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Recommended Method for Chromosome Exploitation: RMCE-based Cassette-exchange Systems in Animal Cell Biotechnology

机译:推荐的染色体开发方法:动物细胞生物技术中基于RMCE的盒式交换系统

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The availability of site-specific recombinases has revolutionized the rational construction of cell lines with predictable properties. Early efforts were directed to providing pre-characterized genomic loci with a single recombinase target site that served as an address for the integration of vectors carrying a compatible tag. Efficient procedures of this type had to await recombinases like ΦC31, which recombine attP and attB target sites in a one-way reaction — at least in the cellular environment of the higher eukaryotic cell. Still these procedures lead to the co-introduction of prokaryotic vector sequences that are known to cause epigenetic silencing. This review illuminates the actual status of the more advanced recombinase-mediated cassette exchange (RMCE) techniques that have been developed for the major members of site-specific recombinases (SR), Flp, Cre and ΦC31. In RMCE the genomic address consists of a set of heterospecific recombinase target (RT-) sites permitting the exchange of the intervening sequence for the gene of interest (GOI), as part of a similar cassette. This process locks the GOI in place and it is ‘clean’ in the sense that it does not co-introduce prokaryotic vector parts nor does it leave behind a selection marker.
机译:位点特异性重组酶的可用性彻底改变了具有可预测特性的细胞系的合理构建。早期的努力致力于为预先表征的基因组位点提供单个重组酶靶位点,该位点用作整合携带兼容标签的载体的地址。这种类型的高效程序必须等待重组酶(如ΦC31)重组,至少在高级真核细胞的细胞环境中,重组酶才能以单向反应重组atP和atB靶位点。这些程序仍然导致已知导致表观遗传沉默的原核载体序列的共同引入。这篇综述阐明了针对位点特异性重组酶(SR),Flp,Cre和ΦC31的主要成员开发的更高级的重组酶介导的盒式交换(RMCE)技术的实际状况。在RMCE中,基因组地址由一组异源重组酶靶(RT-)位点组成,允许将目的序列(GOI)的插入序列交换为相似盒的一部分。该过程将GOI锁定在适当的位置,并且从某种意义上讲它是“干净的”,因为它不会共同引入原核矢量部分,也不会留下选择标记。

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