化学联合激活可明显提高小鼠孤雌胚胎发育率

为探讨一种高效的小鼠卵母细胞孤雌激活的方案,进一步提高孤雌囊胚发育率。用不同浓度的氯化锶及不同作用时间的乙醇,并分别联合6-DMAP对不同卵龄小鼠卵母细胞进行活化,统计小鼠卵母细胞卵裂率和体外发育状况。结果显示,15～16h、18～19h和20～21h卵龄组卵母细胞经6mmol/LSrCl2联合6-DMAP处理后,三组的激活率随卵龄增长而升高,其中20～21h卵龄组显著高于15～16h、18～19h组(P<0.05),激活胚胎的发育率以18～19h时最高;6mmol/L和10mmol/L的SrCl2联合6-DMAP均能有效地激活小鼠卵母细胞,激活率分别为76.4%和83.6%,桑葚胚率分别为50.0%和56.3%;70ml/L乙醇联合6-DMAP以处理7min组获得了较好的激活率和囊胚发育率,分别为77.1%和42.4%,囊胚率均显著高于4min和10min处理组(P<0.05)。6-DMAP与SrCl2或乙醇联合应用可以有效抑制第二极体的排出,提高激活胚的二倍体比率;孤雌囊胚的平均细胞数显著低于正常受精囊胚(P<0.05)。不同激活方案对孤雌活化胚的核型和发育能力的作用差异较大,小鼠卵母细胞孤雌激活率与卵龄...     

6-DMAP对小鼠卵母细胞减数分裂启动及孤雌发育作用

小鼠卵泡卵母细胞体外培养过程中加入2 mmol/L 6-DMAP可抑制卵母细胞自发的染色质浓缩和生发泡破裂(GVBD)。源自超排的MⅡ期卵母细胞则能为6-DMAP所激活。hCG注射后18—19h的卵母细胞置于2 mmol/L6-DMAP的CZB溶液中培养0.5 h、1h、2h、3h,卵母细胞的激活率分别为26.1%、75.2%、75.8%、77.3%、;卵裂率分别为88.2%、73.2%、67.0%、58.4%。与乙醇激活法相比,6-DMAP处理引起了不同的孤雌激活类型。     

两种激活处理促进小鼠孤雌胚胎原核形成

不同人工处理方法激活哺乳动物卵母细胞的机理相似,但其激活效率存在差异。本研究以昆明(KM)、129/Sv×KM F1和C3H×KM F1雌鼠来源的卵母细胞为对象,利用氯化锶(SrCl2,Sr2+)联合细胞松弛素B(cytochalasin B,CB)(Sr2++CB)和离子霉素(ionomycin,Ion)联合6-二甲胺基嘌呤(6-dimethylaminopurine,6-DMAP)(Ion+6-DMAP)两种激活方法处理下对比分析不同品系小鼠卵母细胞的激活效率,并以卵母细胞原核形成率、原核数量和孤雌胚胎体外发育来评价两种激活剂的激活效率。研究结果表明,Ion+6-DMAP激活卵的1原核比率显著高于2原核(p0.05),Sr2++CB激活卵的2原核比率显著高于1原核(p0.05);KM、129/Sv×KM F1和C3H×KM F1各组孤雌胚胎卵裂率和激活率没有显著差异(P0.05),但129/Sv×KM F1和C3H×KM F1囊胚发育率显著高于KM组(p0.05)。3种小鼠品系的卵母细胞用Sr2++CB处理的孤雌胚胎发育率显著高于Ion+6-DMAP。结果证明,Sr2++CB处理小鼠卵母细胞的激活效率明显优于Ion+6-DMAP;129/Sv×KM F1和C3H×KM F1的孤雌胚胎体外发育率显著高于KM小鼠,为研究小鼠遗传背景影响孤雌胚胎发育的机理提供参考。     

