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Long-term stability of large insert genomic DNA episomal shuttle vectors in human cells.

机译:大插入基因组DNA游离穿梭载体在人类细胞中的长期稳定性。

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摘要

We have constructed an episomal shuttle vector which can transfer large (>100 kb) human genomic DNA inserts back and forth between bacteria and human cells and which can be tracked in rapidly dividing human cells using a live cell assay. The vector (p5170) is based on the F factor-derived bacterial artificial chromosome cloning vector used in Escherichia coli, with the addition of the family of repeats element from the Epstein-Barr virus (EBV) latent origin of replication. This element provides nuclear retention in cells expressing the EBV protein EBNA-1. We have subcloned a series of genomic DNA inserts into p5170 and transfected the constructs into an EBNA-1(+) human cell line. Episomal mitotic stability was quantitatively analysed using flow cytometry. The episomes were also tracked by time course photography of expanding colonies. A 117 kb episome was retained at approximately 2 copies/cell and could be shuttled unrearranged from the human cells into bacterial cells after 15 months of continuous cell growth. Furthermore, the episome could still be rescued from human cells cultured in the absence of selection for 198 days. Such a trackable E.coli /human cell line shuttle vector system capable of carrying >100 kb of genomic DNA in human cells could prove a valuable tool in gene expression studies.
机译:我们已经构建了一种游离型穿梭载体,该载体可以在细菌和人类细胞之间来回转移大的(> 100 kb)人类基因组DNA插入片段,并且可以使用活细胞测定法在快速分裂的人类细胞中进行追踪。载体(p5170)基于大肠杆菌中使用的F因子衍生的细菌人工染色体克隆载体,并添加了来自爱泼斯坦-巴尔病毒(EBV)潜在复制起点的重复序列家族。该元素在表达EBV蛋白EBNA-1的细胞中提供核保留。我们已经将一系列基因组DNA插入片段亚克隆到p5170中,并将该构建体转染到EBNA-1(+)人类细胞系中。使用流式细胞仪定量分析了游离染色体的有丝分裂稳定性。还通过扩展菌落的时程摄影来追踪附加体。 117 kb的附加体保留在大约2个拷贝/细胞中,并且在连续细胞生长15个月后可以不重排地从人细胞穿入细菌细胞。此外,附加体仍可从无选择条件下培养198天的人类细胞中拯救出来。这种可在人细胞中携带> 100 kb基因组DNA的可追踪大肠杆菌/人细胞系穿梭载体系统可证明是基因表达研究中的宝贵工具。

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