卵母细胞去核及卵丘细胞移核方法对猪体细胞核移植的影响

以猪体外成熟卵母细胞周围分离得到的卵丘细胞作为猪体细胞核移植的供核细胞,研究了卵母细胞不同去核方法(盲吸法、活性荧光染色去核法、盲吸法和活性荧光染色法联合去核法)的去核率差异,并比较了卵丘细胞透明带下注核和胞质内注核两种重建胚构建方法的胚胎裂解率、4 8细胞发育率和桑椹胚率的差异。结果表明:(1)以荧光染料染色法的去核率(87.18%)最高,与其他试验组相比差异显著(P<0.05);盲吸法去核所用时间最少(1.2 min/个),与其他试验组相比差异显著(P<0.05)。(2)透明带下注核比卵母细胞质内直接注核的卵裂率(40.11%/29.75%)和4 8细胞率(11.86%/6.81%)高,差异显著(P<0.05);桑椹胚率(1.75%/1.79%)无明显差异(P>0.05)。     

不同去核方法对猪手工克隆重构胚发育效果的影响

为探讨不同去核方法对猪手工克隆(HMC)重构胚发育效果的影响,本研究比较了盲切法,第一极体(Pb1)定位法及脱羰秋水仙碱(DM)辅助去核法3种不同的去核方法的去核效率及HMC胚胎发育的影响。结果表明:第一极体定位法和DM辅助去核法的整体去核效率显著高于盲切法去核法(P0.05);应用0.4μg/m L DM处理卵母细胞60 min的突起率、整体去核效率显著高于其他浓度和时间处理组(P0.05);DM辅助去核与pb1定位去核法2种不同去核方法对HMC重构胚的发育效果的影响差异不显著。本研究表明,添加适量的DM可以提高徒手克隆去核效率,且对后期重构胚发育没有显著影响。     

影响核移植后小鼠重构胚存活因素的研究

将不同类型的供体细胞(卵丘细胞、心肌细胞和上皮细胞)的遗传物质注射到去核的MⅡ卵母细胞中,获得各种重构胚胎,以分析对小鼠卵母细胞进行核移植操作获得重构胚过程中的各种影响因素。结果表明,用Gi emas染料将挤出的卵母细胞质染色证实,可以完整地去除MⅡ卵母细胞核。对370个MⅡ卵母细胞进行去核,去核成功率为92.4%,注核成功率为82.1%;给予90 v/mm,80μsec,1次电脉冲刺激,融合率为72.1%;将融合激活后的重组胚转入KSOM培养基中,平均囊胚率达到35.8%。在胚胎重构过程中,出现了核仁显著变大,出现不同数量核仁的现象。通过比较各种重构胚胎体外后续发育,结果卵丘细胞重构胚胎的体外发育率最好。     

卵丘细胞对猪卵母细胞体外成熟及孤雌胚胎体外发育的影响

为探讨表皮生长因子(epidermal growth factor,EGF)的添加浓度及脱卵丘细胞时间对猪卵母细胞体外成熟及孤雌胚胎体外发育的影响.试验通过在体外成熟液中添加不同浓度(0、10、15、20、30、40 ng/mL)的EGF来研究其对培养44 h的卵母细胞成熟率以及孤雌胚胎发育的影响;在培养开始后的不同时间(18、24、38、44 h)进行脱卵丘细胞处理来研究不同时间脱卵丘处理对培养44 h的卵母细胞成熟率以及孤雌胚胎发育的影响.结果表明,成熟培养基中添加10 ng/mL EGF能显著提高卵母细胞的卵裂率和囊胚率(P <0.05).共培组和独培组卵母细胞培养18 h后脱卵丘细胞成熟率均低于44 h,但差异不显著(P >0.05);共培组卵母细胞培养18 h后脱卵丘细胞的卵裂率和囊胚率显著高于培养44 h(P <0.05);独培组卵母细胞培养18 h后脱卵丘细胞的卵裂率与44 h无显著差异(P >0.05),但囊胚率显著高于培养44 h后脱卵丘细胞(P <0.05).添加10 ng/mL EGF对猪卵母细胞体外成熟及孤雌胚胎体外发育较好;卵母细胞培养18 h后脱卵丘细胞可提高孤雌胚胎早期发育能力.     

