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Method to Assemble Genomic DNA Fragments or Genes on Human Artificial Chromosome with Regulated Kinetochore Using a Multi-Integrase System

机译:用多整体酶系统将人造染色体上的基因组DNA片段或基因组装基因组DNA片段或基因的方法

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The production of cells capable of carrying multiple transgenes to Mb-size genomic loci has multiple applications in biomedicine and biotechnology. In order to achieve this goal, three key steps are required: (i) cloning of large genomic segments; (ii) insertion of multiple DNA blocks at a precise location and (iii) the capability to eliminate the assembled region from cells. In this study, we designed the iterative integration system (IIS) that utilizes recombinases Cre, Phi C31 and Phi BT1, and combined it with a human artificial chromosome (HAC) possessing a regulated kinetochore (alphoid(tetO)-HAC). We have demonstrated that the IIS-alphoid(tetO)-HAC system is a valuable genetic tool by reassembling a functional gene from multiple segments on the HAC. alphoid(tetO)-HAC has several notable advantages over other artificial chromosome-based systems. This includes the potential to assemble an unlimited number of genomic DNA segments; a DNA assembly process that leaves only a small insertion (&60 bp) scar between adjacent DNA, allowing genes reassembled from segments to be spliced correctly; a marker exchange system that also changes cell color, and counter-selection markers at each DNA insertion step, simplifying selection of correct clones; and presence of an error proofing mechanism to remove cells with misincorporated DNA segments, which improves the integrity of assembly. In addition, the alphoid(tetO)-HAC carrying a locus of interest is removable, offering the unique possibility to revert the cell line to its pretransformed state and compare the phenotypes of human cells with and without a functional copy of a gene(s). Thus, alphoid(tetO) allows investigation of complex biomedical pathways, gene(s) regulation, and has the potential to engineer synthetic chromosomes with a predetermined set of genes.
机译:能够将多个转基因携带到MB尺寸基因组基因座的细胞的产生在生物医学和生物技术中具有多种应用。为了实现这一目标,需要三个关键步骤:(i)大型基因组细分的克隆; (ii)在精确的位置和(iii)中插入多个DNA块,(iii)能够消除来自细胞的组装区域的能力。在这项研究中,我们设计了利用重组酶CRE,PHI C31和PHI BT1的迭代整合系统(IIS),并将其与具有受调节的KINETOCHORE的人工染色体(HAC)组合(血管(Teto)-Hac)。我们已经证明,IIS-alphoid(Teto)-HAC系统是一种有价值的遗传工具,通过从HAC上的多个区段重新组装功能基因。字母(Teto)-HAC具有与其他基于染色体的系统的几个显着的优势。这包括组装无限数量的基因组DNA段的可能性; DNA组装过程仅在相邻DNA之间仅留下小的插入(& 60bp)瘢痕,允许从段正确剪接的基因重新组装;一个标记交换系统,也改变每个DNA插入步骤的细胞颜色和反选择标记,简化了正确的克隆的选择;并且存在误报机制以除去具有混合性DNA段的细胞,这提高了组装的完整性。此外,携带感兴趣轨迹的字母(Teto)-HAC是可拆卸的,提供了将细胞系重新转化为其预形状态的独特可能性,并将人体细胞的表型与基因的功能拷贝进行比较。因此,字母单(Teto)允许研究复杂的生物医学途径,基因(S)调节,并且具有工程师与预定一组基因的合成染色体。

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