Efficient production of pronuclear embryos in breeding and nonbreeding season for generating transgenic sheep overexpressing TLR4

Background： Brucella is a zoonotic Gram-negative pathogen that causes abortion and infertility in ruminants and humans. TLR4 is the receptor for LPS which can recognize Brucella and initiate antigen-presenting cell activities that affect both innate and adaptive immunity. Consequently, transgenic sheep over-expressing TLR4 are an suitable model to investigate the effects of TLR4 on preventing Brucellosis. In this study, we generated transgenic sheep overexpressing TLR4 and aimed to evaluate the effects of different seasons（breeding and non-breeding season） on superovulation and the imported exogenous gene on growth.Results： In total of 43 donor ewes and 166 recipient ewes in breeding season, 37 donor ewes and 144 recipient ewes in non-breeding season were selected for super-ovulation and injected embryo transfer to generate transgenic sheep.Our results indicated the no. of embryos recovered of donors and the rate of pronuclear embryos did not show any significant difference between breeding and non-breeding seasons（P 〉 0.05）. The positive rate of exogenous TLR4 tested were 21.21 % and 22.58 % in breeding and non-breeding season by Southern blot. The expression level of TLR4 in the transgenic sheep was 1.5 times higher than in the non-transgenic group（P 〈 0.05）. The lambs overexpressing TLR4 had similar growth performance with non-transgenic lambs, and the blood physiological parameters of transgenic and non-transgenic were both in the normal range and did not show any difference.Conclusions： Here we establish an efficient platform for the production of transgenic sheep by the microinjection of pronuclear embryos during the whole year. The over-expression of TLR4 had no adverse effect on the growth of the sheep.

Relationship between Different Pronuclear Patterns and Potential of Embryo Development and Pregnancy

Objective To explore the relationship between the patterns of pronucleus and embryo development and pregnancy potential in the pronuclear stageMethods According to the number and distribution of nucleolar precursor bodies, the embryos at pronuclear stage were classified into 6 pronuclear patterns from 0 to 5, 16 - 18 h after in vitro fertilization (IV F) or intracytoplasmic sperm injection (ICSI). For each, pattern, the subsequent embryonic morphology and the pregnancy rate were analyzed.Results Embryos of Pattern 0 developed to significantly more embryos with good quality and higher pregnancy potential than the embryos developing from other patterns (83. 14% and 76. 11% respectively, P<0. 05). The pregnancy rate was decreased as less embryos of Pattern 0 were transferred . The pregnancy rate of the groups of only Pattern 0, with Pattern 0, and without Pattern 0 were 48. 08% , 32. 14% and 21. 28% respectively (P<0. 05).Conclusions The pronuclear patterns are of the predictive value of embryo development and pregnancy potential, which can be used as a new tool for the selection of embryos in IVF and ICSI.

Relationship between Pronuclear Scoring and Embryo Quality and Implantation Potential in IVF-ET

To assess the relationship between pronuclear scoring and day-3 embryo quality and pregnancy outcome and to determine the Clinical value of pronuclear stage scoring system in human in vitro fertilization-embryo transfer （IVF-ET） program, a pronuclear scoring system was used to score zygotes 16-20 h after insemination during conventional IVF or intracytoplasmic sperm injection （ICSI）. The embryos were classified into groups Z1, Z2, Z3 and Z4, Comparisons were made of the rates of arrested embryos and excellent embryos on day 3. Comparisons of pregnancy outcome were made only in those patients in whom cohorts of similarly Z-scored embryos were transferred, The results showed that there were less arrested embryos and more excellent embryos on day 3 in groups Z1 and Z2 than those in group Z3 and Z4, More embryos arrested and less excellent embryos developed in group Z4 than group Z3. The clinical pregnancy rates resulting from the transfer of single pronuclear score homologous embryo types were similar among groups Z1, Z2 and Z3. Implantation rates of group Z1 were higher （P〈0.05） than that of group Z3, These findings suggests that pronuclear scoring can predict developmental ability on day 3 and implantation potential. A evaluation that combines the Z-score and day 3 embryo morphology is useful in the determination of the most viable embryos and the number of embryos for transfer.

