牛卵泡卵母细胞体外受精和发育的研究

利用屠宰黄牛卵巢作为供试材料 ,对卵巢表面 2～8mm卵泡卵母细胞体外受精(IVF) -受精卵的体外发育 (IVD)进行了系列研究 ,采用上游法、Percoll法和本实验室沿用的直接洗涤法处理牛冻精 ,观察 3种精子处理方法处理牛冷冻精子对卵母细胞体外受精胚胎发育的影响。实验结果 ,就卵裂率指标 ,采用Percoll法处理的精子进行卵母细胞体外受精 ,和上游法及洗涤法分别比较 ,差异均不显著 (P >0 .0 5 ) ;桑囊率指标 ,只有上游法比洗涤法高 ,差异显著 (P <0 .0 5 ) ,其余差异均不显著。以FERT -TALP液作为受精液采用常规培养方法 ,精卵作用 18～ 2 0h后分开 ,与精卵作用 6～ 8h后分开卵母细胞受精后的 8-细胞发育率及桑囊率变化不大 (P >0 .0 5 ) ;卵裂率指标 ,18～ 2 0h处理组高于 6～ 8h处理组 ,但两组之间差异也不显著。表明 ,在生产中采用FERT -TALP液做为受精液 ,应用上游法处理精子 ,不需要另购试剂 ,精卵孵育时间由 18～ 2 4h缩短至 6～ 8h是可行的 ,其现实意义是可以简化胚胎体外生产的程序 ,节省人力 ,降低成本     

猪卵子体外受精方法研究

本试验分析研究了：（1）猪卵子体外成熟所需要的培养时间；（2）促性腺激素和猪卵泡液对猪卵子体外成熟的作用；（3）不同体外受精次数对猪卵子体受精率的影响；（4）不同精子获能辅助剂对猪精子体外获能的作用；（5）不同种类猪精液的体外受精能力。研究结果表明，猪卵子体外成熟所需培养时间是32－36小时，在体外成熟培养液中加入0.25IU/ml PMSG（或FSH）和10％猪卵泡液可以促进猪卵子体外成熟，在精子体外获能培养液中加入0.05mg/ml肝素，在体外受精培养液中加入2mg/ml咖啡因可以促进猪精子体外获能并可提高体外受精率，体外成熟后的猪卵子进行2次受精可以获得较高的体外受精率，本试验用新鲜射出精子，冷冻射出精子，新附睾精子，冷冻附睾精子对体外成熟猪卵子进行体外受精，受精后卵裂率（2－4细胞期）分别是24.26％、23.40%,22.65%和24.24%。     

猪精子及卵子质量对猪体外受精胚胎发育的影响

应用体外受精(in vitro fertilization, IVF)等生物技术可以缩短种猪培育时间,地方猪精液的冷冻保存可以解决保存和运输问题。通过对不同个体冷冻前后的精子质量、获能方式、卵子质量及多精受精率对IVF的影响进行了研究。结果显示:当精子活率从83.26%降至74.20%时,IVF的卵裂率、桑椹胚率显著下降(P0.05)。不同的获能方式对IVF胚胎的卵裂率无显著影响(P0.05)。3层(及以上)卵丘细胞的卵子IVF的卵裂率、桑椹率显著高于3层以下组(P0.05)。冷冻精子的IVF中,2-细胞、4-细胞和囊胚的发育能力显著低于新鲜精子(P0.05),受精后6～12 h的多精受精率也显著高于新鲜精子组(P0.05)。猪体外受精胚胎的发育能力受精子和卵母细胞的影响。无论使用新鲜精液还是冷冻精液的IVF胚胎,在桑椹胚期后的发育能力都会受到阻碍,多精受精可能是原因之一,但具体原因还需要更多的研究。     