应用氯化锶对小鼠卵母细胞孤雌活化的研究

目的　探讨小鼠卵母细胞孤雌激活的最佳作用条件。方法　将MⅡ期小鼠卵母细胞随机分为 2组 ,第一组 ,将小鼠卵母细胞分别放入 2、4、6、8、10mmol ml不同浓度的氯化锶激活液中 ,作用 6h ,观察激活率及囊胚发育率。第二组 ,将小鼠卵母细胞放入 10mmol ml氯化锶激活液中 ,分别作用 3、6、9h ,观察激活率及囊胚发育率。结果　第一组 ,激活率分别为 86 49%、82 6 1%、88 0 0 %、86 6 7%、81 18%。各组间差异无显著性。体内培养 72h回收囊胚 ,囊胚发育率分别为 0、31 42 %、43 33%、6 2 5 0 %、5 0 0 0 %。 6～ 10mmol mlSrCl2 激活液激活后囊胚发育率高于 0～ 4mmol ml(P <0 0 5 )。第二组 ,激活率分别为 82 86 %、89 6 1%、91.40 %。 72h囊胚发育率分别为 2 6 5 3 %、5 0 0 0 %、5 3 2 2 %。激活 6、9h的囊胚发育率高于激活 3h的囊胚发育率 (P <0 0 1)。结论　结果表明 ,6～ 10mmol ml的SrCl2 为卵母细胞孤雌活化的最佳作用浓度 ,6～ 9h的激活时间为最佳作用时间 ;表明SrCl2 的浓度和作用时间对小鼠卵母细胞的活化有显著的影响。     

牛卵母细胞孤雌激活及马-牛异质克隆胚构建

首先用不同的激活剂孤雌激活体外成熟培养的牛卵母细胞,经试验获得:离子霉素、A23187和7%乙醇联合6-DMAP可有效地激活牛卵母细胞,并支持其发育到囊胚,但离子霉素激活效率显著优于其他两种(P<0.05);以10?S SOFaa 颗粒细胞为发育体系培养激活的成熟牛卵母细胞可得到较高的卵裂率和囊胚率(72.30%,14.91%)。其次,通过体外培养成年马皮肤成纤维细胞,将获得的成纤维细胞经血清饥饿培养后,作为核供体移入去核牛卵母细胞透明带下,电融合后,能得到融合的马牛重构胚,在交流电脉冲起始电压20V,持续时间10s,频率0.2MHz,结束电压15V,2次脉冲和融合间隔为0.125s的条件下,当融合电压为2.0kV/cm,脉冲时程为40μs时,重组胚的融合率和卵裂率最高(52.27%,71.74%)。     

不同卵龄小鼠卵母细胞激活和受精的比较研究

本实验比较了不同卵龄的小鼠卵母细胞受酒精人工刺激后的激活率和体外受精率,以探索卵母细胞激活和受精的机制。向NIH雌鼠腹腔注射孕马血清促性腺激素（PMSG）7．5单位,48小时后注射人绒毛膜促性激素（HCG）7．5单位,于不同时间杀小鼠,取卵母细胞与卵丘细胞的复合体（OCC）。从注射HCG后到取OCC的时间视为卵母细胞的卵龄。将OCC置于含8％酒精的M2中7分钟,再在16中培养5小时后,用0．3mg/mL的透明质酸酶去卵丘细胞。卵母细胞形成原核或速即卵裂为激活的标志,将OCC加入已获能的精子悬液中,5小时后将从卵丘细胞中释放出来的卵母细胞转移到M16中,将日发生卵裂为卵母细胞体外受精和激活的标志。小鼠卵母细胞卵龄为20h,其激活率为81．6％,速即卵裂率为48．0％;而卵龄进一步增加到24h,激活率和卵裂率转为下降（Table1）。而卵母细胞受精子激活和受精则不同,卵龄为15h ,卵母细胞的体外受精率为45．4％;随着卵龄的进一步增加,体外受精率则下降（Table2)。Fig.1显示：新排出的卵母细胞容易被精子激活而受精;卵龄较大的卵母细胞较易被酒精的人工刺激而激活。可能是卵母细胞从成熟到老化过程中,细胞的结构、功能及对外界刺激的敏感状态都在发生一些规律性的变化,而激活和受精的机制不完全,还不能精对卵龄的要求要严格。     