兔原核胚体外序贯培养

采用添加 10 % FBS的 RPMI16 4 0培养液和 m RPMI16 4 0培养液对兔原核期受精卵进行了体外序贯培养 ,并与添加 10 % FBS的 RD培养液单一培养作了比较。结果显示 :体外培养至 72 h时 ,2个培养组 8-细胞胚率、桑葚胚率和囊胚发育率无显著差异 (P>0 .0 5 ) ,但 RD单一培养组已有 10 .3%出现退化 ,与序贯培养组之间差异显著 (10 .3%比0 ,P<0 .0 5 ) ;体外培养 16 8h,序贯培养组和 RD培养组的贴附率分别为 5 9.7%和 4 1.4 % ,外延生长率分别为 4 3.1%和 2 2 .4 % ,桑葚胚率为 10 0 %和 89.7% ,脱带率为 33.3%和 5 .2 % ,二者之间贴附率、外延生长率差异显著 (P<0 .0 5 ) ,桑葚胚率、脱带率差异极显著 (P<0 .0 1) ;序贯培养 96 h的囊胚细胞数为 (12 4 .6± 6 .36 )个 /枚 ,RD培养同期囊胚细胞数为 (118.2± 5 .2 5 )个 /枚 ,差异显著 (P<0 .0 5 )。结果表明 ,序贯培养能够有效克服兔早期胚胎发育阻滞 ,促进胚胎的正常生长发育 ,提高胚胎质量 。

昆明小鼠原核胚在不同培养液中的体外发育

目的 优化昆明小鼠原核胚胎体外培养系统 ,提高胚胎发育率。方法 小鼠经超排获得原核期胚胎 ,制备小鼠输卵管上皮共培养系统 ,使用M16、CZB和KSOM培养液进行体外培养 ,并对体内和体外发育的囊胚细胞计数。结果 在KSOM和CZB中添加胎牛血清能显著提高胚胎囊胚发育率 (14 71%对 85 71% ;6 4 5 %对10 81% ) ;输卵管上皮共培养可以提高胚胎的卵裂率和囊胚发育率 ,同时提高胚胎质量和同步发育 ,小鼠胚胎在KSOMFBS中囊胚发育率达 85 19% ,显著高于CZB和M16。结论 在小鼠输卵管上皮共培养条件下 ,KSOMFBS能够很好支持昆明小鼠原核期胚胎体外发育。

自制载体冷冻小鼠原核期胚胎效果分析

目的探讨自制冷冻载体冷冻保存昆明小鼠体内原核期胚胎的可行性。方法首先,比较了两种流行的商业化载体:开放式拉长麦管(open pulled straw,OPS)和冷冻帽(cryotop)开展小鼠原核胚玻璃化冷冻保存效果。其次,以cryotop为对照,利用自制简易载体(cryotip)开展小鼠原核期胚胎的玻璃化冷冻保存。之后,利用ANOVA对各组胚胎在复苏后的体外培养卵裂率、囊胚率进行统计分析。结果 OPS和cryotop两组之间,胚胎在玻璃化冷冻/复苏后发育的2-细胞率、4-细胞率和囊胚率差异均无显著性(P>0.05),但cryotop冷冻效果更接近对照组;cryotip玻璃化冷冻载体与cryotop相比,胚胎复苏后各组差异均无显著性(P>0.05),数值上除了2-细胞发育率外,cryotip其他几项结果都稍微高于cryotop组。结论 OPS,cryotop,cryotip冷冻保存昆明小鼠体内原核期胚胎均是可行的;cryotop在冷冻效果上要优于OPS,笔者自制的cryotip因其成本低,制作简单,操作安全可靠,在实验中替代昂贵的商业化载体OPS和cryotop是可行的。