猪卵丘细胞核移植研究

以卵丘细胞为供核体细胞,采用胞质内注射法进行猪体细胞核移植,对去核、激活和培养等关键技术过程进行研究,结果表明,①点压法、挤压法对卵母细胞去核率明显高于盲吸法(三者分别为62.5%,64.6%,50.7%,P<0.05)。盲吸法去核染色体容易发生位置偏离,影响去核效果,但对早成熟的卵母细胞(36h～44h)进行去核可明显提高去核效率(P<0.05),在成熟培养36h～38h、39h～41h、42h～44h去核率分别为60.9%、67.8%、64.3%,而45h～48h为48.4%。②体细胞预激活有助于提高核移胚卵裂率(28.0%,20.1%,P<0.05)。A23187(Ca2 ionophore,钙离子载体)单独或与6DMAP(6Dimethylaminopurine,6二甲基氨基嘌呤)联合作用能使猪体细胞核移胚激活继续发育。③核移胚以胚胎培养液NCSU23(NorthCarolinaStateUniversity23medium,北卡洲立大学培养液23)及卵丘颗粒单层共培养体系进行分别培养,核移胚卵裂率无明显差异(30.06%,31.5%,P>0.05)。但NCSU23培养4细胞后发育能力更高(13.5%,3.9%,P<0.05)。     

猪卵母细胞化学辅助手工去核及手工核移植胚胎发育能力因素的研究

本研究在筛选猪化学辅助手工去核最佳脱羰秋水酰碱(Demecolcine,DC)浓度的基础上,探讨了各种因素对手工重构胚发育的影响,以期建立高效的猪手工体细胞核移植技术体系.观察不同成熟时间卵母细胞在不同DC浓度下的去核效率,并进一步比较了化学辅助手工去核法和荧光染色去核法、不同类型的供体细胞(颗粒细胞、新生巴马肌肉成纤维细胞和胎儿成纤维细胞)和供体细胞的不同处理方法(70％～80％汇合、血清饥饿法和100％接触抑制法)对重构胚发育能力的影响.结果表明:(1)利用DC诱导去核,对体外成熟培养44 h的卵母细胞以浓度0.4 μg· mL-1作用0.5～1 h为宜.(2)用DC化学辅助手工去核与用荧光染色去核的重构胚囊胚发育率差异不显著(13.11％ vs 9.25％,P＞0.05).(3)以胎儿成纤维细胞、颗粒细胞和新生巴马小型猪肌肉成纤维细胞为供体构建的重构胚的融合率、卵裂率及囊胚率均差异不显著(P＞0.05).(4)用70％～80％汇合(对照组)组、接触抑制组和血清饥饿组的细胞作供体构建的重构胚,在融合率上,接触抑制组显著高于对照组(P＜0.05);在分裂率与囊胚率上,各组之间均无显著差异(P＞0.05).研究结果表明,化学辅助手工去核法在实际生产中可以替代荧光染色去核法,能省去去核过程中荧光染色及紫外光照射去核等步骤,从而简化了猪手工体细胞核移植程序,提高了猪手工体细胞核移植效率,能为高效的猪手工体细胞核移植技术体系的建立提供参考.     

家兔胚胎细胞核移植与连续移植

将发育不同时期的兔胚和移核胚的卵裂球细胞核与去核的成熟卵母细胞共同组成移核胚,通过中间受体培养和移植实验检验胚胎的发育能力。结果表明,（１）兔囊胚之前各个时期的胚胎细胞核均可使移核胚发育到囊胚;（２）胚胎极化前后的卵裂球参与组成的移核胚发育到囊胚的比例无显著差异。但极化后 ６４细胞胚的卵裂球与去核卵母细胞的融合率低于极化前的 ８细胞胚胎卵裂球;（３）兔 １６细胞胚与去核的卵母细胞组成的移核胚可以发育到期,产仔率为 ３．１６％ ;（４）兔移核胚卵裂球用于连续核移植,其后 ２ 代均可发育成囊胚,其中第 １ 代移核胚与第 ２ 代移核胚发育率相似,但显著高于第 ３ 代移核胚;（５）兔移核胚和各代连续移核胚卵裂球与去核卵的融合率无显著差异。     