受精液和受精时间对牦牛卵泡卵母细胞体外受精的影响

利用屠宰牦牛卵巢，抽取其表面2～5mm的卵泡内卵母细胞，经体外成熟后分别用BO液和改良Tyrode’S液进行体外受精研究。结果表明，BO液受精6h和改良Tyrode’s液分别受精6h和18h，牦牛体外受精卵的卵裂率差异不显著（分别为52．48％、47．67％和50．00%,P〉0．05）。它们的4细胞发育率分别为75．47％、78．05％和64．10％，8细胞发育率分别为56．60％、56．10％和48．72％，使用改良Tyrode’s液受精18h的发育率最低，与其他2组相比，差异极显著（P〈0．01）；而受精时间同为6h时，2种受精液之间发育率的差异不显著（P〉0．05）。     

获能液及精子密度对牛性控精子体外受精成功率的影响

本实验探讨了不同的精子获能添加物、精子密度、精子获能液对牛性别分离精子体外受精（IVF）的影响。结果表明：受精液中同时添加10μg/mL的肝素与5mmol／L的咖啡因,能促进牛性控精子体外获能与受精。精子密度在1．0×10^6个/mL时其囊胚发育率最高。用BO液和mTyrode’s液对牛性控精子进行获能和受精处理．其受精效果差异不显著（P〉0．05）,但BO液作用时间短对早期胚胎的发育影响较小,比较适合牛性控精子IVF。     

影响猪卵母细胞体外受精效率因素的研究

通过比较参与受精的卵母细胞颗粒细胞存在与否、精子上浮时间、精卵共孵育时间、不同受精液等4个方面的因素,研究这些因素对猪卵母细胞体外受精后胚胎发育能力的影响,以求找到最佳的猪卵母细胞体外受精体系。将选择带有不同颗粒细胞的卵丘卵母细胞复合体分为3组：含全部颗粒细胞、2~3层颗粒细胞和裸卵;调整精子在受精液里的上浮时间为0、30、60、120min研究其受精能力;比较3、6、20h精卵共孵育时间对体外受精的影响;结果表明：在本试验体系下,在mTBM受精液中,将精子上浮处理60min,与含2~3层颗粒细胞的卵丘-卵母细胞复合体共孵育6h的IVF体系最为有效,其卵裂率为（77.6±2.3）%,囊胚率为（25.7±2.6）%。     

昆明小鼠与西门塔尔牛异种体外受精初步研究

卵母细胞胞质能否支持异种动物体外受精及受精卵能否发育可为揭示受精本质提供理论参考。为研究异种动物体外受精影响因素，本实验利用昆明小鼠卵母细胞为受体，进行西门塔尔牛冷冻精子体外受精，并从受精液组成、受精条件和有无透明带3个方面考察雄原核的形成及受精卵发育情况。结果显示：在西门塔尔牛冷冻精子的受精液和受精条件下，雄原核形成率高于小鼠试验组（11.7%vs2%）(P<0.05)；且在无透明带条件下，其雄原核的形成率（17.8%vs 12.79%）和卵裂率（27.27%vs 5.2%）均高于有透明带组（P<0.05）。以上结果初步表明，模拟精子源体外受精所需的“原生境”条件可提高异种动物体外受精的成功率。     

牛体外受精的精子处理方法对受精率和胚胎发育的影响

从屠宰场获得牛的卵巢 ,成熟培养用 TCM1 99 犊牛血清 ;体外受精的精子获能处理 ,以 BO液作为基础液。 BO液 肝素钠为对照组 ,对照组中分别添加 Caffein、Theophelline和 Pentoxifylline3种黄嘌呤诱导体为试验组 ,每组分别处理相同的 3头种公牛冷冻精液。用醋酸 Orcein染色 1 h检查受精精况。结果表明 ,平均受精率试验组均高于对照组 ( P <0 .0 1 ) ;DAY8平均囊胚率 ,Caff、Theo、Pent组分别为 2 0 .4 %、1 9.3 %、2 1 .2 %。 3种黄嘌呤诱导体中以 Pentoxifylline的效果最好     

