EFS40 and VS11 by simple procedure.

• 한국수정란이식학회지
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• 제21권3호
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• pp.255-262
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• 2006

본 연구는 Open Pulled Straw(OPS)방법에 의해 동결-융해한 돼지 수정란의 체외 생존 능력을 검토하기 위하여 수행되었다. 미성숙 난자의 체외 성숙을 위하여, 돼지 난소는 도축장에서 회수하였으며, 난구세포로 쌓여있는 난자는 직경 $2{\sim}6mm$의 난포로부터 난포액과 함께 흡입에 의하여 회수하였다. 회수된 미성숙 난자의 체외 성숙을 위하여 5 mM hypotaurine, 0.57 mM cysteine, 10% 난포액, 10 IU/ml PMSG 및 10 IU/ml hCG가 함유된 NCSU-23 배양액 내에서 $21{\sim}22$ 시간 배양 후, 호르몬 물질을 제거한 성숙 배양액 내에서 $21{\sim}22$ 시간 동안 추가 배양하였다. 한편 체외 수정을 위하여 동결-융해한 정액은 5.56 mM glucose, 0.33 mM na-pyruvate, 100 IU/ml penicillin, $100 {\mu}g/ml$ streptomycin 및 4 mg/ml BSA가 첨가된 D-PBS 액을 가지고 1,500 rpm에서 10분간 2회 원심분리를 실시하여 세척하였다. 체외 수정을 위한 배양액은 pH $7.2{\sim}7.4$에서 2 mM caffeine과 2 mg/ml BSA가 첨가된 mTBM 배양액을 이용하였다. 체외 수정시 정자의 최종 농도는 $2.5{\times}10^6cells/ml$로 조정하였다. 수정 8시간 후, 체외 발육을 위하여 5.0 mM hypo-taurine, 4 mg/ml BSA 및 10 ng/ml EGF가 첨가된 NCSU- 23액으로 옮겨 7일간 배양을 계속하였다. 그 후 배반포의 여러 단계에서 OPS 법에 의해 동결-보존하였다. 그 결과, 동결-융해 후 형태학적으로 정상적인 수정란의 비율은 초기 배반포(28.3%)보다는 확장 배반포(38.9%)단계에서 동결했을 때 유의적으로 높게 나타났다(p<0.05). 한편, 동결-융해 후 상해를 입은 수정란의 비율은 확장 배반포보다는 초기 배반포 단계에서 동결된 수정란에서 유의적으로 높은 성적을 보였다(p<0.05). 또 다른 실험에서, 수정란의 동결-융해 후 형태학적으로 정상인 수정란을 48시간 추가 배양했을 때, Hatching 된 수정란의 비율은 초기 배반포, 배반포 및 확장배반포기 단계에서 동결-융해한 수정란에서 각각 6.7, 20.0 및 33.3%로 발육 단계가 높을수록 동결-융해 후의 생존율도 높게 나타났다. 본 연구의 결과로부터, 돼지에서 수정란의 동결-융해 후 생존성의 향상을 위해서는 발육 단계가 높은 배반포기 단계에서의 동결이 요구되며 본 연구에서 이용된 OPS 동결 방법이 폭넓게 활용될 것으로 사료된다.

• 한국수정란이식학회지
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• 제9권2호
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• pp.181-188
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• 1994

• Toxicological Research
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• 제22권2호
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• pp.127-133
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• 2006

Recently, we have reported that the environmental pollutant 2-bromopropane (2-BP) induces a significant embryo-fetal developmental toxicity in rats. However, the cause of developmental toxicity and the relationship between maternal and developmental toxicities could not be elucidated because the developmental toxicity of 2-BP was observed only in the presence of maternal toxicity The in vitro teratogenicity study using whole embryo culture was carried out to understand the teratogenic properties and the possible mechanism of teratogenicity induced by 2-BP in rats. Rat embryos aged 9.5 days were cultured in vitro for 48 hrs at medium concentrations of 0, 1, 3, or 10 mg/ml of 2-BP. Embryos were evaluated for growth, differentiation, and morphological alterations at the end of the culture period. At 10 mg/ml, 2-BP caused a delay in the growth and differentiation of embryos and an increase in the incidence of morphological alterations, including altered yolk sac circulation, abnormal axial rotation, craniofacial hypoplasia, open neuropore, absent optic vesicle and kinked somites. At 3 mg/ml, only a delay in the growth and differentiation of embryos was observed. There were no adverse effects on embryonic growth and development at the concentration of 1 mg/ml. The results showed that the exposure of 2-BP to rat embryos results in a developmental delay and morphological alterations at dose levels of 3 mg/ml culture media or higher and that 2-BP can induce a direct developmental toxicity in rat embryos.