原核期胚胎的原核模式与胚胎发育及妊娠关系的研究

目的:探讨原核期胚胎的原核模式与胚胎发育及妊娠能力的关系。方法:在IVF/ICSI后16～18 h,根据原核期胚胎的核仁前体数目和分布,将其分为模式0～5;并进行随后的胚胎形态学评估和计算妊娠率。结果:模式0的优良胚胎率(83.13％)高于其它各模式之和(76.11％,P<0.05);单纯移植模式0、含模式0和不含模式0组的妊娠率分别为48.08％、32.14％和21.28％,三组间差异有显著性(P<0.05)。结论:原核期胚胎的原核模式对预测胚胎质量和种植能力有一定参考价值。

类固醇激素对牛输卵管上皮细胞分泌的调节及其分泌物对小鼠胚胎发育的影响

模拟发情期（０～６ｄ）母牛外周血浆雌激素和孕酮变化水平，在添加相应水平１７β－雌二醇和孕酮的ＴＣＭ－１９９液中，培养间情期牛输卵管上皮细胞（ＢＯＥＣ）。５％ＳＤＳ－ＰＡＧＥ分析ＢＯＥＣ分泌物，发现上皮细胞受类固醇激素作用分泌的２类蛋白质分子量与自然发情期（０～６ｄ）分泌的特异蛋白相似。证明类固醇激素可以调节和启动间情期ＢＯＥＣ的分泌活动。当雌二醇浓度高达１ｍｇ／Ｌ时，即使不加孕酮，ＢＯＥＣ仍能分泌这２类蛋白质。在培养小鼠原核胚的ＣＺＢ培养液内添加牛输卵管上皮细胞分泌蛋白（ＢＯＥＰ），与添加间情期牛输卵管冲洗蛋白（ＢＯＰ）和小牛输卵管冲洗蛋白（ＣＯＰ）相比，能显著提高通过２－细胞阶段胚胎的百分率和桑囊形成率，表明ＢＯＥＰ能较好地促进胚胎的分裂和发育。但ＢＯＥＰ组的桑囊形成率显著低于对照组，表明ＢＯＥＰ中可能缺少某些低于Ｍｒ１．０×１０４的蛋白因子的协调作用，以及含有Ｍｒ３．０×１０４～５．６×１０４的分泌蛋白的抑制作用而阻碍胚胎分裂与发育。

不同冷冻保护剂对小鼠原核期胚胎玻璃化冷冻的影响

研究不同冷冻保护剂对小鼠原核期胚胎玻璃化冷冻的影响。结果表明,15%乙二醇(EG)+15%1,2-丙二醇(PROH)+蔗糖与15%EG+15%二甲基亚砜(DMSO)+蔗糖相比,解冻后成活率分别为84.83%和95.83%,无显著差异(P>0.05);卵裂率(60%、70%)显著低于对照组(92.5%)(P<0.05),冷冻组间差异不显著(P>0.05);PROH组囊胚率(33.84%)显著低于DMSO组与对照组(56.35%、76.90%)(P<0.05);DMSO组囊胚细胞数与PROH、对照组差异显著(P<0.05)。试验证明,在乙二醇中添加PROH的冷冻效果不及添加DMSO组,玻璃化冷冻影响原核期胚胎的后期发育。

胚胎发育潜能的评估及其研究进展

在体外受精一胚胎移植（IVF—ET）技术中，人类的配子和胚胎存在大量浪费的现象，如约20％的卵子不受精、约35％的胚胎被直接作为废弃胚胎而丢弃、约60％胚胎在体外培养过程中不能发育到囊胚。即使胚胎被移植入子宫，也是大部分不能着床。人类胚胎的低利用率除了与超排卵、体外培养、胚胎评估、选择方法和内膜容受性等有关外，还与人类自身的生理状况相关。在自然状态下，生育年龄妇女每周期的妊娠率也仅为25％～35％，而流产率则高达10％～15％。

