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首页> 外文期刊>The Journal of Reproduction and Development >Analysis of the telomere shortening in the cloned caprine cultured cell line, CPF-1, derived from placenta of Shiba goat (Capra hircus)
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Analysis of the telomere shortening in the cloned caprine cultured cell line, CPF-1, derived from placenta of Shiba goat (Capra hircus)

机译:芝山羊胎盘克隆的山羊克隆培养细胞系CPF-1中端粒缩短的分析

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As a prerequisite for the production of cloned goats by nuclear transfer from the cultured somatic cells, we established cloned fibroblast cell lines, CPF-1 and other related CPF subclones from the placenta of the Shiba goat. CPF-1 cells ceased to proliferate at and about the 51st population doubling level (PDL) when the morphological signs of senescence, such as an unusual increase in cell volume, became obvious. The mean surface area of a cell at 51PDL was about 3 times greater than that of an early-passage cell (3PDL) (p<0.001). When the CPF-1 cells at 14PDL were subjected to chromosomal analysis, 49.3% of the cells turned out to be of normal diploid chromosomal constitution (2n=60). All the chromosomes were of acrocentric types. Part of the reason for the rather high incidence of aneuploidy might be due to the well-known technical difficulty in preparing good chromosomal spreads in the caprine cells. We analyzed the rates of telomere length shortening in the CPF-1 cells, according to the number of passages and culture periods. The telomere length in the late-passage cells became approximately 1/2.5 of that of the early-passage cells (p<0.05). The estimated mean rate of telomere shortening in the CPF-1 cells was approximately 260 bases per PDL and faster than the values (50-200 bases/PDL) so far reported in the literature for other types of cells. Furthermore, in the CPF-1 cells the replicative capacity was exhausted when the mean telomere length reached approximately 7.5 kb which is significantly longer than the values generally obtained in other cultured cell lines. The reasons for the observations have not yet been clarified.
机译:作为通过从培养的体细胞进行核转移生产克隆山羊的前提,我们从芝山羊的胎盘中建立了克隆的成纤维细胞系,CPF-1和其他相关的CPF亚克隆。当衰老的形态学迹象(例如细胞体积的异常增加)变得明显时,CPF-1细胞在第51个种群倍增水平(PDL)左右停止增殖。在51PDL处,细胞的平均表面积是早期传代细胞(3PDL)的约3倍(p <0.001)。当对14PDL处的CPF-1细胞进行染色体分析时,发现49.3%的细胞具有正常的二倍体染色体组成(2n = 60)。所有的染色体均为近端型。非整倍性的发生率很高的部分原因可能是由于在山羊细胞中制备良好的染色体铺展性的众所周知的技术困难。我们根据传代次数和培养时间分析了CPF-1细胞中端粒长度缩短的速率。晚期传代细胞的端粒长度约为早期传代细胞的端粒长度的1 / 2.5(p <0.05)。 CPF-1细胞中端粒缩短的估计平均速率约为每个PDL 260个碱基,并且比迄今为止文献中报道的其他类型细胞的值(50-200个碱基/ PDL)要快。此外,在CPF-1细胞中,当平均端粒长度达到约7.5 kb时,复制能力已耗尽,该长度明显长于在其他培养的细胞系中通常获得的值。观察的原因尚未阐明。

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