显微受精废弃的人类卵母细胞体外成熟及孤雌激活

以卵胞浆单精注射(intracytoplasmic sperm injection,ICSI)后废弃的未成熟人类卵母细胞(生发泡期卵母细胞(the germinal vesicle,GV)和第一次减数分裂中期卵母细胞(the metaphase,MI))为材料,使用卵母细胞体外成熟培养液培养未成熟的卵母细胞,分别在人类绒毛膜促性腺激素(human chorionic gonadotrophin,hCG)注射后45、60、84 h观察卵母细胞成熟情况.分别使用钙离子载体(calcium ionophore,CI)A23187联合6-二甲基氨基嘌呤(6-DMAP)法或精子提取物卵胞质内注射(sperm extracts intracytoplasmic injection,SEII)法两种不同的激活方法对体外成熟MII的卵母细胞进行孤雌激活,评价其体外发育潜能.MI卵子体外成熟率要显著高于GV(75.2%vs 30.6%)(P<0.01).与CI/6-DMAP法相比使用SEII/6-DMAP法在激活率(87.5%vs 70.2%)上要明显高于CI/6-DMAP法(P<0.05),但在卵裂率(65.7%vs 72.5%)和桑囊率(0%vs 5.0%)上SEII/6-DMAP法要低于CI/6-DMAP法.注射hCG 45 h组的卵母细胞激活率(91.3%vs 57.9%)、卵裂率(85.7%vs 57.9%)及桑囊率(9.5%vs 0%)均显著高于注射hCG 60 h组(P<0.01).56.8%(117/206)的ICSI废弃的未成熟卵母细胞可以在体外发育成熟,激活后具有一定的发育潜能,卵龄对卵母细胞的质量和发育能力影响较大.     

应用氯化锶和放线菌酮对小鼠卵母细胞进行孤雌活化的研究

本试验研究了SrCl_2浓度和作用时间,以及卵龄和蛋白合成抑制剂放线菌酮等对昆明种小鼠卵母细胞活化的影响。研究表明,以含1.6mmol/L SrCl_2的无钙M16液对小鼠卵母细胞活化效果最好(87.0％),显著(P<0.05)优于SrCl_2浓度为1.0、5.0、10.0mmol/L的同种液体。SrCl_2作用时间10分钟显著(P<0.05)好于5、20、30或60分钟。注射hCG后18和20小时卵母细胞的活化率(分别为87.0％和84.6％)显著(P<0.01)高于14或16小时的活化率(分别为4.8％和16.5％)。CHX与SrCl_2联合使用产生显著的协同促进卵母细胞活化作用。     

不同因素对大鼠卵母细胞孤雌激活作用影响的研究

本实验比较了SrCl_2,放线菌酮(CHX),电刺激和乙醇等理化因素对SD大鼠卵母细胞激活的作用。结果表明,SrCl_2,CHX和电刺激均能有效激活SD大鼠卵母细胞,其最高激活率分别达到93.24％,91.89％和85.90％。8％乙醇对注射hCG 21小时后的卵母细胞激活率也达70％。SrCl_2在1.6和3.2mmol/L浓度,作用10—30分钟均有较好激活效果。电刺激强度在160V,80μs作用较佳。当SrCl_2与CHX联合作用时,激活率可有明显提高。但电刺激或乙醇与CHX的联合作用不能有效提高激活 率。本研究还比较了卵丘细胞的存在与否对激活的影响,发现卵丘-卵母细胞复合体中的卵母细胞不能被有效激活。刚离体的超排卵母细胞也不能被有效激活,须在体外培养一定时间后才能被激活。     

化学激活和季节对克隆猪出生率的影响

为了解化学激活对克隆猪出生效率的影响, 研究了体外成熟的猪卵母细胞被激活恢复减数分裂到克隆猪出生的整个过程. 首先研究了电激活(Ele), Ele+CHX+CB和Ele+6-DMAP 3种激活方法对猪卵母细胞孤雌激活(parthenogenetic, PA)和核移植(nuclear transfer, NT)重构胚体外发育的影响. 比较了Ele或Ele+CHX+CB激活方法对克隆猪出生效率的影响. 实验中单独列出了PA胚的扩张囊胚率或NT优质囊胚率来代表囊胚的质量. 结果表明: 化学联合激活提高了PA的囊胚率和扩张囊胚率, 但对PA胚的卵裂率和囊胚细胞数没有显著影响(P>0.05). Ele+6-DMAP对PA胚的囊胚率和扩张囊胚率有显著提高(P<0.05), 但对NT胚的囊胚率和优质囊胚率没有提高甚至降低了NT胚的发育. Ele+CHX+CB虽然提高了NT胚的囊胚率(P<0.05), 但对优质囊胚率没有影响. Ele+CHX+CB激活方法使克隆猪出生率有所提高但不显著. 本文还研究了季节对猪孤雌发育和克隆猪出生率的影响. 结果表明, 春季收集的猪卵母细胞使用3种激活方法卵母细胞的孤雌囊胚率均高于冬季收集的猪卵母细胞的囊胚率. 春季和冬季进行移植, 克隆猪出生率没有区别. 综上, 在PA中获得的结果与NT胚中获得的结果不一定完全匹配, 说明孤雌激活和重构胚的激活机制还是有区别的. 化学联合激活虽然能提高囊胚率, 但它的作用相当于降低囊胚形成的门槛, 却不是从本质上改变囊胚发育能力, 因此不能显著提高克隆猪出生效率. 春季收集的卵母细胞在体外培养中的发育能力好于冬季收集的卵母细胞, 但季节对克隆猪出生率没有显著影响.     

