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Generation of parthenogenetic goat blastocysts: effects of different activation methods and culture media

机译:单性生殖山羊胚泡的产生:不同激活方法和培养基的影响

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摘要

The present study was carried out to investigate the effects of different activation methods and culture media on the in vitro development of parthenogenetic goat blastocysts. Calcium (Ca2+) ionophore, ethanol or a combination of the two, used as activating reagents, and embryo development medium (EDM), modified Charles Rosenkrans (mCR2a) medium and research vitro cleave (RVCL) medium were used to evaluate the developmental competence of goat blastocysts. Quantitative expression of apoptosis, stress and developmental competence-related genes were analysed in different stages of embryos. In RVCL medium, the cleavage rate of Ca2+ ionophore-treated oocytes (79.61 +/- 0.86) was significantly (P < 0.05) higher than in ethanol (74.90 +/- 1.51) or in the combination of both Ca2+ ionophore and ethanol. In mCR2a or EDM, hatched blastocyst production rate of Ca2+ ionophore-treated oocytes (8.33 +/- 1.44) was significantly higher than in ethanol (6.46 +/- 0.11) or in the combined treatment (6.70 +/- 0.24). In ethanol, the cleavage, blastocyst and hatched blastocyst production rates in RVCL medium (74.90 +/- 1.51, 18.30 +/- 1.52 and 8.24 +/- 0.15, respectively) were significantly higher than in EDM (67.81 +/- 3.21, 14.59 +/- 0.27 and 5.59 +/- 0.42) or mCR2a medium (65.09 +/- 1.57, 15.36 +/- 0.52 and 6.46 +/- 0.11). The expression of BAX, Oct-4 and GlUT1 transcripts increased gradually from 2-cell stage to blastocyst-stage embryos, whereas the transcript levels of Bcl-2 and MnSOD were significantly lower in blastocysts. In addition, different activation methods and culture media had little effect on the pattern of variation and relative abundance of the above genes in different stages of parthenogenetic activated goat embryos. In conclusion, Ca2+ ionophore as the activating agent, and RVCL as the culture medium are better than other tested options for development of parthenogenetic activated goat blastocysts.
机译:本研究旨在研究不同活化方法和培养基对孤雌生殖山羊胚泡体外发育的影响。钙(Ca2 +)离子载体,乙醇或两者的组合用作激活剂,并使用胚胎发育培养基(EDM),改良的Charles Rosenkrans(mCR2a)培养基和体外研究裂解(RVCL)培养基来评估卵白蛋白的发育能力。山羊胚泡。分析了胚胎不同阶段中凋亡,应激和发育能力相关基因的定量表达。在RVCL培养基中,Ca2 +离子载体处理过的卵母细胞的裂解速率(79.61 +/- 0.86)显着(P <0.05)高于乙醇(74.90 +/- 1.51)或Ca2 +离子载体和乙醇的组合。在mCR2a或EDM中,Ca2 +离子载体处理过的卵母细胞的孵化胚泡生产率(8.33 +/- 1.44)显着高于乙醇(6.46 +/- 0.11)或联合处理(6.70 +/- 0.24)。在乙醇中,RVCL培养基中的卵裂,囊胚和孵出的囊胚生产率(分别为74.90 +/- 1.51、18.30 +/- 1.52和8.24 +/- 0.15)显着高于EDM(67.81 +/- 3.21、14.59) +/- 0.27和5.59 +/- 0.42)或mCR2a培养基(65.09 +/- 1.57、15.36 +/- 0.52和6.46 +/- 0.11)。 BAX,Oct-4和GlUT1转录物的表达从2细胞期到胚泡期胚胎逐渐增加,而胚泡中Bcl-2和MnSOD的转录水平显着降低。此外,不同的活化方法和培养基对孤雌生殖活化山羊胚胎不同阶段中上述基因的变异模式和相对丰度影响很小。总之,Ca2 +离子载体作为活化剂,RVCL作为培养基比单性生殖活化山羊胚泡发育的其他测试方法更好。

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