小鼠卵母细胞化学去核及手工构建核移植胚胎

为优化脱羰秋水仙碱（DC）诱导去核程序,研究以DC去核卵母细胞为核受体的、无透明带体细胞核移植方法在小鼠体细胞核移植中的应用,试验比较了乙醇、SrCl2两种激活方法及脱羰秋水仙碱处理开始时间对小鼠MⅡ期卵母细胞去核效率的影响;将DC诱导去核成功的卵母细胞去除透明带,与胎儿成纤维细胞粘合、电融合和SrCl2激活后,体外培养重构胚。结果显示,7%乙醇激活后0 min起始DC处理可得到最高的诱导去核率（66.4%）;而在8 mmol/L SrCl2中激活15 min后用DC处理可得到最高的诱导去核率（64.3%）;目前重构胚可以体外发育到8-细胞。试验结果首次证明了SrCl2在小鼠卵母细胞DC诱导去核中的作用效果与乙醇相当,初步证明了将DC诱导去核技术与无透明带技术相结合手工克隆生产小鼠重构胚的可能性,它的成功将大大简化核移植程序。     

电激活对完全体外化牛细胞核移植的影响

牛卵母细胞在体外成熟２３～２４ｈ时去核，去核卵用８０Ｖ／ｍｍ４０μｓ两次电脉冲激活（Ⅰ组）或不激活（Ⅱ组），然后将体外受精、发育的８～３２细胞期胚胎的单个卵裂球注入卵周隙，用８０Ｖ／ｍｍ４０μｓ两次电脉冲诱导卵裂球与去核卵母细胞融合。Ⅰ组操作后存活率和融合率（８８．４％和５５．０％）显著低于Ⅱ组（９５．９％和６５．１％，Ｐ＜０．０５）。融合卵体外培养２４ｈ和５～８ｄ后，Ⅰ组核移植胚胎的卵裂率和桑椹／囊胚发育率（６３．０％和１５．２％）与Ⅱ组（５０．５％和７．８％）无显著差异，但Ⅰ组结果均好于Ⅱ组。将来自两组的２５枚桑椹和囊胚移植到１６头同期受体，在已检查过的８头受体中２头受体妊娠，其中１头于妊娠后４个多月流产，１头于妊娠期满后产出一雄性牛犊。研究结果表明：去核卵母细胞的电激活尽管对重组卵的存活与融合不利，但可改善核移植胚的卵裂和发育。本研究在我国首次获得牛细胞核移植的成功，证明用ＩＶＭ卵母细胞和ＩＶＦ胚胎进行完全体外化的牛细胞核移植是可行的。     

克隆山羊"白雪"满月科研人员验明身份

<正>在山东农大动物胚胎工程中心实验羊场,即将满月的"白雪"蹦蹦跳跳,活泼可爱。它时而拱到"母亲"的身下吃奶,时而钻过窄窄的栅栏撒欢,时而看着人昂头鸣叫。该校动物胚胎工程实验中心主任谭景和教授介绍,体细胞核移植克隆山羊的研究,得到了国家重点基础研究发展(973)计划和山东省"三O"工程项目资助。在研究过程中,他们将体外成熟卵丘细胞,经显微操作,植入山羊体外成熟卵母细胞卵周隙,并经电刺激使供核细胞与去核卵母细胞融合而组成克隆胚胎,再用特殊方法处理激活克隆胚胎,然后将培养发育好的49枚克隆胚胎,经手术移植到自然同步发情的5只受体母羊输卵管内。     

The Construction of Cloned Sika Deer Embryos (Cervus nippon hortulorum) by Demecolcine Auxiliary Enucleation

