The goal of this study was to establish and validate a protocol for preparing bovine cardiomyocytes from slaughterhouse material for nuclear transfer experiments. The cardiomyocyte was selected because it is a terminally differentiated cell and strongly expresses a unique subset of genes which can be monitored during the reprogramming period. A total of 39 trials were conducted, and an optimized protocol was developed yielding individual contractile cardiomyocytes from 3-5-month-old bovine fetuses The basic protocol involves stabilization of bovine heart tissue for transportation from the slaughterhouse to the laboratory by perfusion with Custodiol. This was followed by an enzymatic dissociation with collagenase in calcium-free medium and yielded individual contractile rod-shaped cardiomyocytes. Subsequent addition of Ca2+ caused the cardiomyocytes to round up which was an essential pre-condition for drawing them into glass transfer pipettes for delivery into the perivitelline space and for efficient electrofusion with cytoplasts derived from in vitro matured bovine oocytes. The use of cardiomyocytes maintained at 37 degrees C in nuclear transfer, resulted in a significantly reduced proportion of blastocysts compared to adult fibroblasts (14.0% versus 32.7%). Storage of cardiomyocytes at 4 degrees C prior to nuclear transfer was not compatible with blastocyst development. It is expected that this system will be valuable for investigating the reprogramming of gene expression which occurs after somatic cell nuclear transfer.

译文

这项研究的目的是建立和验证从屠宰场材料中制备牛心肌细胞以进行核移植实验的协议。选择心肌细胞是因为它是终末分化的细胞,并且强烈表达可以在重编程期间监测的独特基因子集。总共进行了39项试验,并开发了一种优化的方案,从3-5个月大的牛胎儿中产生了单个收缩心肌细胞。基本方案涉及稳定牛心脏组织,以便通过灌注从屠宰场运输到实验室。保管二醇。随后在无钙培养基中与胶原酶酶解离,并产生单个收缩的杆状心肌细胞。随后添加Ca2会导致心肌细胞四舍五入,这是将其吸入玻璃转移移液管以输送到卵黄周围空间以及与来自体外成熟牛卵母细胞的细胞质进行有效电融合的必要前提。与成人成纤维细胞相比,在核转移中使用维持在37 ℃ 的心肌细胞导致胚泡的比例显著降低 (14.0% 对32.7%)。在核转移之前在4摄氏度下储存心肌细胞与胚泡发育不相容。预计该系统对于研究体细胞核移植后发生的基因表达的重编程将很有价值。

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