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首页> 外文期刊>Theriogenology >In vitro-produced equine embryos: production of foals after transfer, assessment by differential staining and effect of medium calcium concentrations during culture
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In vitro-produced equine embryos: production of foals after transfer, assessment by differential staining and effect of medium calcium concentrations during culture

机译:体外产生的马胚:转移后产生小马驹,通过差异染色进行评估,并在培养过程中测定中等钙浓度

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Viability of equine embryos produced by oocyte maturation, intracytoplasmic sperm injection and embryo culture to the blastocyst stage in vitro was evaluated after transfer of embryos to recipient mares. No pregnancies were produced after transfer of five blastocysts that had been cultured in G media. Transfer of 10 blastocysts cultured in modified DMEM/F-12 medium produced five pregnancies and three live foals; the two lost pregnancies developed only trophoblast (based on transrectal ultrasonography). To evaluate the status of the inner cell mass, equine blastocysts produced in vivo and in vitro were assessed after differential staining. A discrete inner cell mass could not be appreciated in blastocysts of either source after staining; this was attributed to the presence of a network of cells within the trophoblastic vesicle. Because increased medium calcium concentrations have been reported to decrease the incidence of trophoblast-only pregnancy after transfer of equine nuclear transfer embryos, we investigated the effect of increased calcium concentrations during oocyte maturation or during embryo culture. Increasing calcium concentration of culture medium from 2 to 5.6mM during in vitro oocyte maturation did not affect maturation rate (75 and 68%, respectively) or blastocyst development after fertilization (23 and 27%). However, increasing calcium concentration (from 1.3 to 4.9 mM) of medium used for embryo culture significantly decreased blastocyst development (27% versus 13%, respectively) and adversely affected embryo morphology. More work is needed to optimize culture systems for in vitro production of equine embryos.
机译:在将胚胎转移到受体母体后,评估了通过卵母细胞成熟,胞浆内精子注射和胚胎培养到胚泡期产生的马胚的生存能力。在G培养基中培养的五个胚泡转移后,没有怀孕。在改良的DMEM / F-12培养基中培养的10个胚泡的转移产生了5个怀孕和3个活驹。两次怀孕的孕妇仅滋养细胞(基于经直肠超声检查)。为了评估内部细胞团的状态,在差异染色后评估了体内和体外产生的马胚泡。染色后,在任一来源的胚泡中都看不到离散的内部细胞团;这归因于滋养细胞囊泡中细胞网络的存在。由于据报道增加的中等钙浓度可降低马核移植胚胎移植后仅滋养细胞妊娠的发生率,因此我们研究了卵母细胞成熟或胚胎培养过程中钙浓度升高的影响。在体外卵母细胞成熟过程中,将培养基中的钙浓度从2mM增加到5.6mM不会影响成熟率(分别为75%和68%)或受精后胚泡发育(23%和27%)。但是,用于胚胎培养的培养基中钙浓度的增加(从1.3到4.9 mM)显着降低了胚泡发育(分别为27%和13%),并对胚胎形态产生了不利影响。需要更多的工作来优化用于体外生产马胚胎的培养系统。

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