The objective of our study was to establish the feasibility of experimental protocols for cloning sika deer. We performed auxiliary enucleation to improve the efficiency of nuclear transfer operation by optimizing the demecolcine concentration to induce cytoplasmic protrusions in the sika deer oocytes. In the present study,we had studied the impact of different demecolcine concentrations on cytoplasmic protrusions and enucleation rates. We determined that 95.9% of the sika deer oocytes formed cytoplasmic protrusions when treated for 1 h with 0.8 μg/ml demecolcine. The lowest observed rate of protrusion was 19.3% after overnight treatment with demecolcine. When the oocytes aged or had a poor cumulus expansion, they exhibited a significant decrease in the ability to form cytoplasmic protrusions. The rates of enucleation (94.9% vs 85.8%, p < 0.05), cell fusion (84.6% vs 70.1%, p < 0.05) and blastocyst formation (15.4% vs 10.9%, p < 0.05) using demecolcine auxiliary enucleation were significantly higher than those after blind enucleation. These results demonstrated that sika deer oocytes could be enucleated quickly and effectively using demecolcine auxiliary enucleation, which could enhance the enucleation rate, cell fusion rate and blastocyst rate of cloned embryos in vitro.     

生长激素和胰岛素对猪卵母细胞体外成熟及孤雌胚卵裂的影响

本研究探讨了生长激素(STH)和胰岛素对猪卵母细胞体外成熟及孤雌激活后卵裂的影响。结果表明:在mNCSU-23液中,添加0.15μg/mLSTH组的成熟率(73.83%)和卵裂率(64.76%)显著高于对照组和添加0.01、0.05、0.1、0.2μg/mLSTH组(P<0.05);添加5μg/mL和8μg/mL胰岛素组的成熟率(66.25%、60.64%)显著高于添加0、0.5、2μg/mL及10μg/mL组(P<0.05);添加5μg/mL胰岛素组的卵裂率(61.63%)显著高于添加0、0.5、2、8、10μg/mL组(P<0.05);最佳的联合添加组为0.15μg/mLSTH+2μg/mL胰岛素,其体外成熟率为79.37%、卵裂率为72.31%。     

微量元素锌对牛卵母细胞体外成熟及其体外受精胚胎发育的影响

本研究旨在探讨锌对牛卵母细胞体外成熟及体外受精胚胎发育的影响。首先使用锌螯合剂TPEN去除锌,并检测缺锌对牛卵母细胞体外成熟的影响;然后在体外成熟液中分别添加0(对照组)、0.4、0.8、1.2、1.6μg/mL硫酸锌,探索不同浓度硫酸锌对体外成熟及后续胚胎发育的影响。结果表明:锌元素在体外成熟液中的含量低于牛卵泡液和颈静脉血清(P<0.05);去除体外成熟液中的锌后牛卵母细胞的体外成熟效率下降(P<0.05),且具有时间依赖性,补充适宜浓度硫酸锌后成熟效率恢复;向体外成熟液中添加硫酸锌并未对卵母细胞体外成熟效率产生显著影响,但添加0.8μg/mL硫酸锌成熟后的卵母细胞中活性氧含量显著降低,后续体外受精胚胎的囊胚发育效率显著提高;RT-qPCR分析结果显示,与对照组相比,添加0.8μg/mL硫酸锌成熟后的卵母细胞中抗氧化基因SOD1、CAT、TXN1、PRD1和卵丘扩展基因PTX3、TSG6的表达水平均提高(P<0.05)。研究表明,添加0.8μg/mL硫酸锌可以通过提高卵母细胞内抗氧化酶基因的表达水平,降低卵母细胞内活性氧含量,促进卵丘扩展,从而提高卵母细胞成熟质量和体外受精胚胎的发育效率。     

Study of the efficiency of chemically assisted enucleation method for handmade cloning in goat (Capra hircus)