6—DMAP对小鼠卵母细胞减数分裂启动及孤雌发育作用

小鼠卵泡卵母细胞体外培养过程中加入２ｍｍｏｌ／Ｌ６－ＤＭＡＰ可抑制卵母细胞自发的染色持浓缩和生发泡破裂（ＧＶＢＤ）。源自超排的ＭⅡ期卵母细胞则能为６－ＤＭＡＰ所激活。ｈＣＧ注射后１８－１９ｈ的卵母细胞置于２ｍｍｏｌ／Ｌ６－ＤＭＡＰ的ＣＺＢ溶液中培养０．５ｈ、１ｈ、２ｈ、３ｈ,卵母细胞的激活率分别为２６．１％、７５．２％、７５．８％、７７．３％、卵裂率分别为８８．２％、７３．２％、６７．０％、５８．     

6-DMAP和胚胎干细胞代数对异种重构卵体外发育的影响(简报)

核移植技术已经广泛应用于动物克隆,但是克隆动物的成活率仍然很低。许多克隆胚胎死于妊娠期,少部分能发育到期,正常出生,但多数在出生后由于心肺和消化道的问题,很快就夭折,有些克隆动物有异常表型,如出生时体重和胎盘过大等。研究发现,在同种克隆动物实验中用胚胎干细胞(Embryonic stem cell,ES细胞)作为核供体,发育到期的克隆动物比例明显高于体细胞,并且用杂交一代的小鼠ES细胞为核供体,绝大多数克隆仔     

Improved parthenogenetic development of vitrified-warmed bovine oocytes activated with 9% ethanol plus 6-DMAP

The objective was to compare various activation protocols on developmental potential of vitrified bovine oocytes. Bovine oocytes matured in vitro for 23 h were vitrified with EDFSF30 in open pulled straws. After warming, they were cultured in vitro for 1 h, followed by parthenogenetic activation. Vitrified-warmed oocytes had a morphologically normal rate similar to that of controls (nonvitrified oocytes cultured in vitro for 24 h; 98.6% vs. 100%, P > 0.05). When vitrified-warmed oocytes were first activated with 7% ethanol for 5 min and then incubated in 6-dimethylaminopurin (6-DMAP) for 4 h, cleavage and blastocyst rates were 41.2% and 23.2%, respectively, which were lower than those of controls (77.5% and 42.0%, P < 0.05). Subsequently, we varied the ethanol concentration to increase the effectiveness of parthenogenetic activation. When either 5%, 6%, 7%, 8%, 9%, 10%, or 11% ethanol alone (for 5 min) or in combination with 6-DMAP (4 h) was used to activate vitrified-warmed oocytes, cleavage rates ranged from 22.3% to 61.1% and blastocyst rates ranged from 1.1% to 30.6%. These rates were optimized when oocytes were treated with 9% ethanol plus 6-DMAP; this was verified in experiments evaluating other activation protocols with 9% ethanol, calcium ionophore A23187, or ionomycin alone, or in combination with DMAP or cycloheximide (CHX). In conclusion, the oocyte activation protocol affected developmental capacity of vitrified bovine oocytes; 9% ethanol (5 min) followed by 6-DMAP (4 h) promoted optimal parthenogenetic activation.     