小鼠去透明带裸卵的体外受精及其胚胎发育

为了建立提高小鼠弱精子体外受精率的新方法 ,将小鼠宰杀在 2 0℃下搁置 14 h,然后取出附睾尾精子进行冷冻保存。用解冻后活力明显下降的精子 ,与去透明带裸卵进行体外受精。结果显示 ,与带有颗粒细胞卵的体外受精率(0 % )和透明带切开卵的体外受精率 (4%～ 31% )相比 ,去透明带卵的体外受精率增至 39%～ 6 8% (P<0 .0 1) ;体外受精所获的 2细胞胚 ,经培养有 74 %～ 10 0 %的胚胎发育至扩张囊胚 ;来自 BDF1雄性小鼠精子的 2细胞期体外受精胚 ,经体外培养至囊胚期后再移植 ,获得了正常新生小鼠。以上结果表明 ,去透明带裸卵与小鼠弱精子体外受精 ,可提高小鼠弱精子的利用率     

牦牛卵母细胞的体外成熟、种间受精与胚胎培养

探讨了卵母细胞体外成熟时间、卵母细胞质量、精子准备和受精卵培养体系对牦牛卵母细胞种间体外受精效果的影响。结果表明:牦牛卵母细胞随体外成熟培养时间延长,第一极体排出率增加,囊胚发育率以成熟培养24 h最高;A级卵母细胞种间受精后囊胚的发育率(48.77±3.76)%显著高于B级(32.05±5.24)%和C级(7.54±7.18)%(P<0.05);BO液洗涤离心处理的精子受精后卵裂率(82.53±6.54)%显著高于Percoll液分离精子受精后的卵裂率(67.39±4.50)%(P<0.05),而两者囊胚率差异不显著((42.32±4.13)%vs(35.59±5.62)%,P>0.05);荷斯坦奶牛精子浓度在1×106～5×106/mL范围与牦牛卵母细胞受精效果差异不显著。卵丘细胞、输卵管上皮细胞共培养和SOF液培养种间受精卵,其卵裂率差异不显著,但共培养组的桑葚胚、囊胚和孵化胚发育率均显著高于SOF液培养组。     

In Vitro Maturation and Fertilization of Buffalo Oocytes: Effects of Storage of Ovaries, IVM Temperatures, Storage of Processed Sperm and Fertilization Media

Studies were conducted to examine the possibility of preserving slaughterhouse‐derived buffalo ovaries at 4°C for 0 (control), 12 and 24 h to maintain the developmental competence of the oocytes (experiment 1), to assess the effect of incubation temperature during oocyte maturation on rates of in vitro maturation (IVM) and in vitro fertilization (IVF) of buffalo oocytes and embryo development (experiment 2), and to examine the effect of storage at 25°C for 0 (control), 4 and 8 h of frozen–thawed buffalo sperm and BO and H‐TALP as sperm processing and fertilization media on cleavage and embryo development in vitro of buffalo oocytes (experiment 3) in order to optimize the IVF technology in buffalo. Results suggested that storage of ovaries at 4°C for 12 or 24 h significantly (p < 0.05) reduced the developmental potential of oocytes. Incubation temperatures during the IVM influenced the fertilization rate but had no significant effect on maturation and subsequent embryo development. The incubation temperature of 38.5°C during IVM was found to be optimum for embryo production in vitro. Storage of frozen–thawed sperm at 25°C for 8 h significantly (p < 0.05) decreased its ability to cleave the oocytes. Sperm processed in BO medium had significantly (p < 0.05) higher ability to cleave the oocytes than the H‐TALP medium.     