• Asian-Australasian Journal of Animal Sciences
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• 제22권7호
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• pp.969-976
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• 2009

Use of oocytes from prepubertal animals for in vitro embryo production holds potential application for reducing generation intervals and increasing genetic progress through embryo transfer. The objective of these studies was to compare the effect of three sperm pretreatments (prior to in vitro fertilization) and seven embryo culture protocols on fertilization rate and (or) subsequent development of in vitro fertilized embryos derived from oocytes harvested from ovaries of 1-6 month old prepubertal Boer goats in China. Cleavage rates were highest for embryos fertilized with heparin-treated versus calcium ionophore- or caffeine-treated sperm. Similar rates of blastocyst development were observed using heparin- and ionophore-treated sperm, which were higher than obtained with caffeine-treated sperm. No differences in cleavage or blastocyst rates were observed following embryo culture in basal medias (synthetic oviductal fluid (SOF), Charles Rosenkrans 1 (CR1) or tissue culture medium-199 (TCM-199)) containing 10% fetal bovine serum (FBS). Cumulus or oviductal cell co-culture did not enhance cleavage or blastocyst rates relative to culture in SOF+10% FBS. Replacement of FBS in SOF medium with 0.3% BSA increased cleavage rates, but did not increase rates of blastocyst development. Sequential culture in SOF+0.3% BSA followed by SOF+10% FBS increased blastocyst yield versus continuous culture in SOF+10% FBS and tended to increase blastocyst yield versus continuous culture in SOF+0.3% BSA. These results demonstrate a pronounced effects of sperm pretreatments and in vitro embryo culture systems on rates of blastocyst development and provide a potential protocol (sperm pretreatment with heparin and sequential embryo culture in SOF+0.3% BSA followed by SOF+10% FBS) for generation of the significant numbers of in vitro produced blastocysts from oocytes of prepubertal Boer goats necessary for application of embryo transfer in rural regions of China for distribution of Boer goat genetics.

• Current Research on Agriculture and Life Sciences
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• 제7권
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• pp.83-97
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• 1989

