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Selection of appropriate isolation method based on morphology of blastocyst for efficient derivation of buffalo embryonic stem cells

机译:基于胚泡形态的合适分离方法的选择,以有效衍生水牛胚胎干细胞

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The efficiency of embryonic stem cell (ESC) derivation from all species except for rodents and primates is very low. There are however, multiple interests in obtaining pluripotent cells from these animals with main expectations in the fields of transgenesis, cloning, regenerative medicine and tissue engineering. Researches are being carried out in laboratories throughout the world to increase the efficiency of ESC isolation for their downstream applications. Thus, the present study was undertaken to study the effect of different isolation methods based on the morphology of blastocyst for efficient derivation of buffalo ESCs. Embryos were produced in vitro through the procedures of maturation, fertilization and culture. Hatched blastocysts or isolated inner cell masses (ICMs) were seeded on mitomycin-C inactivated buffalo fetal fibroblast monolayer for the development of ESC colonies. The ESCs were analyzed for alkaline phosphatase activity, expression of pluripotency markers and karyotypic stability. Primary ESC colonies were obtained after 2–5?days of seeding hatched blastocysts or isolated ICMs on mitomycin-C inactivated feeder layer. Mechanically isolated ICMs attached and formed primary cell colonies more efficiently than ICMs isolated enzymatically. For derivation of ESCs from poorly defined ICMs intact hatched blastocyst culture was the most successful method. Results of this study implied that although ESCs can be obtained using all three methods used in this study, efficiency varies depending upon the morphology of blastocyst and isolation method used. So, appropriate isolation method must be selected depending on the quality of blastocyst for efficient derivation of ESCs.
机译:除啮齿动物和灵长类动物外,所有物种的胚胎干细胞(ESC)衍生效率都非常低。然而,在转基因,克隆,再生医学和组织工程领域中,主要期望从这些动物获得多能细胞有多种兴趣。世界各地的实验室都在进行研究,以提高其下游应用中ESC隔离的效率。因此,本研究旨在基于囊胚形态研究不同分离方法对水牛胚胎干细胞有效衍生的影响。胚胎通过成熟,受精和培养的过程在体外产生。将孵化的胚泡或分离的内部细胞团(ICM)接种在丝裂霉素C灭活的水牛胎成纤维细胞单层上,以培养ESC菌落。分析了ESC的碱性磷酸酶活性,多能性标志物的表达和核型稳定性。在丝裂霉素C灭活的饲养层上播种孵化的胚泡或分离的ICM后2-5天获得了主要的ESC集落。机械分离的ICM比通过酶分离的ICM更有效地附着并形成原代细胞集落。对于从定义不明确的ICM衍生出ESC,完整的孵化胚泡培养是最成功的方法。这项研究的结果暗示,尽管可以使用本研究中使用的所有三种方法获得ESC,但效率取决于囊胚的形态和所用的分离方法而有所不同。因此,必须根据胚泡的质量选择适当的分离方法,以有效地获得ESC。

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