Sperm preparation through Sephadex™ filtration improves in vitro fertilization rate of buffalo oocytes

Routinely, swim‐up method is used to separate high‐quality sperm; however, long processing time and close cell‐to‐cell contact during the centrifugation step are inevitable elements of oxidative stress to sperm. The objective was to evaluate Sephadex^? and glass wool filtration to separate motile, intact and viable sperm for in vitro fertilization in buffalo. The cumulus–oocyte complexes (COC s) were collected from ovaries of slaughtered buffaloes by aspiration and matured for 24 hr in CO ₂ incubator at 38.5°C and 5% CO ₂. Matured COC s were rinsed twice in fertilization TALP and placed in the pre‐warmed fertilization medium without sperm. Cryopreserved buffalo semen was thawed at 37°C for 30 s and processed through Sephadex^?, glass wool filtration and swim‐up (control). Total and motile sperm recovery rates were assessed, resuspended in fertilization TALP and incubated for 15–20 min in CO ₂ incubator. Samples prepared by each method were divided into two aliquots: one aliquot was studied for sperm quality (progressive motility, membrane integrity, viability, liveability), while the other was subjected to co‐incubation with sets of 10–15 in vitro matured oocytes. Data on sperm quality were analysed by ANOVA , while in vitro fertilizing rates were compared by chi‐squared test using SPSS ‐20. Least significant difference (LSD ) test was used to compare treatment means. Glass wool filtration yielded higher total and motile sperm recovery rate, while Sephadex^? filtration improved (p  <  .05) sperm quality (progressive motility, membrane integrity, viability, liveability). Sperm preparation through Sephadex filtration yielded higher in vitro fertilization rate in terms of cleavage rate compared to glass wool filtration and swim‐up (control). In conclusion, cryopreserved Nili‐Ravi buffalo sperm selected through Sephadex filtration showed improved quality and yielded better fertilization rates (cleavage rate) of in vitro matured/fertilized oocytes. Sephadex filtration could be a promising technique for use in in vitro fertilization in buffalo.     

牛卵母细胞体外成熟和体外受精技术的研究进展

论述牛卵母细胞体外成熟和体外受精的最新研究进展，包括卵丘卵母细胞复合体、卵母细胞的体内、体外成熟，以及体内、体外的异常成熟和卵母细胞的体外成熟方法，无蛋白质、无血清系统的限定性培养液的研究进展，卵母细胞体外成熟状态与标志的某些理论上的突破；体外受精中精子供体的选择、精子活力和正常形态的选择、冷冻解冻精液的体外获能、精子的体外受精力，以及体外的异常受精；还论述了牛卵母细胞体外成熟和体外受精技术在家畜育种和胚胎克隆等方面的应用前景     

In vitro fertilization and development of in vitro matured bovine follicular oocytes

Bovine follicular oocytes matured in vitro were fertilized in vitro using epididymal spermatozoa from five different bulls and then cultured to the blastocyst stage in vitro. The fertilization rate, based on one pair of pronuclei and presence of one sperm tail, ranged from 55.2 to 64.3%. Embryo development (cleavage to blastocyst stage) ranged from 21.4 to 31.0% of the cultured ova reaching 8 cells at 3 to 4 d after insemination to 1.3 to 3.7% reaching hatched blastocysts at 9 to 10 d. It is concluded that individual variation among bulls is not a significant factor in fertilization and development rates of bovine follicular oocytes when epididymal spermatozoa are used.     

Sperm‐TALP: An Alternative Extender for Retrieving and Diluting Epididymal Sperm in the Domestic Cat

Effects of sperm‐TALP (TALP) on the quality of fresh‐extended and frozen‐thawed epididymal cat sperm were evaluated. The epididymides suspended in Tris–glucose–citrate solution (Tris), a conventional medium, and TALP were cut into small pieces to recover epididymal sperm. In experiment 1, the sperm pellets remained after centrifugation were re‐suspended (1 : 2, v/v) in Tris and TALP. The sperm quality in all four groups, that is, sperm retrieved with Tris (I and II) or TALP (III and IV) and diluted with Tris (I and III) or TALP (II and IV) was assessed. The sperm motility at the 0‐h incubation in TALP–TALP was superior to that of the rest (p < 0.001 to p = 0.04). At the 2‐h incubation, the motility in Tris/TALP–TALP was greater than that in Tris/TALP–Tris (p ≤ 0.001). In experiment 2, after centrifugation, the sperm pellets were added with freezing extenders and frozen. The thawed sperm previously retrieved from the epididymides with Tris and TALP were allotted so as not to further diluted (Tris/TALP–O) and to further diluted (1 : 1, v/v) with Tris (Tris/TALP–Tris) and TALP (Tris/TALP–TALP) and were evaluated the quality. At both incubation times, the motility of frozen‐thawed sperm recovered with TALP (TALP–O/Tris/TALP) was comparable with or significantly higher than that in the Tris groups (Tris–O/Tris/TALP; p = 0.003 to p > 0.05). The motility and viability of thawed sperm in Tris–Tris were significantly decreased during the 2‐h incubation (p = 0.007 for the motility and p = 0.01 for the viability). In both experiments, neither type of diluent (Tris vs TALP) nor incubation time (0 vs 2 h) significantly affected the sperm membrane integrity under hypo‐osmotic condition (p > 0.05). According to beneficial effects on the quality of fresh‐extended and frozen‐thawed sperm demonstrated, sperm‐TALP could be used as an alternative medium for recovering sperm from the epididymides and for diluting epididymal sperm in the domestic cat.     