不同活化方法对小鼠卵母细胞孤雌发育的影响（简报）

In order to study effects of electro-fusion and strontium chloride (SrCl2) activation in nuclear transfer experiment on activation and development of mouse oocytes, concentration and treatment duration of SrCl2, electro-pulse and electro-pulse combining SrCl2 were used to activate mouse oocytes which were obtained after hCG 17h. Activated oocytes were cultured in vitro in CZB medium. The results were as follows: 82.4% activation percentage was obtained when the oocytes were treated with 10mmol/L SrCl2 for 6h, it was significantly (P>0.05) higher than those obtained from that treated with the 5mmol/L or 10mmol/L SrCl2 for 4h. The activation percentage was not significantly different between 5mmol/L and 10mmol/L SrCl2 for 6h, but the percentage of morula and blastocyst in 10mmol/L SrCl2 6h group was significantly (P > 0.05) higher than those in 5mmol/L SrCl2 6h group. In the groups of treatment with electro-pulse, the best activation percentage (70.9%) was obtained when the oocytes were treated with 1.0kv/cm, 320micros, 3 pulses, but M + B percentage (7.9%) was low. In the groups of treatment with electro-pulse combining with SrCl2, the best result was acquired (activation and M + B percentage were 75.0% and 57.3% separately) when the oocytes were treated in 10mmol/L SrCl2 for 6h interval 1h after treated with 1.8kv/cm, 10s, 1pulse. These results show that the treatment with electro-pulse combining SrCl2 is a better way to mouse parthenogenesis.     

Effects of post-treatment with 6-dimethylaminopurine (6-DMAP) on ethanol activation of mouse oocytes at different ages

To study the effect of post-treatment with 6-Dimethylaminopurine (6-DMAP) on oocyte activation and development, mouse oocytes collected at different times post human chorion gonadotropin (hCG) injection were incubated in 6-DMAP-containing Chatot-Ziomek-Bavister (CZB) medium for different periods after ethanol exposure, and activation and development were observed. When oocytes were cultured in 6-DMAP without prior ethanol exposure, the highest activation rate was only 40%. Incubation in 6-DMAP for 6 h following ethanol exposure significantly (P < 0.05) increased the activation rate in oocytes recovered 15 and 18 h post hCG, but this effect was not significant in the 21 h oocytes. When oocytes were incubated in 6-DMAP for 1 h at different time points after ethanol, a 6-DMAP susceptible temporal window was found to be located from the second to the fifth h in the 18 h oocytes and from the fourth to the fifth h in the 15 h oocytes, and within the window, the duration of 6-DMAP incubation can be reduced to 0.5 h with more than 80% activation. With the 13 h oocytes, however, 6-DMAP-incubation can only be shortened to 3 h and no specific temporal window was identified. Oocytes that were incubated in 6-DMAP for 1 or 2 h after ethanol exposure developed to morula/blastocyst stages at significantly (P < 0.05) higher rates than those incubated in 6-DMAP for 6 h. Our results suggested that (i) long duration of 6-DMAP incubation impaired the development of mouse parthenogenotes; (ii) the effect of 6-DMAP alone was limited without prior ethanol exposure; (iii) the egg age affected both the timing of 6-DMAP susceptibility and the duration of exposure required to obtain a maximal activating effect; (iv) the most effective activating protocols varied for oocytes of different ages.     

Parthenogenetic development of porcine oocytes treated by ethanol, cycloheximide, cytochalasin B and 6-dimethylaminopurine

This study was carried out to investigate the various concentrations and exposure times of ethanol, one of many intracellular calcium elevating agents, and a sequential combination of ethanol (8%), cycloheximide (CHX, 10 microg/ml), cytochalasin B (CCB, 7.5 microg/ml) and 6-dimethylaminopurine (6-DMAP, 2 mM) to improve parthenogenetic activation and development of in vitro matured porcine oocytes. Cumulus-oocyte complexes (COCs) were matured in tissue culture medium (TCM) 199 for 44 h at 38.5 degrees C, 5% CO2 in air. Cumulus-free oocytes showing first polar body were activated by concentrations of 0, 5, 6, 7, 8, 9 and 10% ethanol for 10 min and exposure times of 0, 5, 8, 10, 12 and 15 min with 8% ethanol in HEPES buffered (25 mM) NCSU-23 medium. Also, oocytes were activated with the NCSU-23 medium containing 8% ethanol for 10 min. After that, oocytes were incubated in the NCSU-23 medium supplemented with CHX, CCB, 6-DMAP, CHX + CCB, CHX + 6-DMAP, CCB + 6-DMAP and CHX + CCB + 6-DMAP for 3h, respectively. Following activation, oocytes were transferred into the NCSU-23 medium containing 0.4% BSA for further culture of 20 and 144 h at 38.5 degrees C, 5% CO2 in air. The activation rates of oocytes were higher in 6, 7 and 8% ethanol concentrations compared with 0, 5, 9 and 10% ethanol concentrations. Significantly, more oocytes (29.3-33.7%) were activated in the exposure for 8, 10, 12 and 15 min than those in the exposure for 0 and 5 min, but there was no difference due to exposure to 8% ethanol for 8-15 min. Oocytes treated by chemical agents (40.5-70.5%) after exposure to ethanol significantly improved the rate of oocyte activation compared with ethanol alone (31.2%). The percentage of cleaved oocytes was higher in the ethanol+CHX+CCB+6-DMAP treatment (66.4%) than in other treatments (24.9-57.6%). Also, the rate of blastocyst formation was higher in the ethanol+CHX+CCB+6-DMAP treatment (25.0%) than in other treatments (0.0-19.3%). In conclusion, the optimal activation treatment of ethanol exposure alone for the in vitro matured porcine oocytes was 8% ethanol for 8-15 min. Oocytes activated by 8% ethanol for 10 min and incubated in the NCSU-23 medium supplemented with CHX, CCB and 6-DMAP for 3 h were more efficient for parthenogenetic development of in vitro matured porcine oocytes.     