The present investigation was carried out to find an efficient chemically assisted procedure for enucleation of goat oocytes related to handmade cloning (HMC) technique. After 22-h in vitro maturation, oocytes were incubated with 0.5 μg/ml demecolcine for 2 h. Cumulus cells were removed by pipetting and vortexing in 0.5 mg/ml hyaluronidase, and zona pellucida were digested with pronase. Oocytes with extrusion cones were subjected to oriented bisection. One-third of the cytoplasm with the extrusion cone was removed with a micro blade. The remaining cytoplasts were used as recipients in HMC. Goat foetal fibroblasts were used as nuclear donors. The overall efficiency measured as the number of cytoplasts obtained per total number of oocytes used was significantly (p < 0.05) higher in chemically assisted handmade enucleation (CAHE) than oriented handmade enucleation without demecolcine (OHE) (80.02 ± 1.292% vs. 72.9 ± 1.00%, respectively, mean ± SEM). The reconstructed and activated embryos were cultured in embryo development medium (EDM) for 7 days. Fusion, cleavage and blastocyst development rate were 71.63 ± 1.95%, 92.94 ± 0.91% and 23.78 ± 3.33% (mean ± SEM), respectively which did not differ significantly from those achieved with random handmade enucleation and OHE. In conclusion, chemically assisted enucleation is a highly efficient and reliable enucleation method for goat HMC which eliminates the need of expensive equipment (inverted fluorescence microscope) and potentially harmful chromatin staining and ultraviolet (UV) irradiation for cytoplast selection.     

不同浓度紫杉醇预处理对绵羊卵母细胞玻璃化冷冻保存效果的影响

细胞骨架系统的稳定对于提高卵母细胞或胚胎冷冻后的存活率及其发育能力具有重要作用。紫杉醇(Taxol)作为细胞骨架稳定剂,可增强α、β-微管蛋白二聚体的紧密联系,增大微管交联,促进微管聚合和稳定。本实验以绵羊体外成熟卵母细胞为材料,旨在探讨紫杉醇预处理对玻璃化冷冻绵羊卵母细胞存活率、形态正常率及体外受精后胚胎发育率的影响。采用0、0.5、1.0、1.5μmol/L的紫杉醇预处理绵羊卵母细胞并进行玻璃化冷冻保存,未经处理的新鲜卵母细胞为对照组。结果表明:采用浓度为0.5μmol/L紫杉醇预处理绵羊卵母细胞冷冻保存效果最佳,其解冻后的存活率(82.38%)与其他3个试验组相比有显著差异性(P0.05);体外受精卵裂率(51.17%)和桑囊胚率(20.30%)也显著高于其他3个试验组(P0.05),但低于对照组(69.42%,34.77%)(P0.05)。由此可见,以0.5μmol/L浓度的紫杉醇预处理组绵羊体外成熟卵母细胞冷冻后能获得较好的效果。     

Milrinone treatment of bovine oocytes during in vitro maturation benefits production of nuclear transfer embryos by improving enucleation rate and developmental competence

In the production of cattle nuclear transfer embryos, the production efficiency is affected by the oocyte developmental competence and successful enucleation rate. This study investigated the effect of treating oocytes with milrinone, a phosphodiesterase inhibitor, on these two characteristics. When cumulus-oocyte complexes (COCs) were cultured for 19 h with 0, 50 or 100 μM of milrinone, the enucleation rate was significantly improved by 100 μM milrinone. However, milrinone treatment during in vitro maturation (IVM) also delayed meiotic progression by at least 2 h, which would affect the examination of enucleation rate and developmental competence of oocytes. Thus, in the second experiment, meiotic resumption was temporarily inhibited with butyrolactone I (BL-I; 100 μM, 18 h) to decrease the delayed maturation caused by milrinone; this enabled a more accurate comparison of the effects of milrinone after oocyte maturation. In nuclear transfer embryo production, oocytes treated with milrinone (100 μM, 20 h) showed a significantly higher rate of enucleation compared with that of control oocytes. This improved enucleation rate was associated with a closer location of the metaphase plate to the first polar body in the treated oocytes compared with that in control oocytes. Furthermore, milrinone improved the frequency of development to the blastocyst stage in the resulting embryos. In conclusion, milrinone supplementation during IVM improved enucleation rates by rendering the metaphase plate in close proximity to the first polar body, and this treatment also improved oocyte developmental competence. These benefits additively improved the yield of cloned embryos that developed to the blastocyst stage.     