早期卵裂与常规体外受精胚胎质量的相关性研究

目的探讨早期卵裂(EC)与常规体外受精(IVF)胚胎质量的关系,评估EC能否作为胚胎体外发育潜能的一个预测指标。方法对619个IVF周期共3 646枚正常受精胚胎进行早期卵裂观察和第3天(D3)卵裂期胚胎质量评估;对其中682枚D3优质胚胎和2 180枚D3非优质胚胎进行囊胚培养,于第5天(D5)和第6天(D6)进行囊胚期胚胎质量评估。根据EC观察结果,将胚胎分成三组:EC组、原核消失(PNBD)组和原核还在(NPNBD)组。结果 D3胚胎平均卵裂球数EC组胚胎显著多于PNBD组和NPNBD组(P <0. 05),NPNBD组最低; D3优质胚胎率EC组与PNBD组差异无统计学意义(P> 0. 05),但是两组均显著高于NPNBD组; EC组D3可冻胚胎率和D3可用胚胎率均显著高于PNBD组和NPNBD组(P <0. 05),NPNBD组最低。D3优胚行囊胚培养,D5囊胚形成率和D5优质囊胚率三组之间差异无统计学意义(P> 0. 05),D5可冻囊胚率PNBD组显著高于NPNBD组(P <0. 05);总囊胚形成率、总优质囊胚率和总可冻囊胚率在三组之间差异无统计学意义(P> 0. 05)。D3非优胚行囊胚培养,EC组D5囊胚形成率、D5优质囊胚率、D5可冻囊胚率、总囊胚形成率、总优质囊胚率和总可冻囊胚率均显著高于PNBD组和NPNBD组(P <0. 05)。结论发生EC的胚胎发育速度较快,更容易发育成高质量的D3卵裂期胚胎,EC可以作为D3胚胎质量的一个预测指标。早期卵裂D3优质卵裂胚胎体外囊胚发育结局与非早期卵裂D3优质胚胎相比没有明显差异,EC可能不足以作为D3优质卵裂胚胎囊胚体外发育潜能的额外预测指标。

原核期形态特征与胚胎体外发育能力和体内着床潜能的关系

目的探讨原核期评分系统与受精后第3天胚胎形态、受精后第6天囊胚形成和着床率之间的关系,以评估其在体外受精-胚胎移植(in vitro fertilization-embryo transfer,IVF-ET)中的应用价值。方法于常规IVF或卵胞浆内单精子注射(intracytoplasmic sperm injection,ICSI)受精后16～20 h观察受精情况,将正常受精卵母细胞参照Scott提出的Z评分系统分为Z1～Z4四种类型,比较不同原核类型之间的卵裂率,胚胎第3天(D3)优质胚胎率和第6天(D6)囊胚形成率。并通过分析着床结局明确的移植胚胎,比较各种类型受精卵之间的着床率。结果 Z4组受精卵的卵裂率(92.9%)、D3优质胚胎率(14.25%)、D6囊胚形成率(10.48%)均明显低于其他各组(P<0.01)。Z4组的着床率(5.88%)很低,但各组的着床率之间差异无显著性(P>0.05)。Z1、Z2、Z3三组间的卵裂率、D3优质胚胎率、D6囊胚形成率和着床率之间差异均无统计学意义(P>0.05)。结论异常的原核形态(Z4型)可预测胚胎的体内外发育潜能,但核仁的形态特征并不一定能预测胚胎的活力,Z1、Z2和Z3胚胎可能具有相同的发育潜能。

The fertilization-induced Ca^(2+) oscillation in mouse oocytes is cytoplasmic maturation dependent

Mature eggs (at metaphase Ⅱ stage) produce a series of Ca2+ oscillation at fertilization. To define whether the fertilization-induced Ca2+ oscillation is restrict to the metaphase Ⅱ eggs and cell cycle dependent, mouse oocytes at prophase Ⅰ (arrested at germinal vesicle stage),metaphase Ⅰ, metaphase Ⅱ, as well as the pronuclear embryos at interphase of the first mitotic division derived from fertilization or parthenogenetic activation were inseminated after removal of zona pellucida. The results show that the fertilization-induced Ca2+ oscillation is not specific to metaphase Ⅱ eggs. This is supported by the fact that immature oocytes generated the Ca2+ oscillations at fertilization regardless of their nuclear progression from prophase Ⅰ to metaphase Ⅰ (in vitro matured) stage. More interestingly, it was first found that pronuclear embryos at interphase derived from parthenogenetic activation showed Ca2+ oscillations in response to fertilization while the zygotes at interphase did not after reinsemination or intracytoplasmic injection of sperm extracts which induce Ca2+ oscillations in MII eggs. This suggests that the ability of oocytes to generate Ca2+ oscillation in response to sperm penetration is not regulated in a cell cycle dependent manner but dependent on the cytoplasmic maturation.