본 실험은 일정한 발달단계(發達段階)에 있는 생쥐배(胚)를 응집시킬때 세포응집소인 Phytohemagglutinin-P(PHA-P)를 첨가 라화배(裸化胚)의 응집율과 응집된 배(胚)를 in vitro에서 배양하였을때의 배양율 및 적당한 PHA-P의 첨가농도를 조사하여 Chimera배(胚)를 생산하는데 필요한 기초지식을 얻기 위하여 실시(實施)하였다. Albino BALB/C와 CBA계통 및 C57BL 계통의 생쥐에 pregnant mare Serum gonadotropin와 human chorionic gonadotropin를 투여하여 과배란 생쥐에 PMSG와 hCG를 투여하여 과배란을 유기, 회수된 생쥐의 4세포기, 8세포기 및 상실배기 수정란을 1.0% Protease 용액으로 투명대를 제거(除去)하고 PHA-P를 첨가한 배양액에서 미세한 초자봉(硝子棒)으로 계통(系統)이 다른 두 계통(系統)의 생쥐의 배(胚)를 응집시킨 다음 응집된 배를 $37^{\circ}C$, 5% $CO_2$, 95% Air의 배양기 조건하에서 13~50 시간 배양하면서 Chimera배(胚)의 발달상태를 조사하였다. 본(本) 실험에서 얻어진 결과를 요약하면 다음과 같다. 1. 1.0% Protease 또는 1.0% Protease 및 $5ug/m{\ell}$ PHA-P가 첨가된 산성 Tyrode액에서 투명대를 제거한 라화배(裸化胚)를 배반포까지 배양했을때 유의차는 없었으나 4세포기배와 8세포기배 보다 상실기배가 더 잘 발달되었으며 또한 PHA-P를 첨가하였을때가 첨가하지 아니한 때 보다 다소 좋은 경향을 보였다. 2. PHA-P $2ug/m{\ell}$첨가시 4세포기, 8세포기 및 상실기배의 응집율은40.0~82.0%, $5ug/m{\ell}$첨가시에는 52.0~94.0%, $10ug/m{\ell}$ 첨가시에는 48.0~96.0%로 배(胚)의 발달단계(發達段階)에 따라서는 4세포기, 8세포기가 상실배기 보다 유의적으로 높았다 (P<.05). PHA-P의 처리수준에 의한 응집율에 있어서는 5 또는 $10ug/m{\ell}$첨가구가 $2ug/m{\ell}$첨가구 보다 조금 높게 나타났으나 유의차는 없었다. 3. 응집배의 상실배까지의 배양율은 PHA-P의 각(各) 수준간 및 각(各) 세포기간에 유의차가 인정되지 않았다. 응집배의 배반포까지의 배양율은 PHA-P 수준사이에는 유의차가 없었으나 4세포기와 8세포기의 배(胚)는 상실기 배(胚)보다 유의적으로 높은 배양율을 보였다 (P<.05). 4. 응집된 배(胚)가 배반포까지 발달하는데 소요되는 평균시간은 4세포기배가 38.5~40시간, 8세포기배가 26~27시간, 상실기배가 19~20시간이었다. 5. 응집율은 34.0~94.0%의 범위로서 PHA-P를 첨가할때 응집율이 더 좋은 경향을 보였으나 유의성은 인정되지 않았다. 4세포기와 8세포기의 배(胚)가 상실기배 보다 유의적으로 높았다(P<.05). 6. 응집배의 상실배까지의 발달율은 4세포기배가 52.7~84.7%, 8세포기배가 73.8~872% 였으며 세포기 사이에는 유의차는 나타나지 않았다. 그러나 PHA-P를 첨가한 것이 발달이 더 좋았다. 7. 응집배의 배반포까지의 발달율은 4세포기의 배(胚)가 41.7~77.7%, 8세포기의 배(胚)는 78.7~83.0% 상실기배가 0~19.2%였으며 4세포기의 PHA-P 처리가 미처리(未處理) 보다 유의적으로 높았다(P<.05). PHA-P를 처리했을 때 4세포기와 8세포기가 상실기의 배(胚) 보다 더 높은 발달율을 보였다.

• Asian-Australasian Journal of Animal Sciences
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• 제20권6호
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• pp.842-849
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• 2007

The purpose of the present study was to produce live offspring from in vitro fertilized goat embryos. Oocytes were collected from abattoir ovaries and kept in oocyte collection medium. Oocytes were washed 4-5 times with maturation medium containing medium-199 with 5 ${\mu}g/ml$ FSH, 100 ${\mu}g/ml$ LH, 1 ${\mu}g/ml$ estradiol-$17{\beta}$ 50 ${\mu}g/ml$ gentamycin, 10% inactivated estrus goat serum, and 3% BSA (fatty acid free). Oocytes were placed in 100 ${\mu}l$ drops of maturation medium containing granulosa cell monolayer and incubated in a 5% $CO_2$ incubator at $38.5^{\circ}C$ for 27 h. For capacitation of spermatozoa fresh semen was processed and mixed in 3 ml fertilization TALP medium containing 50 ${\mu}g/ml$ heparin and kept in the above incubator for 2 h. The capacitated spermatozoa were coincubated with matured oocytes for fertilization. Cleaved embryos were separated and cultured in embryo development medium with oviductal cells and 494 embryos were produced. Recipient goats were synchronized with two injections of 15 mg $PGF_{{2}{\alpha}}$/goat 10 days apart. Eighty early stage embryos were transferred into the uterotubal junction of 14 surrogate mothers using laparoscopy techniques. One recipient delivered twin kids, whereas another two recipients each.delivered a single kid The parentage of these kids was evaluated using highly polymorphic co-dominant microsatellites markers. From the present study, it was concluded that live goat kids can be produced from in vitro matured and fertilized goat embryos, to the best of our knowledge for the first time in India.

