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Establishment and characterization of a fibroblast cell line from the Mongolian horse

机译:蒙古马成纤维细胞系的建立和鉴定

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A fibroblast line was successfully established from Mongolian horse ear marginal tissue by using a primary explant technique and cell cryogenic preservation technology. Biological analysis showed the following: The cells were adherent and exhibited density-dependent inhibition of proliferation; assays of microbial contamination from bacteria, fungi, and mycoplasma were negative; the population doubling time of the cells was 33.9 h; and a 2n chromosome number of 64 at a frequency higher than 80%. A lack of cross-contamination of this cell line with other species was confirmed by isoenzyme analysis of lactic and malic dehydrogenases. In order to study exogenous gene expression, four fluorescent proteins, pEGFP-N3, pEGFP-C1, pDsRed1-N1, and pEYFP-N1, were transfected into the cells. The corresponding fluorescence was distributed throughout the cytoplasm and nucleus 12 h after transfection. This cell line not only preserves the genetic resources of the Mongolian horse at the cellular level but also provides valuable materials for genomic, postgenomic, and somacloning research in this species.
机译:通过使用初级外植体技术和细胞低温保存技术,从蒙古马耳边缘组织成功建立了成纤维细胞系。生物学分析表明:细胞粘附并表现出密度依赖性的增殖抑制;细菌,真菌和支原体对微生物的污染测定为阴性;细胞的群体倍增时间为33.9小时。 2n染色体数目为64,频率高于80%。通过乳酸和苹果酸脱氢酶的同工酶分析证实了该细胞系与其他物种的交叉污染。为了研究外源基因表达,将四种荧光蛋白pEGFP-N3,pEGFP-C1,pDsRed1-N1和pEYFP-N1转染到细胞中。转染后12小时,相应的荧光分布在整个细胞质和细胞核中。该细胞系不仅在细胞水平上保留了蒙古马的遗传资源,而且为该物种的基因组,后基因组和体细胞克隆研究提供了有价值的材料。

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