In vitro developmental potential of nuclear transfer embryos cloned with enucleation methods using pre-denuded bovine oocytes

Enucleation of a recipient oocyte is an important essential process in the procedure of somatic cell nuclear transfer (SCNT). The present study investigated a method for the improvement of enucleation efficiency. Oocytes were denuded of cumulus cells before the completion of nuclear maturation (pre-denuded) after 12 h of culture at MI stage and subsequently cultured for additional 6 h until the completion of nuclear maturation and extrusion of the first polar body (PB1). The extrusion rate of PB1 was not significantly different in the pre-denuded oocyte group, compared with control oocyte group matured for 18 h. However, the number of oocytes showing the metaphase II (MII) located just underneath the PB1 was significantly higher (p<0.05) in the pre-denuded oocyte group than those in control oocyte group. To test the effect of pre-denuding on the enucleation rate and developmental potential of embryos to blastocyst stage, subsequent somatic cell nuclear transfer comparisons were made with three different methods of enucleation at MII stage using vital dyes (demicoline and Hoescht) or the PB1 (blind enucleation) to localize the chromosome plate. Enucleation rate of the oocytes with demicoline, Hoechst and pre-denuding enucleation groups were significantly higher (p<0.05) than those of blind enucleation groups. However, cleavage rate to two-cell stage and, developmental rate to blastocyst and hatched blastocyst stage, the mean numbers of total and ICM cells in the SCNT embryos with Hoechst enucleation groups were significantly decreased (p<0.05), compared to those of blind, demicoline and pre-denuding enucleation groups. Moreover, the level of telomerase activity was also significantly (p<0.05) decreased in SCNT blastocysts of Hoechst enucleation group, compared to those of blind, demicoline and pre-denuding enucleation groups. Taken together, pre-denuding enucleation group using pre-denuded oocytes was a useful and simple enucleation method for bovine SCNT embryos.     

活性氧对猪卵母细胞SUMO-1表达及其质量的影响

本研究旨在调查活性氧过氧化氢（hydrogen peroxide,H₂O₂）对猪卵母细胞体外成熟（in vitro maturation,IVM）过程中蛋白质类泛素SUMO-1表达及精-卵结合能力的影响。试验分为0（control）、10、50、75和100 μg/mL H₂O₂处理组。利用Western blotting、流式细胞术、实时荧光定量PCR、Hoechst染色等方法检测猪卵母细胞体外成熟、蛋白质类泛素SUMO-1含量、细胞活力、凋亡基因mRNA表达、透明带（zona pellucid,ZP）溶解度和精子-卵母细胞结合的表达。结果表明,75 μg/mL H₂O₂组与对照组、10和50 μg/mL H₂O₂组比较卵母细胞体外成熟率及细胞活力显著降低;75 μg/mL H₂O₂组与其他H₂O₂组相比ZP溶解时间显著延长,并减少了精子黏附在成熟卵母细胞透明带上的数量（P<0.05）。在77和18 ku处出现SUMO-1蛋白标记,75 μg/mL H₂O₂组与对照组、10和50 μg/mL H₂O₂组比较SUMO-1蛋白含量显著降低（P<0.05）。75 μg/mL H₂O₂与对照组、10和50 μg/mL H₂O₂组比较显著下调了Bcl-2基因,而Caspase-3基因表达与对照组和10 μg/mL H₂O₂组比较显著升高（P<0.05）,50 μg/mL H₂O₂与对照组和10 μg/mL H₂O₂组相比显著上调了Bax基因水平（P<0.05）。综上所述,H₂O₂能调控猪卵母细胞体外成熟过程中类泛素化水平以及精-卵结合能力。     

黄淮白山羊孤雌胚胎的体外培养

采用离子霉素和6-DMAP对黄淮白山羊体外成熟卵母细胞进行联合激活,分别在不同的培养体系进行体外培养,观察孤雌胚胎的发育情况。培养体系分别为:无共培养条件下,M199(10?S)、CR1aa和HTF P1;颗粒细胞共培养条件下,CR1aa、HTF P1和SOFaa。结果发现,无共培养条件下,CR1aa和HTF P1组孤雌胚胎的卵裂率显著高于M199组(P<0.05),但3组均未有囊胚;共培养条件下,HTF P1组的卵裂率显著高于CR1aa和SOFaa组(P<0.05),而CR1aa组的囊胚率却显著高于其他2组(P<0.05)。综合试验结果说明,CR1aa联合颗粒细胞共培养能够获得较好的培养效果,适用于山羊孤雌胚胎的体外培养。