卵母细胞质移植对兔原核胚体外发育的影响

卵母细胞胞质中存在着大量的母源性信息,正常受精卵的发育启动和早期卵裂主要由这些母源性信息所控制。为了评估卵胞质含量对早期胚胎发育的影响,以假显微注射兔原核胚为对照,采用显微注射技术将兔原核期胚胎去除或增加一定量的细胞质:试验一,增加5%和20%的细胞质;试验二,移入5%小鼠MⅡ期卵母细胞胞质。胚胎经显微操作后进行R1/R2序贯培养。结果显示,(1)增量5%组胚胎的2细胞胚(72.00%)、8细胞胚(60.00%)、桑椹胚(58.00%)和囊胚(54.00%)的发育率均显著(P<0.05)高于增量20%组胚胎(分别为47.62%、35.71%、33.33%和30.95%),但与对照组之间无显著差异(P>0.05);囊胚细胞数在2个增量组和对照组3者之间也无显著差异(P>0.05)。(2)将5%小鼠M期卵胞质移入兔原核胚后,各阶段胚胎发育率和囊胚细胞数与增量5%组、对照组相比均无显著差异;早期胚胎经PCR检测,在2细胞胚(5/5)、8细胞胚(5/5)和桑椹胚(5/5)均全部检测到了供体小鼠mtDNA的D-loop区3′端片段,而在囊胚却仅有1枚(1/5)能够检测到。结果表明,增加少量细胞质不会对兔原核胚的体外发育造成显著影响,但胚胎发育率随着细胞质体积的增加有下降趋势,而异种卵胞质对兔原核胚的发育没有明显影响,在囊胚期虽仍能检测到异种卵胞质中mtDNA的存在,但异种mtDNA会随胚胎发育而逐渐减少。

原核显微注射产生转基因绵羊胚胎

体外采集绵羊卵丘卵母细胞复合体,成熟培养24 h,经过体外受精培养17 h,比较高速离心对胚胎发育的影响;高速离心可以使黑色脂滴甩到一边从而使受精卵原核清晰可见.然后将绵羊乳腺特异表达人肝细胞再生增强因子和真核细胞表达增强绿色荧光蛋白(EnhancedGreen fluorescence protein,EGFP)的载体DNA显微注射于绵羊受精卵雄原核中,并将异构胚在SOF液中发育培养.结果表明:高速离心组囊胚率低于对照组,但是没有显著性差异(P>0.05);显微注射外源基因2天后在激光共聚焦显微镜下可见荧光胚胎;PCR检测5个荧光胚胎均可见特异性条带.在原核显微注射生产转基因胚胎中,绿色荧光蛋白可作为标记基因进行早期胚胎筛选,为提高转基因动物移植效率奠定实验基础.

已知成分培养液中兔原核卵培养到胚泡的研究

用商业化ＲＰＭＩ１６４０添加１５ｍｇｍｌ－ＢＳＡ将１５４枚兔原核卵，经体外２４ｈ、４６ｈ、７０ｈ、９４ｈ和１１８ｈ培养，分别有９８．７％（１５２／１５４）、９８．１％（１５１／１５４）、９２．９％（１４３／１５４）、８６．４％（１３３／１５４）和７５．３％（１１６／１５４）的胚胎得到进一步发育．５６．５％（８７／１５４）经１１８ｈ培养后发育成胚泡．１４０ｈ后孵化率达３５．７％（５５／１５４）．将７０枚发育的４－细胞移植到５只受体，３只妊娠（６０％）产仔５只．结果表明在ＲＰＭＩ１６４０中添加ＢＳＡ，可完成兔受精卵植入前的发育，且发育的４－细胞在植入受体输卵管后，可发育到妊娠期满并产仔．