牛卵母细胞体外受精技术研究

本研究从3方面进行了牛卵母细胞的体外受精试验,即用不同离心法、不同温度上浮法、不同精子浓度等方法对COCs进行体外受精,测定其体外受精率。结果表明,两种离心法中,以上清液二次离心法的精子获能效果最好,受精率最高,该法首次采用低速离心技术,突破了离心法的传统方法,离心效果明显提高;不同温度条件下的精子上浮效果以CO2培养箱恒温（38.5℃）上浮法最好,受精率最高;对于选择受精时获能精子的浓度,宜控制在1.0×106～1.5×106个/ml,不仅能提高受精率,还可避免或降低多精受精现象。     

Capacitation of Frozen Thawed Buffalo Bull (Bubalus bubalis) Spermatozoa with Higher Heparin Concentrations

The present study was conducted to examine the effect of high heparin concentration on capacitation of buffalo spermatozoa with a short incubation time. Frozen thawed spermatozoa from three buffalo bulls were pooled and treated with either 50, 100 or 200 microg/ml heparin for 30 min. Capacitation was evaluated by acrosome reaction of spermatozoa and in vitro fertilization rate (per cent cleavage rate, per cent cleavage index). Acrosome reaction was induced in heparin treated spermatozoa with calcium ionophore A23187 and staining was carried out with Coomassie G-250 to evaluate the response as compared with control (0 heparin + calcium ionophore). Significantly higher percentage of acrosome reaction (AR) spermatozoa was noted after heparin treatment (36.8-48.2%) as compared with control (8.1% ; p < 0.05) but differences among the three heparin concentrations were non-significant. However, a significantly higher in vitro fertilization rate was recorded in spermatozoa capacitated by 50 and 100 microg/ml heparin (80.4 and 75.9% cleavage rate, respectively) as compared with 200 microg/ml heparin (47.2% cleavage rate; p < 0.001). It is concluded that buffalo spermatozoa capacitated with 50-100 microg/ml heparin had significantly higher ability to improve in vitro fertilization rate in buffalo.     

Effect of capacitation of stallion sperm with polyvinylalcohol or bovine serum albumin on penetration of bovine zona-free or partially zona-removed equine oocytes