Effects of different activation protocols on preimplantation development, apoptosis and ploidy of bovine parthenogenetic embryos

The objective of this study was to optimize the protocols for bovine oocytes activation through comparing the effectiveness of different treatments on the activation and subsequent development of oocytes and examining the effects of two combined activation treatments on the blastocyst apoptosis and ploidy. Cumulus-oocyte complexes (COCs) were recovered from abattoir-derived ovaries and matured in vitro. After maturation, cumulus-free oocytes were activated according to the experiment designs. Activated oocytes were cultured in vitro in modified synthetic oviductal fluid (mSOF) medium and assessed for pronuclear formation (15-16 h), cleavage (46-48 h) and development to the blastocyst stage. In Experiment 1, the matured oocytes were treated with single activation agents, including ionomycin (5 microM for 5 min), ethanol (7% for 7 min), calcium ionophore A23187 (5 microM for 5 min) or strontium (10mM for 5h). The pronuclear formation and cleavage rate were higher significantly in ionomycin (39.0 and 30.7%) and ethanol (41.5 and 28.1%) treatment alone compared to other treatments (9.7-25.2 and 11.3-23.7%, respectively, P<0.05). Very low blastocyst rates (3.9-5.3%) resulted which were not significantly different among treatments (P>0.05). For the combined activation treatment (Experiment 2), the same concentrations of ionomycin and ethanol as in Experiment 1 were used in combination with either 6-dimethylaminopurine (6-DMAP, 2.0 mM for 3 h) or cycloheximide (CHX)+cytochalasin B (CB, 10 microg/ml for 3 h). The pronuclear formation, cleavage rate, blastocyst rate and cell number of blastocyst were higher significantly (P<0.05) in ionomycin+6-DMAP treatment (67.1, 69.2, 28.0 and 91.3%, respectively) and ethanol+CHX+CB treatment (68.9, 70.2, 25.5 and 89.3%, respectively) compared to other treatments (11.7-58.1, 10.2-47.1, 1.5-24.2 and 34.2-62.7%, respectively). In Experiment 3, the parthenogenetic blastocysts produced by activation with ionomycin+6-DAMP and ethanol+CHX+CB and in vitro fertilized blastocysts (control group) were examined for apoptosis using a terminal deoxynucleotidyl transferase mediated deoxyuridine 5-triphosphate nick-end labeling (TUNEL) assay. The ethanol+CHX+CB treatment (7.0%) showed significantly lower blastocyst apoptosis index compared to ionomycin+6-DAMP treatment (9.1%, P<0.05). Furthermore, the chromosomal composition in the parthenotes embryos differed (P<0.05) among treatments. The percentage of haploid parthenotes was higher in ionomycin+6-DMAP treatment than ethanol+CHX+CB treatment. These results suggested that ethanol+CHX+CB treatment was more favorable protocol for parthenogenesis of bovine oocytes.     