异常授精对体外受精-胚胎移植结局的影响

目的:探讨异常受精对体外受精-胚胎移植结局的影响。方法:回顾性分析257个IVF-ET周期的临床资料,共3423个卵子,分析异常受精组与无异常受精、多原核受精、单原核受精、晚卵裂受精各组间年龄、获卵数、卵裂率、妊娠率、种植率等的关系。结果:各组比较年龄、卵裂率、可移植胚胎率、优质胚胎率、妊娠率、种植率、无显著性差异;获卵数、可移植胚胎数、优质胚胎数、异常受精各组均显著高于无异常受精组;2pn率显著低于无异常受精组。结论:获卵数是影响异常受精的因素之一,异常受精可能导致新鲜周期妊娠率偏低,但可移植胚胎数较高,最终可能获得更好的临床结局。

影响黑萨福克绵羊体内原核胚生产的因素

为提高黑萨福克绵羊原核期胚胎的生产效率,通过CIDR＋FSH＋PMSG和CIDR＋FSH＋PG两种激素方案对供体进行超数排卵,将冲出的胚胎移植入同期发情处理的受体。其中CIDR＋FSH＋PMSG注射组供体平均黄体数、可用胚数和移植妊娠率均高于CIDR＋FSH＋PG注射组（P〈0.05）。同时,在CIDR＋FSH＋PMSG注射组,不同FSH剂量注射对黑萨福克绵羊超数排卵有影响。在180-240 IU剂量组,供体羊的平均黄体数、可用胚胎数高于另一组。繁殖季节（秋季）供体平均黄体数、可用胚胎数均显著高于春季（P〈0.05）。

牛血清白蛋白对小鼠原核期胚胎玻璃化冷冻的影响

以小鼠原核期胚胎为对象,以胚胎的存活率、卵裂率、囊胚率以及囊胚细胞数作为检测指标,在M2液的基础上添加8种浓度(0,2,4,8,16,32,64,96mg/mL)牛血清白蛋白(BSA)配置防冻液,探讨防冻液和玻璃化冷冻后对胚胎发育的影响。BSA防冻液对胚胎发育影响的实验结果表明,8个浓度组间以及与对照组间胚胎的卵裂率、囊胚率以及囊胚细胞数无显著差异(P>0.05),说明在防冻液中加入一定浓度的BSA对小鼠胚胎无毒性作用。防冻液经玻璃化冷冻后对胚胎发育影响的实验表明,8个浓度组间冷冻胚胎复苏后的存活率、卵裂率、囊胚率及囊胚细胞数无显著差异(P>0.05)。表明BSA在这种防冻液中没有明显的保护作用。从经济、实用、生物安全角度考虑,不支持在玻璃化防冻液中添加BSA。

早期原核分裂对于胚胎发育潜能预测的研究

目的通过比较移植早期原核与晚期原核分裂胚胎的临床妊娠率和种植率,探讨早期原核分裂与胚胎发育潜能之间的关系。方法回顾性分析05年11月至07年1月在生殖医学中心行体外受精胚胎移植的妇女240例,通过移植不同时期的原核分裂胚胎将其分为早期原核分裂组(143例),晚期原核分裂组(47例)和混合组(50例),比较三组的妊娠率和种植率。结果早期原核分裂组的受精率和早卵裂率分别为80.39%和54.16%,而晚期原核分裂组的受精率和早卵裂率分别为71.01%和8.99%,差异具有统计学意义(P<0.001)。早裂组的妊娠率(47.55%)高于晚裂组的妊娠率(38.30%),差异具有统计学意义(P<0.001)。种植率前者为29.72%,高于后者(22.99%),差异无统计学意义(P>0.05)。结论早期原核分裂有更好的妊娠结局,能够预测胚胎发育潜能,评价早期原核分裂是筛选高质量胚胎的一种简单有效、非侵袭性方法 。