Experiments were conducted to study effects of macromolecules on stallion sperm capacitation and fertilization as determined by penetration of bovine zona-free and equine partially zona-removed oocytes. Stallion sperm were capacitated in TYH medium (modified Krebs-Ringer bicarbonate) supplemented with either 1 mg/mL of polyvinylalcohol (PVA) or 4 mg/mL of BSA. Capacitation was induced with 8 bromoadenosine cyclic monophosphate (8BrcAMP; 0.5 mM) alone or in combination with 0.1 microM of ionomycin. Intraspecies gametes were co-incubated in TYH/PVA or TYH/BSA for 18 to 20 h. For zona-free bovine oocytes, penetration rate (35%) with the combination of 8BrcAMP and ionomycin in PVA-containing medium was higher (P < 0.05) than any treatment in BSA-containing medium (5 to 6%). A similar study was conducted using equine oocytes with partially removed zonae. Sperm capacitated and used for in vitro fertilization (IVF) in PVA-containing medium had higher penetration rates (P < 0.01) than sperm in BSA-containing medium (54 vs. 11%). The effect of equine preovulatory follicular fluid on bovine oocyte penetration was assessed. Bovine oocytes were matured in tissue culture medium-199 with 0, 20, 50, or 100% equine preovulatory follicular fluid, and 1 IU/mL of equine chorionic gonadotropin. Stallion sperm were treated with 8BrcAMP + ionomycin in PVA- or BSA-containing media. The penetration rates of bovine zona-free oocytes by stallion sperm were again higher with PVA (47%) than BSA (18%; P < 0.01). Penetration rates of oocytes matured in 100% follicular fluid were higher (P < 0.05) than for oocytes matured with 0% follicular fluid. The effects of equine follicular fluid and PVA/BSA during sperm capacitation on standard bovine IVF were examined. Culture of bovine oocytes with equine follicular fluid did not affect oocyte maturation or penetration rates after IVF. Bovine sperm capacitated with heparin in PVA-containing medium yielded lower (P < 0.05) fertilization rates than those capacitated in BSA-containing medium when incubated with both zona-intact and zona-free bovine oocytes. In summary, PVA was superior to BSA for ionophore-induced capacitation of equine sperm for penetration of zona-free bovine oocytes or partially zona-removed equine oocytes, but not for standard bovine IVF with bovine sperm. Zona-free bovine oocytes may be useful for assaying in vitro capacitation and fertilization of stallion sperm.     

不同培养液对蓝狐精子体外获能效果的比较试验

采用上游法分离优化精子,用mTyrod’s液(T)、BO液(B)以及高渗液(HIS)3种不同培养液,在5%CO2的培养箱中进行获能培养,获能培养时间为6h。利用考马斯亮蓝染色法检测精子顶体反应率,伊红-苯胺黑染色法检测活精子比率以及观测法检测精子活力。在培养的0、1、2、4、6h时分别检测上述指标并统计分析,从而筛选出适合蓝狐精子体外获能的培养液。结果显示:B培养液优于T、HIS培养液,最佳获能培养时间t≥6h;HIS可以提高精子顶体反应率,但较高的渗透压不利于精子保存,不建议使用。     

提高牛体外性控胚胎效率关键技术研究

为了提高牛体外受精效果,试验从性控冷冻精液体外获能方法及抗氧化剂的添加、体外成熟24h后卵母细胞是否部分脱除卵丘细胞3个方面,研究了影响牛性控精液体外受精效率的关键技术。结果表明,一次离心体外获能法体外受精卵裂率[(68.3±3.7)%]、囊胚率[(30.9±2.3)%]与精子上浮获能法体外受精卵裂率[(67.8±2.6)%]、囊胚率[(29.7±3.7)%]无显著差异(P>0.05),但显著高于二次离心体外获能法体外受精卵裂率[(56.1±4.1)%]、囊胚率[(21.6±4.6)%](P<0.05);获能液和体外受精液添加1.0%抗坏血酸组体外受精卵裂率[(70.2±3.2)%]、囊胚率[(35.0±4.7)%]显著高于不添加组体外受精卵裂率[(60.0±4.5)%]、囊胚率[(28.3±3.6)%](P<0.05);在体外受精前,成熟卵母细胞周围的卵丘细胞脱除情况为部分脱除组体外受精卵裂率[(70.1±4.6)%]、囊胚率[(35.5±3.7)%]显著高于不脱除组体外受精卵裂率[(52.9±4.1)%]、囊胚率[(26.1±3.6)%](P<0.05)。由此可见,性控精液体外受精时,获能方法宜采用一次离心体外获能法或上浮获能法,且精子获能液和体外受精液中宜添加抗坏血酸;体外受精前,成熟卵母细胞部分脱除卵丘细胞对于提高性控精液体外受精胚胎发育率具有重要意义。