Evaluation of an internal control in a multiplex-PCR assay for sex determination of <i>in vitro</i>-produced bovine embryos

The use of an internal control in a multiplex-PCR assay for sex determination of In Vitro-produced bovine embryos was evaluated in biopsies of groups of 54 fresh and 44 frozen embryos. The internal controls used were the primers BOV 1 and BOV 2, which amplify a product with 626 base pairs (bp) of bovine mitochondrial DNA ND5 gene. The primers BRY.4aF and BRY.4aR were used for bovine Y chromosome sequence amplification. The specificity of multiplex- PCR reactions realized in biopsies corresponding to about 20% of each fresh embryo (10 male and 10 female) by means of confirming the sexing in the remaining embryo content (~80%) presented 100% specificity. Amplicons of the internal control and Y chromosome were both amplified until dilution corresponding to 6.25% of total extracted DNA from a male embryo. Sex determination was possible in 53 (98.1%) fresh embryos and 40 (90.9%) frozen embryos. The products related to the Y chromosome and mitochondrial DNA were simultaneously amplified in 34 (63%) fresh embryos and 27 (61.4%) frozen embryos, showing a male embryo. The female sex, distinguished by internal control amplification only, was detected in 19 (35.2%) and 13 (29.5%) biopsies, respectively, of fresh and frozen embryos. In one (1.8%) and four (9.1%) biopsies of fresh and frozen embryos, respectively, neither product was amplified, most likely due to the absence of embryonic cells or the presence of embryonic cells going through apoptosis. The multiplex-PCR assay developed in this work showed avoided the limitation of a lack of an internal standard, and was also sensitive, specific, and efficient in reaction failure identification. This technique shows great potential for use on a commercial scale in routine sex determination of In Vitro-produced embryos.

不同超数排卵方案与供体牛月龄对高产荷斯坦奶牛体外性控胚胎生产效率的影响

旨在探讨激素处理方案、供体牛月龄对高产荷斯坦奶牛超数排卵效果和性控体外胚胎生产效率的影响,为建立稳定高效且适用于高产荷斯坦奶牛的超数排卵方案以及提高高产奶牛性控胚胎体外生产效率提供技术支持。实验共选取高产荷斯坦奶牛60头,随机分为3组,分别按照注射FSH两周采卵一次(bi-weekly,BW)、注射FSH一周采卵一次(once weekly,OW)与不注射激素(control,CON)进行OPUIVF体外性控胚胎生产,应用以上最佳方案进一步研究青年牛与经产牛在体外胚胎生产效率上是否存在差异。BW组的超排效果要优于OW组与CON组,BW组头均可用卵数(15.30±0.60)、可用卵占比(68.83%±1.92%)、头均A级卵数(9.86±0.38)与头均B级卵数(5.44±0.37)均显著高于OW组;BW组IVF早期胚胎体外发育优于OW组与CON组,其中BW组卵裂率(77.80%±1.08%)与头均胚胎数(5.11±0.27)均高于OW组与CON组且差异显著,BW组和CON组B级胚胎占比(13.95%±1.23%)均显著低于OW组;经产牛组头均卵子数(27.10±1.35)与头均胚胎数(5.29±0.28)均显著高于青年牛组,但卵子可用率经产牛组显著低于青年牛组,分别为64.44%±1.81%和75.01%±2.33%。BW组可获得最佳的超排效果,应用BW超排方案发现经产牛的体外胚胎生产效率优于青年牛。

羊胚胎生物技术研究进展及应用

阐述了胚胎移植、胚胎冷冻、胚胎分割、胚胎性别控制及体外受精等胚胎生物技术在养羊业的研究进展及应用现状。

家畜繁育生物技术研究开发与产业化推广应用

家畜繁育生物技术包括人工授精、胚胎移植、体外受精、动物性别控制、动物克隆、转基因动物、干细胞等多元化的生殖生物工程技术。繁育生物技术的早期研究开发阶段主要集中在20世纪,到产业化推广应用经历了大约一个世纪的历程。目前,包括动物细胞性别控制、转基因-克隆技和干细胞技术已经进入产业化应用阶段,并且在人类疾病治疗方面显示了潜在的应用前景。

家畜繁殖生物技术研究现状及趋势

牛胚胎移植技术已趋于成熟。我国新疆牧科院用一步细管法移植牛冻胚受胎率达41%;牛和羊鲜胚四分胚移植也产下1头犊牛和6只羔羊。家畜体外受精,因卵子体外成熟和受精卵体外培养尚不过关,目前仍停留在实验室阶段。胚胎性别鉴定,1990年Koopman发现单拷贝基因,该基因是Y染色体的性决定区,命名为SRY,可利用PCR技术制成雄性特异DNA探针盒,进行马、牛、羊、猪早期胚胎性别鉴定。北京农学院等单位用PCR扩增牛SRY序列进行奶牛胚胎性别鉴定准确率达100%。英、日、法等国已获得牛胚胎细胞核移植后代;我国也获得1只核移植兔。北农大和新疆牧科院合作以绵羊精子为载体导入牛生长激素基因rMTbGH DNA成功,外源基因整合率为3%。

奶牛体外受精胚胎的性别控制研究

为加速母牛胚胎的生产,实现性控制胚胎产业化和体外扩繁优质品种的奶业工程发展,本研究在体外受精技术(invitro fertilization,IVF)不断成熟和完善的基础上,通过对牛非性控IVF胚胎与常规人工受精体内胚胎移植的妊娠成功率及其两者出生后牛的性别比例进行比较分析,结果发现,两组妊娠成功率基本相同,且IVF胚胎出生的公牛比例高于体内胚;采用性控和非性控精液进行IVF试验,并对非性控IVF胚胎及性控IVF胚胎用牛Y染色体性别决定特异基因(SRY)核心序列进行分子生物学性别鉴定,结果显示,性控IVF胚胎的公牛比例显著低于普通IVF胚胎;此外,作者还比较了性控IVF与普通非性控IVF的囊胚发育率,结果显示两者并无显著差异。以上研究结果证明,体外扩繁优质良种母牛的奶业工程必须依靠性别控制体外授精技术来提高其效率和有效性。