Effect of different parthenogenetic activation methods on the developmental competence of in vitro matured porcine oocytes

The aim of this study was to investigate the effect of electrical pulse, ethanol, and ionomycin combined with cycloheximide (CHX), cytochalasin B (CB), and 6-dimethylaminopurine (6-DMAP) on parthenogenetic developmental competence of in vitro matured porcine oocytes. In experiment 1, oocytes were treated with direct current electrical pulse (DC pulse) and then incubated in the NCSU-23 medium supplemented with CHX, 6-DMAP, CB + CHX, and CB + 6-DMAP for 6 h, respectively. The rate of blastocyst development in DC pulse + CB + 6-DMAP group was significantly higher than those in other groups (42.4% vs 23.9% approximately 35.8%; P < 0.05); however, there were no differences in both of the cleavage rate and the cell number of blastocysts among four groups. In experiment 2, oocytes were treated with NCSU-23 medium containing 20 muM ionomycin for 40 min and then incubated in the NCSU-23 medium supplemented with CHX, 6-DMAP, CB + CHX and CB + 6-DMAP for 6 h, respectively. The rates of cleavage and blastocyst development in ionomycin + 6-DMAP group were higher than those obtained in other groups (66.2% vs 46.3% approximately 57.3%; 22.3% vs 7.4% approximately 16.1%; P < 0.05). In experiment 3, the activation effects of ethanol combined with 6-DMAP, CHX, CB + 6-DMAP and CB + CHX were investigated. The rates of cleavage and blastocyst development in ethanol + CB + 6-DMAP group were significantly higher than those in other groups (55.5% vs 42% approximately 46.2%; 18.0% vs 7.1% approximately 11.9%; P < 0.05). In experiment 4, the optimal activation protocols in each group plus DC pulse + ionomycin + 6-DMAP were compared. The results showed the rates of cleavage in DC pulse + CB + 6-DMAP group and ionomycin + 6-DMAP were higher than those in ethanol + CB + 6-DMAP and DC pulse + ionomycin + 6-DMAP (73.8-74.4% vs 56.5-57.5%; P < 0.05), but the blastocyst development only in DC pulse + CB + 6-DMAP group was significantly higher than that in other groups (34.1% vs 13.4% approximately 22.3%; P < 0.05). Total cell number of blastocysts in the group of DC pulse + ionomycin + 6-DMAP was higher than that in other groups (34.1 vs 25.3-27.2; P < 0.05). In conclusion, DC pulse, ethanol, CB, and 6-DMAP all affected the parthenogenesis of porcine oocytes matured in vitro, but their combination of DC pulse + CB + 6-DMAP showed the best result in both of cleavage and blastocyst development.     

绵羊体外成熟卵母细胞的电激活及其在体外孤雌发育的研究

首先对绵羊卵母细胞收集及其体外成熟（ＩＶＭ）条件进行了摸索,然后对影响电刺激激活ＩＶＭ卵母细胞的因素进行了研究,观察激活后卵母细胞在体外的发育能力。结果表明,剥离法比注射器吸卵法所获得的卵母细胞成熟率高,激活更加正常。剥离法收集的卵母细胞体外成熟培养２７小时后,以含０．１ｍｍｏｌ／Ｌ ＣａＣｌ２、０．１ｍｍｏｌ／Ｌ ＭｇＳＯ４和１０ｍｍｏｌ／Ｌ组氨酸的０．２８ｍｏｌ／Ｌ肌醇（ｉｎｏｓｉｔｏｌ）作基     

6—DMAP和胚胎干细胞代数对异种重构卵体外发育的影响（简报）

The development of reconstructed oocytes and the survival rate of cloned animal were affected by many factors during nuclear transfer. The genetic constitution and the genetic state of donor nucleus were proposed to be primary factors, which affected the survival rate of cloned animal. In addition, the survival rate of cloned animal might be influenced by nuclear transfer technique itself and passages of donor cells as well as the activation methods of oocytes. We reconstructed oocytes with outbreeding Kunming albino mouse ES cells and enucleated rabbit oocytes, and analyzed the effects of the passages of ES cells and 6-DMAP on the development of interspecific reconstructed oocytes. The interspecific reconstructed ES-rabbit oocytes were activated either by combined two set electric pulses and 6-DMAP or by two set electric pulses alone. The rate of cleavage was significantly higher for the group (86.2%) treated with 6-DMAP than the group (64.2%, P < 0.05) treated with electric pulses only, and the rate of blastocysts was 17.0% and 13.4% respectively, which were not significantly different between two groups. When ES cells that had been passed for 24 and 14 generations were used as donors, the cleavage rates of the reconstructed oocytes were 88.5% and 82.1%, respectively (P > 0.05), and the rates of blastolation were 16.7% and 15.4%, respectively (P > 0.05). The results show that 6-DMAP increases the cleavage rate of reconstructed oocytes derived from ES cells, and affects slightly the developmental rate of blastocysts. There are no differences when high passage and low passage ES cells are used as nuclear donors.