• Reproductive and Developmental Biology
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• 제35권2호
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• pp.191-195
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• 2011

The present study was conducted to examine the reactive oxygen species (ROS) generation levels in porcine parthenogenetic embryos. Porcine in vitro matured oocytes were activated by the combination of electric stimulus and 6-DMAP before in vitro culture. Porcine oocytes and parthenogenetic embryos were stained in 10 ${\mu}M$ dichlorohydrofluorescein diacetate (DCF) or 10 ${\mu}M$ hydroxyphenyl fluorescein (HPF) dye each for 30 min at $39^{\circ}C$. The fluorescent emissions from the samples were recoded as JPEG file and the intensity of fluorescence in oocytes and embryos were analyzed. $H_2O_2$ and $^{\cdot}OH$ radical levels of porcine oocytes were reduced immediately after electric stimulation. However, $H_2O_2$ and $^{\cdot}OH$ radical levels of parthenogenetic embryos were increased with time elapsed after electric stimulation from 0 h to 3 h and after DMAP culture. During in vitro culture, $H_2O_2$ and $^{\cdot}OH$ radical levels were gradually increased from the one-cell stage to the two- and four-cell stages. The result of the present study suggests that the ROS was not increased by electric pulse in porcine embryos. Rather than it seems to be associated with the stage of development and the culture condition.

• 한국수정란이식학회지
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• 제11권2호
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• pp.111-124
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• 1996

The present study was carried out to investigate the effects of co-culture cells and growth factors on in vitro culture of Korean native cattle(KNC) embryos fertilized in vitro. Two-eight cell embryos were cultured in vitro using 4 types of co-culture cells and 3 growth factors singly or in combination. The results were as follows, In the co-culture of 2~8 cell embryos with bovine oviductal epithelial cell(BOEC), granulosa cell(BGC), uterine epithelial cell(BUEC) and mouse embryonic fibroblast (MEF) monolayers, the developing rate to blastocysts was significantly(P<0.05) higher with BUEC(32.1%) than with MEF(15.3%), BGC(13.2%) and non co-culture control(11.6%). When the morula co-cultured with BOEC for 5 days following in vitro fertilization were co-cultured with BOEC continuously or with BUEC, respectively, the developing rate to blastocysts was higher with BUEC(73.9%) than with BOEC(56.0%). To examine the effects of growth factors on in vitro development of 2~8 cell embryos, epidermal growth factor(EGF), transforming growth factor-$\beta$l(TGF-$\beta$l) and insulin-like growth factor-1(IGF-1) were added singly or in combination to TCM 199 maturation medium with respective concentration. In a addition of each 10, 30 and SOng /rnl EGF, the developing rate to blastocysts was the highest in lOng /ml EGF(25.3%). In addition of each 1, 2 and Sng /mi TGF-$\beta$1, the developing rate to blastocysts was the highest in lng /ml TGF-$\beta$1(28.8%). In addition of each 50, 100ng/ml JGF-l, the developing rate to blastocysts was higher in 100ng/ml IGF-l(16.5%) than in SOng/mi IGF-1(12.9%). When lOng /ml EGF and lng /ml TGF-$\beta$l was added singly or in combination, the developing rate to blastocysts was similar in groups added singly or in combination with EGF and TGF-$\beta$l (23.l~24.6%), although higher than in control(16.7%). In the co-culture of 2~8 cell embryos Wth BOEC + each 10, 30 and 5Ong /rnl EGF, the developing rate to blastocysts was significantly(p<0.05) higher in BOEC + long /ml EGF(32.3%) than in BOEC + 3Ong /ml EGF(18.9%) and BOEC + song /ml EGF(9.7%). In the co-culture of 2~8 cell embryos with BOEC + each 1, 2, Sng /ml TGF-$\beta$l the developing rate to blastocysts was higher in BOEC + Sng/rnl TGF-$\beta$l(28.2%) than in BOEC + lng /ml TGF-$\beta$l(21.7%) and BOEC + 2ng/ml TGF-$\beta$l(21.4%). In summary, higher developing rate to blastocysts were obtained with co-culture of BUEC for co-culture system, with addition of lOng /ml EGF or lng /ml TGF-$\beta$l for growth factor culture system, and with co-culture of BOEC + lOng /ml EGF or BOEC + Sng /ml TGF-$\beta$l for co-culture + growth factor culture system.